OIV-MA-BS-01 Reference method for the determination of alcoholic strength by volume of spirit drinks of viti-vinicultural origin: General remarks

Type II method

Introduction

 

The reference method includes two Annexes:

Annex I - Preparation of distillate

Annex II - Measurement of density of distillate by three methods A, B, and C

1. Scope

The method is suitable for the determination of the real alcoholic strength by volume of spirit drinks of viti-vinicultural origin.

2. Normative References

ISO 3696:1987 Water for analytical laboratory use - Specifications and test methods.

3. Terms and Definitions
   1.      Reference temperature:

The reference temperature for the determination of alcoholic strength by volume, density and specific gravity of spirit drinks is 20 °C.

Note 1: The term 'at t °C' is reserved for all determinations (of density or alcoholic strength by volume) expressed at a temperature other than the reference temperature of 20 °C.

3.2.     Density:

The density is the mass per unit volume in vacuo of spirit drinks at 20 °C. It is expressed in kilograms per cubic metre and its symbol is ρ_{20 °C} or ρ₂

 

3.3.     Apparent alcoholic strength:

The apparent alcoholic strength of alcohols and spirituous beverages is equal to the number of litres of ethyl alcohol contained in 100 litres of an aqueous-alcoholic mixture with the same density as that of the alcohol or spirituous beverage. Therefore, the apparent alcoholic strength is directly deduced from the density of the product, without distillation. The apparent alcoholic strength is expressed in % vol.

3.4.     Specific gravity:

The specific gravity is the ratio, expressed as a decimal number, of the density of spirit drinks at 20 °C to the density of water at the same temperature. It is denoted by the symbol d_{20 °C/20 °C} or d_20/20, or simply d when there is no possibility of confusion. The characteristic that was measured must be specified on the assay certificate using the above-defined symbols only.

Note 2: It is possible to obtain the specific gravity from the density ρ₂₀ at 20 °C:

ρ₂₀ = 998.203 x d_20/20 or d_20/20 = ρ₂₀ /998.203 where 998.203 is the density of water at 20 °C.

3.5.     Real alcoholic strength by volume:

The real alcoholic strength by volume, or alcohol by volume (ABV), of spirit drinks is equal to the number of litres of ethyl alcohol contained in 100 l of a water-alcohol mixture having the same density as the alcohol or spirit after distillation. The reference values for alcoholic strength by volume (% vol.) at 20 °C versus density at 20 °C for different water-alcohol mixtures that are to be used are those given in the international table adopted by the International Legal Metrology Organisation in its Recommendation no. 22.

Note 3:  For liqueurs and crèmes for which it is very difficult to measure

volume accurately the sample must be weighed and the alcoholic strength is calculated first by mass.

Conversion formula:

Alcoholic strength by volume (%vol)=

where ASM = alcoholic strength by mass,

ρ₂₀ (alcohol) = 789.24 kg/m³

 

3.6.     Density – Alcoholic Strength Correspondence

The reference values for the alcoholic strength (% vol.) at 20 °C, defined in 3.3 and 3.5, versus density at 20 °C for different aqueous-alcoholic mixtures that are to be used are those given in the international table adopted by the International Organization of Legal Metrology in its recommendation N° 22.

3.7.     Obscuration:

Obscuration is defined as the difference between the real alcoholic strength by volume and the apparent alcoholic strength, expressed in % vol.

4. Principle

Following distillation the alcoholic strength by volume of the distillate is determined by pycnometry, electronic densimetry, or densimetry using a hydrostatic balance.

5. Bibliography

• Commission Regulation (EC) N° 2870/2000 of 19 December 2000 laying down Community reference methods for the analysis of spirits drinks, OJEC of 29 December 2000, L333/20
• P. Brereton, S. Hasnip, A. Bertrand, R. Wittkowski, C. Guillou, Analytical methods for the determination of spirit drinks, Trends in Analytical Chemistry, Vol. 22, No. 1, 19-25, 2003

OIV-MA-BS-02 Reference method for the determination of alcoholic strength by volume of spirit drinks of viti-vinicultural origin: Preparation of the distillate

Type II method

1. Scope

The method is suitable for the preparation of distillates to be used to determine the real alcoholic strength by volume of spirit drinks.

2. Principle

The spirits are distilled to separate the ethyl alcohol and other volatile compounds from the extractive matter (substances which do not distil).

 

3. Reagents and Materials
   1. Anti-bumping granules
   2. Concentrated antifoam emulsion (for crème liqueurs)

4. Apparatus and Equipment

Usual laboratory apparatus and in particular the following.

4.1. Water bath capable of being maintained at 10 °C to 15 °C.

Water bath capable of being maintained at 20 ºC ( 0.2 ºC)

4.2. Class A volumetric flasks, 100 ml and 200 ml, that have been certified to 0.1 % and 0.15 % respectively.

4.3. Distillation apparatus:

4.3.1.    General requirements

The distillation apparatus must meet the following specifications:

• The number of joints must be no more than the strict minimum needed to ensure the system is leak-tight.
• Inclusion of a device designed to prevent priming (entrainment of the boiling liquid by the vapour) and to regularise the distillation rate of alcohol-rich vapours.
• Rapid and complete condensation of the alcohol vapours.
• Collection of the first distillation fractions in an aqueous medium.

The heat source must be used with a suitable heat-diffuser to prevent any pyrogenic reaction involving the extractive matter.

4.3.2.    As an example, a suitable distillation apparatus would include the following parts:

• Round bottomed flask, 1 litre, with a standardised ground-glass joint.
• Rectifying column at least 20 cm high (a Vigreux column, for example).
• Elbow connector with an approximately 10 cm long straight-rimmed condenser (a West-type condenser) fitted vertically.
• Cooling coil, 40 cm long.
• Drawn out tube, taking the distillate to the bottom of a graduated collecting flask containing a small amount of water.

Note:  The apparatus described above is intended for a sample of least 200 ml. However, a smaller sample size (100 ml) can be distilled by using a smaller distillation flask, provided a splash-head or some other device to prevent entrainment is used.

5. Storage of test samples

 

Samples are stored at room temperature prior to analysis.

6. Procedure

6.1. Distillation apparatus verification

The apparatus used must be capable of the following:

The distillation of 200 ml of a water-alcohol solution with known concentration close to 50 % vol. must not cause a loss of alcohol of more than 0.1 % vol.

6.2. Spirit drinks with alcoholic strength below 50 % vol.

Measure out 200 ml of the spirit into a volumetric flask.

Record the temperature of this liquid, or maintain at standard temperature (20 ºC).

Pour the sample into the round bottomed flask of the distillation apparatus and rinse the volumetric flask with three aliquots each of approximately 20 ml of distilled water. Add each rinse water aliquot to the contents of the distillation flask.

Note: This 60-ml dilution is sufficient for spirits containing less than 250 g of dry extract per litre. Otherwise, to prevent pyrolysis, the volume of rinse water must be at least 70 ml if the dry extract concentration is 300 g/l, 85 ml for 400 g/l dry extract, and 100 ml for 500 g/l dry extract (some fruit liqueurs or crèmes). Adjust these volumes proportionally for different sample volumes.

Add a few anti-bumping granules (3.1) (and antifoam for crème liqueurs).

Pour 20 ml of distilled water into the original 200 ml volumetric flask that will be used to hold the distillate. This flask must then be placed in a cold water bath (4.1) (10 - 15 °C for aniseed-flavoured spirit drinks).

Distil, avoiding entrainment and charring, occasionally agitating the contents of the flask, until the level of distillate is a few millimetres below the calibration mark of the volumetric flask.

When the temperature of this distillate has been brought down to within 0.5 ºC of the liquid's initial temperature, make up to the mark with distilled water and mix thoroughly.

This distillate is used for the determination of alcoholic strength by volume (Annex II)

6.3. Spirit drinks with alcoholic strength above 50 % vol.

Measure out 100 ml of the spirit drink into a 100 ml volumetric flask and pour into the round bottomed flask of the distillation apparatus.

Rinse the volumetric flask several times with distilled water and add the washings to the contents of the round-bottomed distillation flask. Use enough water to bring the flask's contents up to approximately 230 ml.

Pour 20 ml of distilled water into a 200 ml volumetric flask that will be used to hold the distillate. This flask must then be placed in a cold water bath (4.1) (10 °C to 15 °C for aniseed-flavoured spirits).

Distil, agitating the contents occasionally, until the level of distillate is a few millimetres below the calibration mark of the 200 ml volumetric flask.

When the temperature of this distillate has been brought down to within 0.5 °C of the liquid's initial temperature, make up to the mark with distilled water and mix thoroughly.

This distillate is used for the determination of alcoholic strength by volume (Annex II)

Note: The alcoholic strength by volume of the spirit drink is twice the alcoholic strength of the distillate.

OIV-MA-BS-03 Reference method for the determination of real alcoholic strength by volume of spirit drinks of viti-vinicultural origin: measurement by pycnometry

Type II method

1. Principle

The alcoholic strength by volume is obtained from the density of the distillate measured by pycnometry.

2. Reagents and Materials

During the analysis, unless otherwise is stated, use only reagents of recognised analytical grade and water of at least grade 3 as defined in ISO 3696:1987.

2.1. Sodium chloride solution (2 % w/v)

To prepare 1 litre, weigh out 20 g sodium chloride and dissolve to 1 litre using water.

3. Apparatus and Equipment

Usual laboratory apparatus and in particular the following.

3.1. Analytical balance capable of reading 0.1 mg.

3.2. Thermometer, with ground glass joint, calibrated in tenths of a degree from 10 to 30 °C. This thermometer must be certified or checked against a certified thermometer.

3.3. Pyrex glass pycnometer of approximately 100 ml capacity fitted with a removable ground-glass thermometer (A.3.2). The pycnometer has a side tube 25 mm in length and 1 mm (maximum) in internal diameter ending in a conical ground joint. Other pycnometers as described in ISO 3507 e.g. 50 ml may be used if appropriate.

3.4. A tare bottle of the same external volume (to within 1 ml) as the pycnometer and with a mass equal to the mass of the pycnometer filled with a liquid of density 1.01 (sodium chloride solution A.2.1).

3.5. Thermally insulated jacket that fits the body of the pycnometer exactly.

Note 1: The method for determining the densities in vacuo of spirits calls for the use of a twin-pan balance, a pycnometer and a tare bottle of the same outside external volume to cancel out the effect of air buoyancy at any given moment. This simple technique may be applied using a single-pan balance provided that the tare bottle is weighed again to monitor changes in air buoyancy over time.

4. Procedure

Preliminary remarks:

• The following procedure is described for the use of 100-ml pycnometer for determination of the alcoholic strength; this gives the best accuracy. However, it is also possible to use a smaller pycnometer, for example 50 ml.

4.1. Calibration of pycnometer

The pycnometer is calibrated by determining the following parameters:

• tare of the empty pycnometer,
• volume of the pycnometer at 20 °C,
• mass of the water-filled pycnometer at 20 °C.
  1.     Calibration using a single-pan balance

Determine:

• the mass of the clean, dry pycnometer (P),
• the mass of the water-filled pycnometer at t °C (P1)
• the mass of the tare bottle (T0).
  1.                      Weigh the clean, dry pycnometer (P).
  2.                      Fill the pycnometer carefully with distilled water at ambient temperature and fit the thermometer.

Carefully wipe the pycnometer dry and place it in the thermally-insulated jacket. Agitate by inverting the container until the thermometer's temperature reading is constant

Set the pycnometer flush with the upper rim of the side tube. Read the temperature t °C carefully and if necessary correct for any inaccuracies in the temperature scale.

Weigh the water-filled pycnometer (P1).

4.1.1.3.                     Weigh the tare bottle (T0).

4.1.1.4.                     Calculation

• Tare of the empty pycnometer = P - m
• where m is the mass of air in the pycnometer.
• m = 0.0012 x (P1 - P)

Note 2: 0.0012 is the density of dry air at 20 °C at a pressure of 760 mm Hg

• Volume of the pycnometer at 20 °C:

  = [P1 - (P - m)] x F_t

 where F_t is the factor for temperature t °C taken from Table I below.

  must be known to the nearest 0.001 ml.

• Mass of water in the pycnometer at 20 °C :

  = x 0.998203

 where 0.998203 is the density of water at 20 °C.

Note 3: If necessary, the value 0.99715 of the density in air can be used and the alcoholic strength calculated with reference to the corresponding density in HM Customs and Excise tables in air.

4.1.2.    Calibration method using a twin-pan balance:

4.1.2.1.                     Place the tare bottle on the left-hand pan and the clean, dry pycnometer with its collecting stopper on the right-hand pan. Balance them by placing weights on the pycnometer side: p grams. ( p )

4.1.2.2.                     Fill the pycnometer carefully with distilled water at ambient temperature and fit the thermometer; carefully wipe the pycnometer dry and place it in the thermally insulated jacket; agitate by inverting the container until the thermometer's temperature reading is constant.

Accurately adjust the level to the upper rim of the side tube. Clean the side tube, fit the collecting stopper; read the temperature t °C carefully and if necessary correct for any inaccuracies in the temperature scale.

Weigh the water-filled pycnometer, with p' the weight in grams making up the equilibrium. (p' )

4.1.2.3.                     Calculation

• Tare of the empty pycnometer = p + m

 where m is the mass of air in the pycnometer.

 m = 0.0012 x (p - p')

• Volume of the pycnometer at 20 °C:

  = (p + m - p') x F_t

 where F_t is the factor for temperature t °C taken from Table I below.

 V_{20 °C} must be known to the nearest 0.001 ml.

• Mass of water in the pycnometer at 20 °C:

  = x 0.998203

 where 0.998203 is the density of water at 20 °C.

4.2. Determination of alcoholic strength of test sample

4.2.1.    Using a single-pan balance.

4.2.1.1.                     Weigh the tare bottle, weight T1

4.2.1.2.                     Weigh the pycnometer with the prepared distillate (see Annex I), P2 is its weight at t °C.

4.2.1.3.                     Calculation

• dT = T1 - T0
• Mass of empty pycnometer at moment of measuring

 = P - m + dT

• Mass of the liquid in the pycnometer at t °C

 = P2 - (P - m + dT)

• Density at t °C in g/ml
• ρ_{t °C}= [P₂ –(P - m + dT)]/V_{20 °C}

 Express the density at t °C in kilograms per m³ by multiplying ρ_{t °C} by 1000, the value being known as ρ_t.

• Correct ρ_t to 20 using the table of densities ρT for water-alcohol mixtures in the Manual of Analysis Methods for Wines of the OIV.

In the table find the horizontal line corresponding to temperature T in whole degrees immediately below t °C, the smallest density above ρ_t. Use the table difference found below that density to calculate the density ρ_t of the spirit at that temperature T in whole degrees.

• Using the whole temperature line, calculate the difference between density ρ' in the table immediately above ρ_t and the calculated density ρ_t.  Divide that difference by the table difference found to the right of density ρ'. The quotient provides the decimal portion of the alcoholic strength while the integer of the alcoholic strength is found at the top of the column in which density ρ' is found (Dt, the alcoholic strength).

Note 4:  Alternatively keep the pycnometer in a water bath maintained at 20 °C (± 0.2 °C) when making up to the mark.

4.2.1.4.                     Result

Using the density ρ₂₀ calculate the real alcoholic strength using the alcoholic strength tables identified below:

The table giving the value of the alcoholic strength by volume (% vol.) at 20 °C as a function of the density at 20 °C of water-alcohol mixtures is the international table adopted by the International Legal Metrology Organisation in its Recommendation no. 22.

4.2.2.    Method using a single-pan balance

4.2.2.1.                     Weigh the pycnometer with the distillate prepared (see part I), p" is mass at t °C.

4.2.2.2.                     Calculation

• Mass of the liquid in the pycnometer at t °C

 = p + m - p"

• Density at t °C in g/ml

ρ_{t °C} = (p + m - p")/V_{20 °C}

• Express the density at t °C in kilograms per m³ and carry out the temperature correction in order to calculate the alcoholic strength at 20 °C, as indicated above for use of the single-pan balance.

5. Method performance characteristics (Precision)

 

5.1. Statistical results of the interlaboratory test

The following data were obtained from an international method performance study carried out on a variety of spirit drinks to internationally agreed procedures.

Year of interlaboratory test	1997
Number of laboratories	20
Number of samples	6

Samples	A	B	C
Number of laboratories retained after eliminating outliers	19	20	17
Number of outliers (Laboratories)	1	-	2
Number of accepted results	38	40	34
Mean value (	23.77	40.04	40.29
	26.51*
Repeatability standard deviation (sr) % vol.	0.106	0.176	0.072
Repeatability relative standard deviation (RSDr)  (%)	0.42	0.44	0.18
Repeatability limit ( r )  % vol.	0.30	0.49	0.20
Reproducibility standard deviation (sR) % vol.	0.131	0.236	0.154
Reproducibility relative standard deviation (RSDR)  (%)	0.52	0.59	0.38
Reproducibility limit ( R )   % vol.	0.37	0.66	0.43

Sample types

A Fruit liqueur; split level*

B Brandy; blind duplicates

C Whisky; blind duplicates

Samples	D	E	F
Number of laboratories retained after eliminating outliers	19	19	17
Number of outliers (Laboratories)	1	1	3
Number of accepted results	38	38	34
Mean value (	39.20	42.24	57.03
	42.93*	45.73*	63.03*
Repeatability standard deviation (sr) % vol.	0.103	0.171	0.190
Repeatability relative standard deviation (RSDr)  (%)	0.25	0.39	0.32
Repeatability limit ( r )  % vol.	0.29	0.48	0.53
Reproducibility standard deviation (sR) % vol.	0.233	0.238	0.322
Reproducibility relative standard deviation (RSDR)  (%)	0.57	0.54	0.53
Reproducibility limit ( R )   % vol.	0.65	0.67	0.90

Sample types

D grappa;  split level*

E aquavit;  split level*

F rum; split level*

OIV-MA-BS-04 Reference method for the determination of real alcoholic strength by volume of spirit drinks of viti-vinicultural origin: measurement by electronic densimetry (based on the resonant frequency oscillation of a sample in an oscillating cell)

Type II method

1. Principle

The liquid's density is determined by electronic measurement of the oscillations of a vibrating U-tube. To perform this measurement, the sample is added to an oscillating system, whose specific oscillation frequency is thus modified by the added mass.

2. Reagents and Materials

During the analysis, unless otherwise is stated, use only reagents of recognised analytical grade and water of at least grade 3 as defined in ISO 3696:1987.

2.1. Acetone (CAS 666-52-4) or absolute alcohol

2.2. Dry air.

3. Apparatus and Equipment

Usual laboratory apparatus and in particular the following.

3.1. Digital display densimeter

Electronic densimeter for performing such measurements must be capable of expressing density in g/ml to 5 decimal places.

Note 1: The densimeter should be placed on a perfectly stable stand that is insulated from all vibrations.

3.2. Temperature regulation

The densimeter's performance is valid only if the measuring cell is connected to a built-in temperature regulator that can achieve the same temperature stability of 0.02 ºC or better.

Note 2:  The precise setting and monitoring of the temperature in the measuring cell are very important, for an error of 0.1 °C can lead to a variation in density of the order of 0.0001 g/mL.

3.3. Sample injection syringes, auto sampler, or other equivalent system.

4. Procedure

4.1. Calibration of the densimeter

The apparatus must be calibrated according to the instrument manufacturer's instructions when it is first put into service. It must be recalibrated regularly and checked against a certified reference standard or an internal laboratory reference solution based on a certified reference standard.

4.2. Determination of sample density

4.2.1.    If required prior to measurement clean and dry the cell with acetone or absolute alcohol and dry air. Rinse the cell with the sample.

4.2.2.    Inject the sample into the cell (using a syringe, autosampler, or other equivalent system) so that the cell is completely filled. During the filling operation make sure that all air bubbles are completely eliminated. The sample must be homogeneous and must not contain any solid particles. Any suspended matter should be removed by filtration prior to analysis.

4.2.3.    Once the reading has stabilised, record the density ₂₀ or the alcoholic strength displayed by the densimeter.

4.3. Result:

When the density ₂₀ is used, calculate the real alcoholic strength using the alcoholic strength tables identified below:

The table giving the value of the alcoholic strength by volume (% vol.) at 20 °C as a function of the density at 20 °C of water-alcohol mixtures is the international table adopted by the International Legal Metrology Organisation in its Recommendation No. 22 (Table IVa).

 

5. Method performance characteristics (Precision)

5.1. Statistical results of the interlaboratory test

The following data were obtained from an international method performance study carried out on a variety of spirit drinks to internationally agreed procedures.

 

Year of interlaboratory test	1997
Number of laboratories	16
Number of samples	6

Samples	A	B	C
Number of laboratories retained after eliminating outliers	11	13	15
Number of outliers (Laboratories)	2	3	1
Number of accepted results	22	26	30
Mean value	23.81	40.12	40.35
	26.52*
Repeatability standard deviation (sr)   % vol.	0.044	0.046	0.027
Repeatability relative standard deviation (RSDr)  (%)	0.17	0.12	0.07
Repeatability limit ( r )  % vol.	0.12	0.13	0.08
Reproducibility standard deviation (sR) % vol.	0.054	0.069	0.083
Reproducibility relative standard deviation (RSDR)  (%)	0.21	0.17	0.21
Reproducibility limit ( R )   % vol.	0.15	0.19	0.23

Sample types

A Fruit liqueur ; split level*

B Brandy ; blind duplicates

C Whisky ; blind duplicates

Samples	D	E	F
Number of laboratories retained after eliminating outliers	16	14	13
Number of outliers (Laboratories)	-	1	2
Number of accepted results	32	28	26
Mean value	39.27	42.39	56.99
	43.10*	45.91*	63.31*
Repeatability standard deviation (sr)   % vol.	0.079	0.172	0.144
Repeatability relative standard deviation (RSDr)  (%)	0.19	0.39	0.24
Repeatability limit ( r )  % vol.	0.22	0.48	0.40
Reproducibility standard deviation (sR) % vol.	0.141	0.197	0.205
Reproducibility relative standard deviation (RSDR)  (%)	0.34	0.45	0.34
Reproducibility limit ( R )   % vol.	0.40	0.55	0.58

Sample types

D Grappa; split level*

E Aquavit; split level*

F Rum; split level*

OIV-MA-BS-05 Reference method for the determination of real alcoholic strength by volume of spirit drinks of viti-vinicultural origin: Measurement by densimetry using hydrostatic balance

Type II method

1. Principle

The alcoholic strength of spirits can be measured by densimetry using a hydrostatic balance based on Archimedes' principle according to which a body immersed in a liquid receives a vertical upward thrust from the liquid equal to the weight of liquid displaced.

 

2. Reagents and Materials

During the analysis, unless otherwise is stated, use only reagents of recognised analytical grade and water of at least grade 3 as defined in ISO 3696:1987.

2.1. Float cleaning solution (sodium hydroxide, 30 % w/v)

To prepare 100 ml weigh 30 g sodium hydroxide and make up to volume using 96 % volume ethanol.

 

3. Apparatus and Equipment

Usual laboratory apparatus and in particular the following.

3.1. Single-pan hydrostatic balance with a sensitivity of 1 mg.

3.2. Float with a volume of at least 20 ml, specially adapted to the balance, suspended with a thread of diameter not exceeding 0.1 mm.

3.3. Measuring cylinder bearing a level mark. The float must be capable of being contained completely within the volume of the cylinder located below the mark; the surface of the liquid may only be penetrated by the supporting thread. The measuring cylinder must have an internal diameter at least 6 mm larger than that of the float.

3.4. Thermometer (or temperature-measuring probe) graduated in degrees and tenths of a degree from 10 to 40 °C, calibrated to 0.05 °C.

Weights, calibrated by a recognised certifying body.

Note 1:  Use of a twin-pan balance is also possible; the principle is described in the Manual of Analysis Methods for Wines of the OIV.

 

4. Procedure

The float and measuring cylinder must be cleaned between each measurement with distilled water, dried with soft laboratory paper which does not shed fibres and rinsed with the solution whose density is to be determined. Measurements must be made as soon as the apparatus has reached stability so as to restrict alcohol loss by evaporation.

4.1. Calibration of the balance

Although balances usually have an internal calibration system, the hydrostatic balance must be capable of calibration with weights checked by an official certifying body.

4.2. Calibration of the float

4.2.1.    Fill the measuring cylinder to the mark with double-distilled water (or water of equivalent purity, e.g. microfiltered water with a conductivity of 18.2 M/cm) at a temperature between 15 °C and 25 °C but preferably at 20 °C.

4.2.2.    Immerse the float and the thermometer, stir, read off the density of the liquid from the apparatus and, if necessary, correct the reading so that it is equal to that of the water at measurement temperature.

4.3. Control using a water-alcohol solution

4.3.1.    Fill the measuring cylinder to the mark with a water-alcohol mixture of known strength at a temperature between 15 °C and 25 °C but preferably at 20 °C.

4.3.2.    Immerse the float and the thermometer, stir, read off the density of the liquid (or the alcoholic strength if this is possible) from the apparatus. The alcoholic strength thus established should be equal to the previously determined alcoholic strength.

Note 2:  This solution of known alcoholic strength can also be used to calibrate the float instead of double-distilled water.

4.4. Measurement of the density of a distillate (or of its alcoholic strength if the apparatus allows)

4.4.1.    Pour the test sample into the measuring cylinder up to the graduation mark.

4.4.2.    Immerse the float and the thermometer, stir, read off the density of the liquid (or the alcoholic strength if this is possible) from the apparatus. Note the temperature if the density is measured at t °C (ρ_t).

4.4.3.    Correct _t to 20 using the table of densities T for water-alcohol mixtures in the Manual of Analysis Methods for Wines of the OIV.

4.5. Cleaning of float and measuring cylinder

4.5.1.    Immerse the float in the float cleaning solution in the measuring cylinder.

4.5.2.    Allow to soak for one hour spinning the float periodically.

4.5.3.    Rinse with copious amounts of tap water followed by distilled water.

4.5.4.    Dry with soft laboratory paper which does not shed fibres.

Carry out this procedure when the float is first used and then regularly as required.

4.6. Result

Using the density ₂₀ calculate the real alcoholic strength using the alcoholic strength tables identified below.

The table giving the value of the alcoholic strength by volume (% vol.) at 20 °C as a function of the density at 20 °C of water-alcohol mixtures is the international table adopted by the International Legal Metrology Organisation in its Recommendation no. 22.

5. Method performance characteristics (Precision)

5.1. Statistical results of the interlaboratory test

The following data were obtained from an international method performance study carried out on a variety of spirit drinks to internationally agreed procedures.

Year of interlaboratory test	1997
Number of laboratories	12
Number of samples	6

Samples	A	B	C
Number of laboratories retained after eliminating outliers	12	10	11
Number of outliers (Laboratories)	-	2	1
Number of accepted results	24	20	22
Mean value (	23.80	40.09	40.29
	26.51*
Repeatability standard deviation (sr) % vol.	0.048	0.065	0.042
Repeatability relative standard deviation (RSDr)  (%)	0.19	0.16	0.10
Repeatability limit ( r )  % vol.	0.13	0.18	0.12
Reproducibility standard deviation (sR) % vol.	0.060	0.076	0.073
Reproducibility relative standard deviation (RSDR)  (%)	0.24	0.19	0.18
Reproducibility limit ( R )   % vol.	0.17	0.21	0.20

Sample types

A Fruit liqueur; split level*

B Brandy; blind duplicates

C Whisky; blind duplicates

Samples	D	E	F
Number of laboratories retained after eliminating outliers	12	11	9
Number of outliers (Laboratories)	-	1	2
Number of accepted results	24	22	18
Mean value (	39.26	42.38	57.16
	43.09*	45.89*	63.44*
Repeatability standard deviation (sr) % vol.	0.099	0.094	0.106
Repeatability relative standard deviation (RSDr)  (%)	0.24	0.21	0.18
Repeatability limit ( r )  % vol.	0.28	0.26	0.30
Reproducibility standard deviation (sR) % vol.	0.118	0.103	0.125
Reproducibility relative standard deviation (RSDR)  (%)	0.29	0.23	0.21
Reproducibility limit ( R )   % vol.	0.33	0.29	0.35

Sample types

D Grappa; split level*

E Aquavit; split level*

F Rum; split level*

OIV-MA-BS-09 Method for the determination of total dry extract of spirit drinks of viti-vinicultural origin: gravimetric method

Type II method

1. Scope

This method is suited to the determination of the total dry extract in spirit drinks of viti-vinicultural origin whichcontain less than 15 g/L of dry matter.

 

2. Normative References

 

ISO 3696:1987 Water for analytical laboratory use - Specifications and test methods.

 

3. Definition

 

The total dry extract or total dry matter includes all matter that is non-volatile under specified physical conditions.

 

4. Principle

 

Weighing of the residue left by evaporation of the spirit on a boiling water bath and drying in a drying oven.

 

5. Apparatus and Equipment
   1.    Flat-bottomed stainless-steel cylindrical capsule, of sufficient dimensions to avoid loss of liquid when evaporating.
   2.    Boiling water bath.
   3.    25 ml pipette, class A.
   4.    Drying oven.
   5.    Dessicator.
   6.    Analytical balance accurate to 0.1 mg.

6. Sampling and Samples.

Samples are stored at room temperature prior to analysis.

 

7. Procedure
   1.    Pipette 25 ml of the spirit drink into a previously-weighed cylindrical capsule (5.1). During the first hour of evaporation the evaporating dish is placed on the lid of a boiling water bath so that the liquid will not boil, as this could lead to losses through splattering. Leave one more hour directly in contact with the steam of the boiling water bath.
   2.    Complete the drying by placing the evaporating dish in a drying oven at 105 °C 3 °C for two hours. Allow the evaporating dish to cool in a dessicator and weigh the evaporating dish and its contents.

 

8. Calculation

The mass of the residue multiplied by 40 is equal to the dry extract contained in the spirit and it must be expressed in g/l to one decimal place.

9. Method performance characteristics (Precision)
   1.    Statistical results of the interlaboratory test

The following data were obtained from an international method performance study carried out on a variety of spirit drinks to internationally agreed procedures.

Year of interlaboratory test	1997
Number of laboratories	10
Number of samples	4

Samples	A	B	C	D
Number of laboratories retained after eliminating outliers	9	9	8	9
Number of outliers (Laboratories)	1	1	2	-
Number of accepted results	18	18	16	18
	9.0	9.1	10.0	11.8
		7.8	9.4	11.1
Repeatability standard deviation (sr) g/l	0.075	0.441	0.028	0.123
Repeatability relative standard deviation (RSDr)  (%)	0.8	5.2	0.3	1.1
Repeatability limit ( r )   g/l	0.2	1.2	0.1	0.3
Reproducibility standard deviation (sR)   g/l	0.148	0.451	0.058	0.210
Reproducibility relative standard deviation (RSDR)  (%)	1.6	5.3	0.6	1.8
Reproducibility limit ( R )   g/l	0.4	1.3	0.2	0.6

Sample types

A Brandy ; blind duplicates

B Rum ; split levels

C Grappa ; split levels

D Aquavit ;  split levels

10. Bibliography

• Commission Regulation (EC) N° 2870/2000 of 19 December 2000 laying down Community reference methods for the analysis of spirits drinks, OJEC of 29 December 2000, L333/20
• P. Brereton, S. Hasnip, A. Bertrand, R. Wittkowski, C. Guillou, Analytical methods for the determination of spirit drinks, Trends in Analytical Chemistry, Vol. 22, No. 1, 19-25, 2003

Method OIV-MA-BS-08 : R2009

Type IV method

ABV by near infrared spectroscopy in spirit drinks of viti-viniculture origin

(OENO 6/94;

OIV/OENO 382A/2009)

1.                Introduction

This method of determining the real alcoholic strength by volume of alcoholic beverages and distillates is based on the physical principle of the spectral analysis of materials with absorption bands in the near infrared range.

Ethanol has this characteristic.

The spectral data of the sample being tested are compared with those obtained during an initial calibration covering the entire measurement range.

Spectrometers employing this principle are commercially available to perform this determination.

2.                Object and scope of application

The purpose of this document is to describe a method for determining the real alcoholic strength of alcoholic beverages and distillates handled at atmospheric pressure.

The application of the method is restricted to products with a viscosity of less than around 15,000 mm²/S (1 mm²/S = 1 cSt) at the test temperature.

The analysis of alcoholic beverages whose composition is estimated to be close may nevertheless require a separate initial calibration for each of them.

With reference to the currently applicable regulations, the test temperature is set to 20°C.

3.                Definition

Real alcoholic strength by volume (See pycnometry).

4.                Principle

4.1.      Physical principle

According to quantum theory, a molecule is capable of absorbing light energy according to Planck's formula:

Where:

• h = Planck constant
• C = speed of light
• E1 = fundamental energy state of the electron
• E2 = excited energy state of the electron,

From which it follows that the energy absorbed is proportional to the frequency of the incident light.

Near-infrared spectroscopy is a physical method of analysis based on the absorption of hv photons with very little energy that can be used to change the vibrational energy of molecules.

The number of v' waves is proportional to the v "frequencies" and hence to the hv energy of the photon.

The observed transitions correspond to vibrations of clearly identified groups of atoms.

They result in non-separable rays clustered into "bands" (band spectra), which can often be used for functional analysis.

In practice, only three transitions can be observed:

• transition from v = 0 to v = 1 with a high intensity,
• transition from v = 0 to v = 2 with a low intensity,
• transition from v = 0 to v = 3 with a negligible intensity,
• v = vibrational quantum number.

The corresponding three spectral bands are approximately at v (fundamental), 2v (first harmonic), 3v (second harmonic) frequencies.

The fundamental vibrations can be observed in the mid-infrared range, while the harmonics are only visible in the near infrared range (700 - 2500 nanometres).

In addition to the harmonics, combination bands can be observed, when several vibrations interact, resulting in bands whose frequency is the sum or difference of multiples of the fundamental frequencies.

Spectroscopy in the near infrared range spans the entire electromagnetic spectrum from 780 nm to 3000 nm. In this range, it is possible to study the transitions, harmonics and low-energy electronic combinations of the stretching and deformation vibrations of hydrogen bonds (C - H, N - H, O - H); the latter have high frequencies and are suitable for quantitative analysis applications.

Although it does not necessarily enable the characterisation of a complete structure, a near infrared spectrum provides useful information about the hydrogen clustering of a molecule.

Accordingly, near IR spectroscopy can be used first of all for the quantitative determination of components comprising clusters such as C - H, O - H or N - H, i.e. including water, alcohols, phenols , etc., preferably for the characterization of molecular structures.

Generally, the C - H cluster is characterized by stretching fundamental bands between: 3.0 and 3.6 microns, stretching bands of the first harmonics, between 1.6 and 1.8 microns and stretching bands of the second harmonics between 1.1 and 1.2 microns.

Because of the influence of other functional clusters of the molecule, these bands are liable to undergo shifts.

The vibrations of N - H secondary movements are characterized by stretching fundamental bands at 2.9 microns, the first harmonics at 1.5 microns and the second harmonics at 1.0 microns. The N - H cluster has a highly characteristic band of combinations around 2.2 microns.

The O-H cluster has

• a fundamental stretching band at 2.8 microns,
• the first harmonics at 1.4 microns and
• the second harmonics at 1.0 microns;

in addition, there is

• a combination band around 2 microns.

Bands of this type are used for the quantitative determination of various organic components, both monomeric and polymeric.

Absorption bands in the near infrared range

2500 nm	_____ C-H	Combinations
2200 nm	_____ O-H N-H	Combinations
1800 nm	_____ C-H	First harmonics
1600 nm	_____ N-H H-O	First harmonics
1420 nm	_____ C-H	Combinations
1300 nm	_____ C-H	Combinations
1100 nm

4.2.      Principle de measurement

4.2.1.                    A sample of a few millilitres of liquid is introduced into a measuring cell thermostated at the test temperature.

4.2.2.                    The sample is exposed to infrared radiation whose wavelengths have been previously selected by a primary calibration specific to the analyte.

With regard to ethanol, these wavelengths are generally four to five in number.

4.2.3.                    The beam of the light source is located through a collimator and a "chopper" directly on a filter wheel, selected automatically by the microprocessor.

The monochromatic light is then directed either to the measuring cell or to the reference by a tilting mirror.

The infrared rays penetrate the sample, interact with its components and are then reflected to the detector(s).

4.2.4.                    The spectral data of the sample are processed by the microprocessor integrated with the spectroscope and compared with calibration curves that have been determined and stored beforehand.

The regression equation is of the type:

Where

• % C = percentage strength by volume,
• F₀ - Fn = constants corresponding to ethanol,
• R₁ - Rn = spectral reflection values measured at wavelengths from 1 to n.

After about a minute, the result is displayed by the apparatus. It is directly expressed as a percentage strength by volume.

5.                Apparatus

5.1.      NIR Spectroscopes

Two variants of apparatus suitable for measuring the real alcoholic strength of alcoholic beverages are available on the market.

They differ mainly by the type of measuring cell used.

Transflectance principle: the bottom of the measuring cell is fitted with a reflector which reflects the light beam having passed through the sample; the light can then interact again with the sample. This combination of transmission and reflection is called transflectance.

Transmission principle: the measuring cell is mounted vertically. The sample is directly crossed by the ray of light.

5.2.      The apparatus consists of the following items:

• sample pumping system,
• light source,
• wavelength selection appliance,
• thermostated measuring cell,
• detectors converting light energy into an electrical signal,
• computer system to process the signals and display the results.

5.2.1.                    Sample pumping system.

The sample is injected into the measuring cell using a peristaltic pump. Some spectroscopes can be fitted with an automatic sample changer.

5.2.2.                    Light source.

Thermal light sources are mainly used. In tungsten filament lamps, the most commonly used, the filament is heated to 2100C by the transformation of electrical energy. The polychromatic light obtained has a spectrum ranging between 320 nm and 2500 nm. It is necessary to control very precisely the intensity of the light in order to obtain repeatable measurements.

5.2.3.                    Wavelength selection appliance

Three basic principles are commonly applied: interference filters, tilting filters, and grating monochromators.

Interference filters are constituted by a layer of a semi-transparent material, such as magnesium fluoride, placed between two semi-reflecting layers. Under these conditions, the incident light interferes inside the filter and only certain wavelengths, depending on the thickness of the transparent layer, pass through the appliance.

Market-available appliances include three to twenty filters whose central wavelengths have been carefully selected.

The filters are attached onto a thermostated wheel, whose rotation is controlled by microprocessor.

Tilting filter systems take into account the fact that the wavelength selected by an interference filter depends on the angle of incidence between the ray of light and the filter. By varying this angle, it is possible to select different wavelengths around the central value. A large number of spectral measurements can thus be obtained with only a few filters. The correspondence between the position of the wheel carrying the filters and the measurement wavelength is, however, difficult to establish.

Grating monochromators are polished mirrors on which numerous parallel grooves are etched. The grooves diffract light and act as light sources that are phase-shifted in relation to each other. This causes light interference, as in the case of filters, and can be used to select wavelengths by turning the grate. Spectral measurements can be taken every 2 nm between 1100 and 2500 nm, providing 700 measurement points for each sample.

5.2.4.                    Thermostated measuring cell.

The optical walls are made of quartz.

Temperature control of the chamber comprising the cell is obtained by means of an integrated semiconductor element which uses the Peltier effect.

5.2.5.                    Detectors.

The detectors most commonly used are made of lead sulphide. These are semiconductors whose resistance decreases as the incident light intensity increases. They operate in the spectral range from 1000 nm to 2500 nm.

5.2.6.                    Data processing and display.

The spectral data are first of all collected in the form of continuous electrical signals. In general, the raw data includes successive measurements of the light intensity of the source (I0) and that of the sample (I). These data are converted analogously into absorbance values [log (I0/I)] and digitized.

On the simplest appliances, digitized spectral data are not stored but are used to predict the response variable, which is immediately displayed.

On other systems, the spectrometer is coupled to a microcomputer which can be used to store spectral information, manage data files, and carry out the mathematical and statistical analyses.

6.                Products

6.1.      Products to clean the measuring cell

Cell cleaning is recommended at the end of each series of measurements and can be performed using the following solutions:

• Aqueous solution of sodium hypochlorite (NaClO), at market-available concentration, diluted to one tenth,
• Laboratory glassware cleaning agent, suitably diluted.

Cleaning should be followed by prolonged rinsing with freshly prepared, distilled or demineralised water.

6.2.      Calibration substances.

The calibration substances must be chosen such that:

• The values of their alcoholic strengths by volume cover those of the products to be measured,
• they are based on a common matrix, except for their alcohol content, with identical compositional characteristics. The nature and composition of the matrix are essential in ensuring the reliability of the NIR spectroscopy technique.

Given the large number of samples required for calibration, their alcoholic strength by volume may be determined beforehand using:

• the reference method,
• the areometric method using EC Class I alcoholmeters, - the electronic densimetry method.

(see the description of these methods).

Remark: The determination of alcoholic strength by volume according to one of these two methods is, where appropriate, performed after distilling the sample.

The analytical application in the near infrared range resulting from this calibration will have at best an accuracy equivalent to that of the method used.

7.                Calibration of apparatus

7.1.      The implementation of a quantitative analysis technique in the near infrared range involves several levels of calibration:

• initial calibration in order to select, according to statistical calculations, a variable number of significant wavelengths of the characteristic (ethanol) to be analyzed,
• periodic re-calibration to verify the reliability of the calibration equation,
• routine calibration to correct the bias of the reference curve. It should be performed before each series of measurements.

7.2.      Initial calibration.

This operation requires the use of a spectroscope in the near IR capable of performing measurements in a series of twenty successive wavelengths.

The connection between the spectral data and the characteristics that are to be predicted by near NIR spectroscopy are often difficult to determine.

The spectral bands overlap to a considerable degree and it is usually impossible to establish an analytical application of the single measurement of the height of a significant peak. On the contrary, a calibration procedure must be used that is quite complex to implement. The calibration is only valid for the determination of the alcoholic strength by volume of alcoholic beverages with strictly identical compositional characteristics.  There are six steps in the process.

7.2.1.                    Establish a set of representative samples and analyze them using the reference method.

The collection of standard solutions must include thirty to fifty individual samples and cover the entire concentration range encountered in practice.

In addition, they must be divided into concentration classes of approximately the same size.

7.2.2.                    The collection is divided into two separate lots: one is used for calibration, the second for verification purposes.

7.2.3.                    Carry out the spectral measurement of the calibration collection: each standard solution must be analyzed twice in succession (double sampling).

7.2.4.                    The alcohol concentration values obtained by the reference method are entered on a microcomputer equipped with software for statistical computing.

The values are then correlated with the spectral measurements.

7.2.5.                    A multi-linear regression program is used to establish the following relation on the calibration samples:

where

• C, is the characteristic being measured,
• a₀, a₁, a₂, ... : are the regression coefficients,
• r₁, r₂, r₃, ... : are the spectral reflectance measurements at wavelengths: L₁, L₂, L₃ ...

Two to ten wavelengths are selected from among those that are available, based on statistical criteria. The residual error of calibration is calculated: it must be small compared with the standard deviation of the characteristic being studied.

where

• d_i = difference between the concentrations obtained by the reference method and those obtained by NIR spectroscopy
• d = average di
• n = number of samples used for calibration
• k = number of calibration wavelengths.

7.2.6.                    Carry out the spectral measurement of the verification collection and apply the equation with the values obtained.

Compare the residual error of verification with that for the calibration: they should be close.

Standard deviation of prediction:

where

• n = number of standard solutions used to verify the calibration,
• di = difference between the concentrations obtained by the reference method and those obtained by NIR spectroscopy,
• d = average di.

When the wavelengths have been selected and the calibration has been performed, and the results are recognized as being statistically consistent, the analytical method can be routinely applied.

7.3.      Periodic recalibration.

Aging of the electronic components, repairs, parts replacement, or other abnormalities, require periodic recalibration of the equipment.

Similarly, the transfer of the calibration process from one appliance to another requires periodic recalibration.

Recalibration involves adjusting the bias and sometimes the slope of the initial calibration equation.

This procedure does not affect the selection of wavelengths.

In practice, in order to limit the sources of error, it is preferable to analyze the spectrum of ten representative samples covering the entire calibration range. These standard substances are recognized beforehand using the reference method.

In this case the multilinear calibration equation becomes a simple linear equation:

where

• F₀, is the bias,
• m, is the slope.

7.4.      Calibration of routine bias correction.

This correction must be made before any series of measurements, and at least once a day.

Using NIR spectroscopy, analyse a standard solution whose alcoholic strength by volume has been determined beforehand using the reference method.

The bias value is adjusted by assigning it the difference obtained between the measurement of the reference method and that of the spectroscopic method. The difference can be negative or positive.

8.                Procedure

8.1.      Preparation of test apparatus.

Place the spectroscope:

• on a perfectly stable support, isolated from any vibrations.
• away from direct sunlight,
• free from corrosive vapours, magnetic fields, and large variations in temperature.

After connecting the apparatus to a power source, allow it to warm for at least thirty minutes.

Fill the thermostat unit of the measuring cell with a coolant in accordance with the manufacturer's instructions. Set the temperature in order to reach and maintain the requisite test temperature.

8.2.      Measurement of alcoholic strength by volume.

8.2.1.                    If necessary, select the spectroscopic method corresponding to the alcoholic beverage to be analyzed.

8.2.2.                    Check the cleanliness of the measuring cell:

• no particles in the cell,
• if necessary, clean the window using a brush and a soft cloth dampened with ethyl alcohol.

8.2.3.                    Calibrate the bias correction in accordance with the method described in point: 7.40.

8.2.4.                    Filter the sample first, if necessary.

8.2.5.                    Rinse at length the measuring cell with the alcoholic beverage to be tested.

Filter if necessary.

8.2.6.                    Carry out the determination. After approximately one minute, the result is displayed on the easy-to-read display.

8.2.7.                    Carry out five determinations in a row for the same sample: (the use of this analytical technique allows measurements to be obtained in a very short period of time).

The value of the alcoholic strength by volume of the sample is based on the calculation of the average for the five determinations.

Note: The five determinations must result in homogeneous values, in all cases covering the range of accuracy of the reference method used.

In the opposite case, carry out a second complete series of measurements after checking the cleanliness of the measuring cell and if necessary re-calibrating the bias of the calibration curve.

8.2.8.                    Check the relevance of the measurement accuracy; determinations performed in series should include the periodic analysis of a standard solution recognized by the reference method.

The cycle is to be respected, under the conditions described above, involves the analysis of a standard after five determinations.

8.2.9.                    Clean and rinse the measuring cell at length, at the end of the analysis.

CALIBRATION OF AN INFRALYSER FOR THE DETERMINATION OF THE ALCOHOLIC STRENGTH BY VOLUME ON BRANDIES OR LIQUEUR WINES

1.                Selection of filters

As an example, the filter selections listed below can be used to measure the alcoholic strength by volume in the following alcoholic beverages:

1.1.      Wine brandies aged in wooden casks

1.1.1.                    First combination.

• 2310 nm
• 1778 nm
• 2100 nm
• 1680 nm

1.1.2.                    Second combination.

• 2310 nm
• 2230 nm
• 1769 nm
• 1940 nm
• 1680 nm

1.2.      "Pastis" aniseed-flavoured alcoholic beverage.

• 2270 nm
• 2230 nm
• 1769 nm
• 1940 nm
• 1680 nm

Use of an infralyser for WINE BRANDIES

Select the following filters: 4, 13, 14 and 20.

Four levels of alcoholic strength by volume are calibrated on raw brandies:

1 : 37.5 to 43 % vol.

2 : 42.5 to 47.5 % vol.

3 : 57.5 to 62 % vol.

4 : 67.5 to 72.5 % vol.

For each level, and by increments of 0.5% vol., 10 to 11 determinations of the alcoholic strength by volume based on the pycnometric method are used to calibrate the infralyser

2.                Bibliography

1. Calibration of an infralyser for the determination of the alcoholic strength by volume on brandies or liqueur wines.
2. Station viticole, Cognac National Interprofessionnel Bureau

OIV-MA-BS-15 Anethole. Gas chromatography determination of trans-anethole in Spirit drinks of viti-vinicultural origin

Type II method

1. Scope

This method is suitable for the determination of trans-anethole in aniseed-flavoured spirit drinks using capillary gas chromatography.

2. Normative references

ISO 3696: 1987 Water for analytical laboratory use - Specifications and test methods.

3. Principle

The trans-anethole concentration of the spirit is determined by gas chromatography (GC). The same quantity of an internal standard, e.g. 4‑allylanisole (estragole) when estragole is not naturally present in the sample, is added to the test sample and to a trans‑anethole reference solution of known concentration, both of which are then diluted with a 45% ethanol solution and injected directly into the GC system.

An extraction is necessary before sample preparation and analysis for liqueurs that contain large amounts of sugars.

4. Reagents and materials

During the analysis use only reagents of a purity of at least 98 %.  Water of at least grade 3 as defined by ISO 3696 should be used.

Reference chemicals should be stored cold (ca. 4°C), away from light, in aluminium containers or in tinted (amber) glass reagent bottles.  The stoppers should preferably be fitted with an aluminium seal. Trans-anethole will need to be "thawed" from its crystalline state before use, but in this case its temperature should never exceed 35°C.

4.1. Ethanol 96 % vol.  (CAS 64-17-5)

4.2. 1-methoxy-4- (1-propenyl) benzene; (trans-anethole) (CAS 4180-23-8)

4.3. 4-allylanisole, (estragole) (CAS 140-67-0), suggested internal standard (IS)

4.4. Ethanol 45 % vol.

Add 560 g of distilled water to 378 g of ethanol 96 % vol.

4.5. Preparation of standard solutions

All standard solutions should be stored at room temperature (15-35°C) away from light in aluminium containers or in tinted (amber) glass reagent bottles.  The stopper should preferably be fitted with an aluminium seal.

Trans-anethole and 4-allylanisole are practically insoluble in water, and it is therefore necessary to dissolve the trans-anethole and 4-allylanisole in some 96 % ethanol (4.1) before the addition of 45 % ethanol (4.4).

The stock solutions must be freshly prepared each week.

4.5.1.    Standard solution A

Stock solution of trans‑anethole (concentration: 2 g/L)

Weigh 40 mg of trans-anethole (4.2) in a 20 mL volumetric flask (or 400 mg in 200 mL, etc.).  Add some 96 % ethanol (4.1) and make up to volume with 45 % vol. ethanol (4.4), mix thoroughly.

4.5.2.    Internal standard solution B

Stock solution of internal standard, e.g. estragole (concentration: 2 g/L)

Weigh 40 mg of estragole (4.3) in a 20 mL volumetric flask (400 mg in 200 mL etc.).  Add some 96 % vol. ethanol (4.1) make up to volume with 45 % vol. ethanol (4.4), mix thoroughly.

4.5.3.    Solutions used to check the linearity response of the FID

The linearity response of the FID must be checked for the analysis taking into account a range of concentrations of trans-anethole in spirits from 0 g/L up to 2.5 g/L. In the procedure of analysis, the unknown samples of spirits to be analysed are diluted 10 times (8.3). For the conditions of the analysis described in the method, stock solutions corresponding to concentrations of 0, 0.05, 0.1, 0.15, 0.2, and 0.25 g/L of trans-anethole in the sample to be analysed are prepared as follows: take 0.5, 1, 1.5, 2, and 2.5 mL of stock solution A (4.5.1) and pipette in separate 20 mL volumetric flasks; pipette into each flask 2 mL of internal standard solution B (4.5.2) and make up to volume with 45 % vol. ethanol (4.4), mix thoroughly.

The blank solutions (8.4) is used as the 0 g/L solution.

4.5.4.    Standard solution C

Take 2 mL of standard solution A (4.5.1) and pipette into a 20 mL volumetric flask then add 2 mL of internal standard solution B (4.5.2) and make up to volume with 45% vol. ethanol (4.4), mix thoroughly.

5. Apparatus and equipment

5.1. A capillary gas chromatograph fitted with a flame ionisation detector (FID) and integrator or other data handling system capable of measuring peak areas, and with an automatic sampler or the necessary equipment for manual sample injection.

5.2. Split/splitless injector

5.3. Capillary column, for example:

Length:  50 m

Internal diameter: 0.32 mm

Film thickness: 0.2 µm

Stationary phase: FFAP ‑ modified TPA polyethylene glycol cross‑linked porous polymer

Common laboratory equipment: A grade volumetric glassware, analytical balance (precision:  ±0.1 mg).

6. Chromatography conditions

The column type and dimensions, and the GC conditions, should be such that anethole and the internal standard are separated from each other and from any interfering substances.  Typical conditions for the column given as an example in 5.3 are:

6.1. Carrier gas: analytical helium.

6.2. Flow rate: 2 mL/min

6.3. Injector temperature: 250°C.

6.4. Detector temperature: 250°C.

6.5. Oven temperature conditions: isothermal, 180°C, run time 10 minutes

6.6. Injection volume: 1µL, split 1:40

7. Samples

Samples should be stored at room temperature, away from light and cold.

8. Procedure

8.1. Sample screening for estragole

To ensure that there is no estragole naturally present in the sample, a blank analysis should be carried out without the addition of any internal standard.  If estragole is naturally present then another internal standard must be chosen (for instance menthol).

Pipette 2 mL sample into a 20 mL volumetric flask and make up to volume with 45% vol. ethanol (4.4), mix thoroughly.

8.2. Preparation of unknown samples

Pipette 2 mL sample into a 20 mL volumetric flask then add 2 mL of internal standard solution B (4.5.2) and make up to volume with 45 % vol. ethanol (4.4), mix thoroughly.

8.3. Blank

Pipette 2 mL of internal standard solution B (4.5.2) into a 20 mL volumetric flask and make up to volume with 45 % vol. ethanol (4.4), mix thoroughly.

8.4. Linearity test

Prior to the commencement of the analysis the linearity of the response of the FID should be checked by successively analysing in triplicate each of the linearity standard solutions (4.5.3).

From the integrator peak areas for each injection plot a graph of their mother solution concentration in g/L versus the ratio R for each.

R = trans-anethole peak area divided by the estragole peak area.

A linear plot should be obtained.

8.5. Determination

Inject the blank solution (8.3), followed by standard solution C (4.5.4), followed by one of the linearity standards (4.5.3) which will act as a quality control sample (this may be chosen with reference to the probable concentration of trans-anethole in the unknown), followed by 5 unknowns (8.2); insert a linearity (quality control) sample after every 5 unknown samples, to ensure analytical stability.

9. Calculation of response factor

Measure peak areas (using an integrator or other data system) for trans-anethole and internal standard peaks.

9.1. Response factor (RF_i) calculation

The response factor is calculated as follows

Where:

• is the concentration of trans-anethole in the standard solution A (4.5.1.)
• is the concentration of internal standard in the standard solution B (4.5.2.)
• is the area of the trans-anethole peak
•  is the area of the internal standard peak
• is calculated from the 5 samples of solution C (4.5.4)
  2. Analysis of the linearity response test solutions

Inject the linearity response test solutions  (4.5.3).

9.3. Analysis of the sample

Inject the unknown sample solution (8.2)

10. Calculation of results

The formula for the calculation of the concentration of trans-anethole is the following:

where:

• is the unknown trans-anethole concentration

• is the concentration of internal standard in the unknown (4.5.2)
• is the area of the trans-anethole peak
• is the area of the internal standard peak
• is the response coefficient (calculated as in 9.1)

The trans-anethole concentration is expressed as grams per litre, to one decimal place.

11. Quality assurance and control

The chromatograms should be such that anethole and the internal standard are separated from each other and from any interfering substances.  The RF_i value is calculated from the results for the 5 injections of solution C (4.5.4).  If the coefficient of variation (CV % = (standard deviation/mean)*100)) is within plus or minus 1 %, the RF_i average value is acceptable.

The calculation above should be used to calculate the concentration of trans-anethole in the sample selected for the quality control from the linearity control solutions (4.5.3).

If the mean calculated results from analysis of the linearity solution selected for Internal Quality Control sample (IQC) are within plus or minus 2.5 % of their theoretical value, then the results for the unknown samples can be accepted.

12. Treatment of spirits sample containing large amount of sugar and of liqueur sample prior to GC analysis

Extraction of alcohol from spirit drink containing a large amount of sugar, in order to be able to determine the trans-anethole concentration using capillary gas chromatography.

12.1.       Principle

An aliquot of the liqueur sample is taken and to this is added the internal standard, at a concentration similar to that of the analyte (trans-anethole) in the liqueur. To this are added sodium phosphate dodecahydrate and anhydrous ammonium sulphate. The resulting mixture is well shaken and chilled, two layers develop, and the upper alcohol layer is removed. An aliquot of this alcohol layer is taken and diluted with 45 % ethanol solution (4.4) (Note: no internal standard is added at this stage, because it has already been added). The resulting solution is analysed in gas chromatography.

12.2.       Reagents and materials

During the extraction use only reagents of a purity greater than 99 %.

12.2.1. Ammonium sulphate, anhydrous, (CAS 7783-20-2)

12.2.2. Sodium phosphate, dibasic, dodecahydrate, (CAS 10039-32-4)

12.3.       Apparatus and equipment

Conical flasks, separating flasks, refrigerator.

12.4.       Procedure

12.4.1. Sample screening for estragole

To ensure that there is no estragole naturally present in the sample, a blank extraction (12.6.2) and analysis should be carried out without the addition of any internal standard.  If estragole is naturally present then another internal standard must be chosen.

12.4.2. Extraction

Pipette 5 mL of 96 % ethanol (4.1) into a conical flask, weigh into this flask 50 mg of internal standard (4.3), and add 50 mL of the sample.  Add 12 g of ammonium sulphate, anhydrous (12.2.1), and 8.6 g of dibasic sodium phosphate, dodecahydrate (12.2.2).  Stopper the conical flask.

Shake the flask for at least 30 minutes.  A mechanical shaking device may be used, but not a Teflon coated magnetic stirring bar, as the Teflon will absorb some of the analyte.  Note that the added salts will not dissolve completely.

Place the stoppered flask in a refrigerator  (T< 5^oC) for at least two hours.

After this time, there should be two distinct liquid layers and a solid residue.  The alcohol layer should be clear; if not replace in the refrigerator until a clear separation is achieved.

When the alcohol layer is clear, carefully take an aliquot (e.g. 10 mL), without disturbing the aqueous layer, place in an amber vial and close securely.

12.4.3. Preparation of the extracted sample to be analysed

Allow extract (12.4.2) to reach room temperature.

Take 2 mL of the alcohol layer of the attemperated extracted sample and pipette into a 20 mL volumetric flask, make up to volume with 45 % ethanol (4.4), mix thoroughly.

12.5.       Determination

Follow the procedure as outlined in 8.5.

12.6.       Calculation of results

Use the following formula to calculate the results

Where:

• is the weight of internal standard (4.3.) taken (12.4.2) (in milligrams)
• V is the volume of unknown sample (50 mL)
• is the response factor (9.1.)
• isthe area of the trans-anethole peak
•   is the area of the internal standard peak

The results are expressed in grams per litre, to one decimal place.

12.7.       Quality control and assurance

Follow the procedure as outlined in 11 above.

13. Method performance characteristics (precision)

Statistical results of the interlaboratory test: the following tables give the values for anethole.

The following data were obtained from an international method performance study carried out on a variety of spirit drinks to internationally agreed procedures.

Year of interlaboratory test	1998
Number of laboratories	16
Number of samples	10
Analyte	Anethole

Pastis :

Samples	A	B	C	D	E	F
Number of laboratories retained after eliminating outliers	15	15	15	13	16	16
Number of outlirs (laboratories)	1	1	1	3	-	-
Number of accepted results	30	30	30	26	16	16
Mean value g/l	1,477	1,955	1,940	1,833	1,741	1,754
Repeatability standard deviation (Sr) g/l	0,022	0,033	0,034	0,017	-	-
Repeatability relative Standard deviation (RSDr) (%)	1,5	1,7	1,8	0,9	-	-
Repeatability limit (r)  g/l	0,062	0,093	0,096	0,047	-	-
Reproducibility standard deviation (sR) g/l	0,034	0,045	0,063	0,037	0,058	0,042
Reproducibility relative standard deviation (RSDR) (%)	2,3	2,3	3,2	2,0	3,3	2,4
Reproducibility limit (R) g/l	0,094	0,125	0,176	0,103	0,163	0,119

Sample types:

A pastis, blind duplicates

B pastis, blind duplicates

C pastis, blind duplicates

D pastis, blind duplicates

E pastis, single sample

F, single sample

Other aniseed-flavoured spirit drinks:

Samples	G	H	I	J
Number of laboratories retained after eliminating outliers	16	14	14	14
Number of outliers (laboratories)	-	2	1	1
Number of accepted results	32	28	28	28
Mean value g/l	0,778 0,530*	1,742	0,351	0,599
Repeatability standard deviation (Sr) g/l	0,020	0,012	0,013	0,014
Repeatability relative standard deviation (RSDr) (%)	3,1	0,7	3,8	2,3
Repeatability limit (r) g/l	0,056	0,033	0,038	0,038
Reproducibility standard deviation (SR) g/l	0,031	0,029	0,021	0,030
Reproducibility relative standard deviation (RSDR) (%)	4,8	1,6	5,9	5,0
Reproducibility limit (R) g/l	0,088	0,080	0,058	0,084

Sample types:

G ouzo, split levels (*)

H anis, blind duplicates

I aniseed-flavoured liqueur, duplicates

J aniseed-flavoured liqueur, duplicates

 

14. Bibliography

• Commission Regulation (EC) N° 2091/2002 of 26 November 2002 amending Regulation (EC) No 2870/2000 laying down Community reference methods for the analysis of spirits drinks, OJEC of 27 November 2002, L322/11
• P. Brereton, S. Hasnip, A. Bertrand, R. Wittkowski, C. Guillou, Analytical methods for the determination of spirit drinks, Trends in Analytical Chemistry, Vol. 22, No. 1, 19-25, 2003

OIV-MA-BS-12 Determination of the acidities of spirit drinks of viti-vinicultural origin

 

Type II method

1. Scope

This method is suitable for the determination of the volatile, total, and fixed acidities of spirit drinks of viti-vinicultural origin.

2. Normative References

ISO 3696: 1987: Water for analytical use - Specifications and test methods

3. Definitions

3.1. Volatile acidity is made up of acetic and higher volatile aliphatic acids that are present in spirit drinks.

3.2. Total acidity is the sum of titratable acidities.

3.3. Fixed acidity is the acidity of the residue left after evaporating the spirit drink to dryness.

4. Principle

The total acidity is determined by direct titration of the sprit drink.  The fixed acidity is determined by titration of the aqueous solution obtained after dissolving the residue from evaporation of the spirit drink.  The volatile acidity is calculated by deducting the fixed acidity from the total acidity.

5. Reagents and Materials

During the analysis, unless otherwise stated, use only reagents of recognised analytical grade and water of at least grade 3 as defined in ISO 3696:1987

5.1. 0.05 M sodium hydroxide solution

5.2. Mixed indicator solution:

Weigh 0.1 g of indigo carmine and 0.1 g of phenol red.

Dissolve in 40 mL water and make up to 100 mL with ethanol.

6. Apparatus and Equipment

Standard laboratory apparatus, “A” grade volumetric glassware and, in particular, the following:

6.1. Equipment for applying vacuum (water pump, vacuum flask, etc.), or other system for eliminating carbon dioxide (bubbling or other).

6.2. Flat-bottomed stainless-steel cylindric capsule, of sufficient dimensions to avoid loss of liquid when evaporating.

6.3. Equipment for potentiometric titration (optional).

7. Sampling and samples

Samples are stored at room temperature prior to analysis.

8. Procedure

8.1 Total acidity

8.1.1.    Preparation of sample

If necessary, the spirit is stirred for at least two minutes under vacuum to remove carbon dioxide, or the latter is eliminated by any other convenient method.

8.1.2.    Titration

Pipette 25 mL of the spirit into a 500 mL conical flask.

Add about 200 mL of cooled boiled distilled water (freshly prepared) and 2-6 drops of the mixed indicator solution (5.2).

Titrate with the 0.05 M sodium hydroxide solution (5.1) until the yellow-green colour changes to violet in the case of colourless spirit drinks, or the yellow-brown colour to red-brown in the case of brown-coloured spirit drinks.

The titration may also be carried out by potentiometry, to pH 7.5.

Let n₁ mL be the volume of the 0.05 M sodium hydroxide solution added.

8.1.3.    Calculation

• The total acidity (TA) expressed in milliequivalents per L of spirit drink is equal to 2 x n₁.
• The total acidity (TA’) expressed in mg of acetic acid per L of spirit drink is equal to 120 x n₁.
• The total acidity (TA’) expressed in g of acetic acid per hL of pure 100 % vol alcohol is equal to 120 x n₁ x 10/A, where A is the alcoholic strength by volume of the spirit drink.

8.2. Fixed acidity

8.2.1.    Preparation of sample

Pipette 25 mL (or a larger volume if the fixed acidity is very low) of the spirit drink into a flat-bottomed cylindrical evaporating dish (6.2). During the first hour of evaporation the evaporating dish is placed on the lid of a boiling water bath so that the liquid will not boil, as this could lead to losses through splattering.

If necessary, complete the drying by placing the evaporating dish in a drying oven at 105 °C for two hours. Allow the evaporating dish to cool in a desiccator.

8.2.2.    Titration

Take up the residue left after evaporating with cooled boiled distilled water (freshly prepared), make up to a volume of about 100 mL and add 2-6 drops of the mixed indicator solution (5.2).

Titrate with the 0.05 M sodium hydroxide solution (5.1) until the yellow-green colour changes to violet if the solution is colourless, or the yellow-brown colour to red-brown if the solution is brown-coloured.

The titration may also be carried out by potentiometry, to pH 7.5.

Let n₂ mL be the volume of the 0.05 M sodium hydroxide solution added, and V mL the volume of sample evaporated.

8.2.3.    Calculation

• The fixed acidity (FA) expressed in milliequivalents per L of spirit drink is equal to 2 x x 25/V.
• The fixed acidity (FA’) expressed in mg of acetic acid per L of spirit drink is equal to 120 x x 25/V.
• The fixed acidity (FA’) expressed in g of acetic acid per hL of pure 100% vol alcohol is equal to 120 x x 25/V x 10/A, where A is the alcoholic strength by volume of the spirit drink.

8.3. Calculation of volatile acidity

8.3.1.    Expression in milliequivalents per L :

Let:

• TA = total acidity in milliequivalents per L
• FA = fixed acidity in milliequivalents per L
• Volatile acidity,VA, in milliequivalents per L is equal to :
• TA - FA

8.3.2.    Expression in mg of acetic acid per L:

Let:

• TA^’ = total acidity in mg of acetic acid per L

 FA^’ = fixed acidity in mg of acetic acid per L

• Volatile acidity,VA, in mg of acetic acid per L is equal to :
• TA‘ - FA’

8.3.3.    Expression in g of acetic acid per hL of pure 100 % vol alcohol is equal to :

• where A is the alcoholic strength by volume of the spirit drink.

9. Method performance characteristics (Precision)

The following data were obtained in 2000 from an international method-performance study on a variety of spirit drinks, carried out following internationally-agreed procedures.

Key to the tables below:

nLT	Number of laboratories (2 results per laboratory)
nL	Number of laboratories to calculate precision values
r	repeatability limit
Sr	repeatability standard deviation
RSDr	repeatability standard deviation expressed in % of the level
R	reproducibility limit
SR	reproducibility standard deviation
RSDR	reproducibility standard deviation expressed in % of the level
PRSDR	RSDR predicted with the Horwitz formula (%)
HoR	HorRat value = RSDR / PRSDR
SH240	Aqueous-alcoholic solution: acetic acid (240 mg/L), tartaric  acid (200 mg/L), sucrose (10 g/L)

All the acidities are expressed as mg of acetic acid per L of spirit drink.

9.1. Total acidity

	nLT	nL	Mean (mg/L)	r (mg/L)	Sr (mg/L)	RSDr (%)	R (mg/L)	SR (mg/L)	RSDR (%)	PRSDR (%)	HoR
Rum 1	18	18	53	8	2,7	5,1	34	12	23	8,8	2,6
Slibowitz	18	17	55	10	3,7	6,7	19	6,6	12	8,8	1,4
Brandy	20	18	193	16	5,7	2,9	43	15	7,9	7,2	1,1
Brandy	18	18	194	16	5,8	3,0	38	13	6,9	7,2	1,0
Calvados	18	17	282	21	7,5	2,7	34	12	4,3	6,8	0,6
SH240	20	17	400	14	4,9	1,2	18	6,2	1,6	6,5	0,2
Marc	18	18	547	16	5,8	1,1	42	15	2,7	6,2	0,4
Armagnac	20	19	580	27	9,4	1,6	53	19	3,2	6,1	0,5
Rum 2	18	18	641	41	14,3	2,2	66	23	3,7	6,0	0,6

9.2. Fixed acidity

	nLT	nL	Mean (mg/L)	r (mg/L)	Sr (mg/L)	RSDr (%)	R (mg/L)	SR (mg/L)	RSDR (%)	PRSDR (%)	HoR
Slibowitz	18	16	9,5	5,1	1,8	19	14	4,9	52	11	4,6
Rum 1	18	18	22	6,1	2,2	9,7	28	10	45	10	4,5
Calvados	18	16	25	7,7	2,7	10,8	24	8,4	34	9,9	3,4
Rum 2	18	18	25	5,7	2,0	7,9	28	9,9	39	9,8	4,0
Marc	18	17	51	25	8,8	17	60	21	42	8,8	4,7
Brandy	18	18	87	17	6,0	6,9	47	17	19	8,2	2,3
Brandy	20	19	89	12	4,2	4,7	33	12	13	8,1	1,6
Armagnac	20	19	159	13	4,7	2,9	80	28	18	7,5	2,4
SH240	20	17	162	12	4,1	2,5	32	11	7,1	7,4	1,0

9.3. Volatile acidity

	nLT	nL	Mean (mg/L)	r (mg/L)	Sr (mg/L)	RSDr (%)	R (mg/L)	SR (mg/L)	RSDR (%)	PRSDR (%)	HoR
Rum 1	18	18	30	10	3,5	12	24	8,4	28	9,6	2,9
Slibowitz	18	14	46	10	3,7	8,1	13	4,6	10	9,0	1,1
Brandy	20	18	107	23	8,0	7,5	44	16	15	7,9	1,8
Brandy	18	18	107	19	6,6	6,2	38	13	13	7,9	1,6
SH240	20	17	242	21	7,2	3,0	48	17	6,9	7,0	1,0
Calvados	18	16	257	23	8,0	3,1	24	8,5	3,3	6,9	0,5
Armagnac	20	17	418	22	7,8	1,9	62	22	5,2	6,5	0,8
Marc	18	18	492	24	8,5	1,7	69	24	5,0	6,3	0,8
Rum 2	18	18	616	42	15	2,4	71	25	4,1	6,1	0,7

10. Bibliography

• R. Wittkowski, A. Bertrand, P. Brereton, C. Guillou, 2000. PROJECT SMT4-CT96-2119, Validation of analytical methods of analysis for spirit drinks. REPORT NO. 02/08- WORKSTREAM 8
• P. Brereton, S. Hasnip, A. Bertrand, R. Wittkowski, C. Guillou, Analytical methods for the determination of spirit drinks, Trends in Analytical Chemistry, Vol. 22, No. 1, 19-25, 2003
• FV 1322 (2009), Measurement of acidities in spirits - estimation of precision

OIV-MA-BS-11 Determination of sugars in spirit drinks of viti-vinicultural origin

Type II method

Introduction

Spirit drinks of viti-vinicultural origin may be sweetened by various compounds, and in certain legislations the concentrations of sweetener are subject to minimum or maximum levels.

1. Scope

This method is suitable for the determination of the glucose, fructose, and sucrose contents of spirit drinks of viti-vinicultural origin. It is not suitable for spirit drinks containing dairy products or eggs.

 

2. Normative References

ISO 3696:1897 Waters for analytical use - Specifications and test methods.

 

3. Principle

High performance liquid chromatography (HPLC) to determine the glucose, fructose, and sucrose concentrations. 

This method is described as an example.  It uses an alkylamine stationary phase and differential refractometry detection.  Other columns/detectors may be used, for example anion exchange resins as the stationary phase.

4. Reagents and Materials
   1. Glucose (CAS 50-99-7), at least 99 % pure.
   2. Fructose (CAS 57-48-7), at least 99 % pure.
   3. Sucrose (CAS 57-50-1), at least 99 % pure.
   4. Pure acetonitrile (CAS 75-05-8) for HPLC analysis.

Acetonitrile is a highly flammable liquid.  It is toxic by inhalation, in contact with skin and if swallowed.  It is irritating to eyes. 

4.5. Distilled or demineralised water, preferably micro-filtered.

4.6. Solvents (example)

The elution solvent is prepared beforehand by mixing:

• 75 parts by volume of acetonitrile (4.4),
• 25 parts by volume of distilled or demineralised water (4.5).

Pass helium through at a slow rate for 5 - 10 minutes prior to use to degas.

If the water being used has not been micro-filtered, it is advisable to pass the solvent through a filter for organic solvents with a pore size less than or equal to 0.45 μm.

4.7. Ethanol, absolute (CAS 64-17-5). 

4.8. Ethanol solution (5 %, v/v). 

4.9. Preparation of stock standard solution (20 g/L)

Weigh 2 g each of the sugars to be analysed (4.1 to 4.3), transfer them without loss to a 100 mL volumetric flask.  Adjust to 100 mL with a 5 % vol. alcohol solution (4.8), shake and store at around +4 °C.  Prepare a new stock solution once a week if necessary.

4.10.       Preparation of working standard solutions (2.5, 5.0, 7.5, 10.0 and 20.0 g/L)

Dilute the stock solution, 20 g/L, (4.9) appropriately with a 5% vol. alcohol solution (4.8) to give five working standards of 2.5, 5.0, 7.5, 10.0 and 20.0 g/L.  Filter with a filter of a pore size less than or equal to 0.45 µm (5.3.).

5. Apparatus and Equipment (as an example - other systems that provide equivalent performance can be used)

Standard laboratory apparatus, “A” grade volumetric glassware and, in particular, the following:

5.1. HPLC system capable of achieving baseline resolution of all of the sugars.

5.1.1.    High-performance liquid chromatograph with a six-way injection valve fitted with a 10 µL loop or any other device, whether automatic or manual, for the reliable injection of micro-volumes.

5.1.2.    Pumping system enabling one to achieve and maintain a constant or programmed rate of flow with great precision.

5.1.3.    Differential refractometer.

5.1.4.    Computational integrator or recorder, the performance of which is compatible with the rest of the set-up.

5.1.5.    Pre-column:

It is recommended that a suitable pre-column is attached to the analytical column.

5.1.6.    Column (example):

Material: stainless steel or glass

Internal diameter: 2-5 mm

Length: 100-250 mm (depending on the packing particle size), for example 250 mm if the particles are 5 µm in diameter

Stationary phase: cross-linked silica with radicals containing the alkylamine functional group, maximum particle size 5 µm.

5.1.7.    Chromatography conditions (example):

Elution solvent (4.6), flow rate: 1 mL/minute

Detection: Differential refractometry

To make certain that the detector is perfectly stable, it may be advisable to switch it on a few hours before use.  The reference cell must be filled with the elution solvent.

5.2. Analytical balance accurate to 0.1  mg.

5.3. Filtration equipment for small volumes using a 0.45 µm membrane.

 

6. Sample storage

On receipt, samples are to be stored at room temperature prior to analysis.

7. Procedure
   1. PART A: Sample Preparation
      1.     Shake the sample.
      2.     Filter the sample through a filter with a pore size less than or equal to 0.45 µm (5.3).
   2. PART B: HPLC
      1.     Determination

Inject 10 µL of the standard solutions (4.10) and samples (7.1.2.). Perform the analysis under suitable chromatography conditions, for example those described above.

7.2.2.    Should any peak of a sample have a greater area (or height) than the corresponding peak in the most concentrated standard, then the sample should be diluted with distilled or demineralised water and re-analysed.

 

8. Calculation

Compare the two chromatograms obtained for the standard solution and spirit.  Identify the peaks by their retention times.  Measure their areas (or heights) to calculate the concentrations by the external standard method.  Take into account any dilutions made to the sample.

The final result by convention is the sum of sucrose,  glucose, and fructose, in g/L.

9. Method performance characteristics (Precision)

The following data were obtained in 2000 from an international method- performance study carried out on a variety of spirit drinks, following internationally-agreed procedures.

Key to the tables below:

nLT	Number of laboratories (2 results per laboratory)
nL	Number of laboratories to calculate precision values
r	repeatability limit
Sr	repeatability standard deviation
RSDr	repeatability standard deviation expressed in % of the level
R	reproducibility limit
SR	reproducibility standard deviation
RSDR	reproducibility standard deviation expressed in % of the level
PRSDR	RSDR predicted with the Horwitz formula (%)
HoR	HorRat value = RSDR / PRSDR

9.1. Glucose

	nLT	nL	Mean (mg/L)	r (mg/L)	Sr (mg/L)	RSDr (%)	R (mg/L)	SR (mg/L)	RSDR (%)	HoR
Liqueur 1	26	24	92,4	5,4	1,9	2,1	13	4,8	5,2	1,8
Liqueur 2	24	23	93,2	9,7	3,5	3,7	28	10	11	3,8

 

9.2. Fructose

	nLT	nL	Mean (mg/L)	r (mg/L)	Sr (mg/L)	RSDr (%)	R (mg/L)	SR (mg/L)	RSDR (%)	HoR
Liqueur 1	26	22	87	3,2	1,2	1,3	8,5	3,0	3,5	1,2
Liqueur 2	24	21	93	6,6	2,3	2,5	22	7,7	8,3	2,9

 

9.3. Saccharose

	nLT	nL	Mean (mg/L)	r (mg/L)	Sr (mg/L)	RSDr (%)	R (mg/L)	SR (mg/L)	RSDR (%)	HoR
Liqueur 1	26	24	174	12	4,2	2,4	24	8,7	5,0	1,9
Liqueur 2	24	18	320	12	4,3	1,3	45	16	5,0	2,1
Liqueur 3	24	18	349	22	8,0	2,3	30	11	3,1	1,3
Pastis	24	19	11	0,2	0,1	0,8	2,2	0,8	7,3	1,9
Ouzo	24	19	24	2,1	0,8	3,1	2,6	0,9	3,8	1,1
Kirsch	24	20	103	6,1	2,2	2,1	12	4,2	4,0	1,4

 

9.4. Sucres totaux

	nLT	nL	Mean (mg/L)	r (mg/L)	Sr (mg/L)	RSDr (%)	R (mg/L)	SR (mg/L)	RSDR (%)	HoR
Liqueur 1	26	21	353	8,7	3,1	0,9	41	15	4,2	1,8
Liqueur 2	24	18	510	16	5,6	1,1	41	15	2,9	1,3
Liqueur 3	24	18	349	22	8,0	2,3	30	11	3,1	1,3
Pastis	24	20	11	0,4	0,1	1,2	2,2	0,8	7,3	1,8
Ouzo	24	19	24	2,1	0,8	3,1	2,6	0,9	3,8	1,1
Kirsch	24	20	103	6,1	2,2	2,1	12	4,2	4,0	1,4

 

10. Bibliography

• R. Wittkowski, A. Bertrand, P. Brereton, C. Guillou, 2000. PROJECT SMT4-CT96-2119, Validation of analytical methods of analysis for spirit drinks. REPORT NO. 02/09 - WORKSTREAM 10.
• P. Brereton, S. Hasnip, A. Bertrand, R. Wittkowski, C. Guillou, Analytical methods for the determination of spirit drinks, Trends in Analytical Chemistry, Vol. 22, No. 1, 19-25, 2003.

OIV-MA-BS-22 Determination by isotope ratio mass spectrometry of the ¹³C/¹²C ratio of wine ethanol of spirit drinks of viti-vinicultural origin

Type II method

1. Field of application

The method enables the measuring of the ¹³C/¹²C isotope ratio of the ethanol of spirit drinks of vitivinicultural origin.

2. Reference standards

ISO 5725 :1994 «Accuracy (trueness and precision) of measurement methods and results: Basic method for the determination of repeatability and reproducibility of a standard measurement method»

V-PDB : Vienna-Pee-Dee Belemnite (R_PDB = 0.0112372).

Method OIV «Detection of enriching musts, concentrated musts, grape sugar and wine by application of nuclear magnetic deuterium resonance (SNIF-NMR)»

3. Terms and definitions

 

¹³C/¹²C : Carbon 13 and carbon 12 isotope ratio for a given sample

δ¹³C : Carbon 13 contents (¹³C) expressed in parts per 1000 (‰)

SNIF-NMR: Site-specific natural isotope fractionation studied by nuclear magnetic resonance

V-PDB : Vienna-Pee-Dee Belemnite. or PDB, is the main reference for measuring natural variations of carbon 13 isotopic contents. Calcium carbonate comes from a Cretaceous belemnite from the Pee Dee formation in South Carolina (USA). Its isotopic ratio ¹³C/¹²C or R_{PDB is} R_PDB = 0.0112372. PDB reserves have been exhausted for a long time, but it has remained the primary reference to express natural variations of Carbon 13 isotopic contents. Reference material is calibrated based on this content and is available at the International Agency of Atomic Energy (IAEA) in Vienna (Austria). The isotopic indications of naturally occurring carbon 13 are expressed by V-PDB, as is the custom.

m/z:Mass to charge ratio

 

4. Principle

During photosynthesis, the assimilation of carbon dioxide by plants occurs according to 2 principle types of metabolism that are: metabolism C₃ (Calvin cycle) and C₄ (Hatch and Slack). These two means of photosynthesis present a different type of isotope fractionation. Products, such as sugars and alcohol, derived from C₄ plants and fermentation, have higher levels of Carbon 13 than from C₃ plants. Most plants, such as vines and sugar beet belong to the C₃ group. Sugar cane and corn belong to the C₄ group. Measuring the carbon 13 content enables the detection and the quantification of C₄ (sugar cane or corn isoglucose) origin sugars which are added to products derived from grapes (grape musts, wines). The combined information on carbon 13 content and information obtained from SNIF-NMR enable the quantification of mixed sugars added or alcohol of plant origin C₃ and C₄.

The carbon 13 content is determined on carbon dioxide resulting from the complete combustion of the sample. The abundance of the main mass isotopomers 44 (¹²C¹⁶O₂), 45 (¹³C¹⁶O₂ et ¹²C¹⁷O¹⁶O) and 46 (¹²C¹⁶O¹⁸O), resulting from different possible combinations of isotopes ¹⁸O, ¹⁷O, ¹⁶O, ¹³C et ¹²C, are determined from ion currents measured by three different collectors of isotopic mass spectrometers. The contributions of isotopomers ¹³C¹⁷O¹⁶O et ¹²C¹⁷O₂ can be neglected because of their low abundance. The ion current for m/z = 45 is corrected for the contribution of ¹²C¹⁷O¹⁶O which is calculated according to the current intensity measured for m/z = 46 while considering the relative abundance of ¹⁸O and ¹⁷O (Craig adjustment). The comparison with the calibrated reference and the international reference V-PDB enable the calculation of carbon 13 content on a relative scale of δ¹³C.

5. Reagents

The material and the consumables depend on the apparatus (6) used by the laboratory. The systems generally used are based on elementary analysers. These systems can be equipped to introduce the samples placed in sealed metal capsules or for the injection of liquid samples through a septum using a syringe.

Depending on the type of instrument used, the reference material, reagents, and consumables can be used:

• Reference material available from the  IAEA:

Name	Material	δ13C   versus V-PDB (9)
-IAEA-CH-6	saccharose	-10,4 ‰
-IAEA-CH-7	polyethylene	-31,8 ‰
- NBS22	oil	-29,7 ‰
- USGS24	graphite	-16,1 ‰

• Available from the IRMM in Geel (B) (Institut des Matériaux et Mesures de Référence) :

Name	Material	δ13C  versus V-PDB (9)
- CRM 656	Wine alcohol	-26,93 ‰
- CRM 657	glucose	-10,75 ‰
- CRM 660	Aqueous alcoholic solution (ABV 12%)	-26,72 ‰

Standard working standard with a known ¹³C/¹²C ratio calibrated with international reference materials.

A standard list of consumables established for continuous flow systems follows below:

• Helium for analysis (CAS 07440-59-7)
• Oxygen for analysis (CAS 07782-44-7)
• Carbon dioxide for analysis, used as a secondary reference gas for the content of carbon13 (CAS 00124-38-9)
• Oxidation reagent for the oven and the combustion system as follows: copper oxide (II) for elementary analysis (CAS 1317-38-0)
• Drying agent to eliminate water produced by combustion. For example: anhydrone for elementary analysis (magnesium perchlorate) (CAS 10034-81-8).

This is not necessary for apparatus equipped with a water elimination system by cryo-trapping or through selective permeable capillaries.

 

6. Apparatus and materials

6.1. Isotope ratio mass spectrometry (IRMS)

Isotope ratio mass spectrometry (IRMS) enables the determination of the relative contents of ¹³C of naturally occurring CO₂ gas with an internal accuracy of 0.05‰ or expressed in relative value (9). Internal accuracy here is defined as the difference between 2 measurements of the same sample of CO₂.  The mass spectrometer used to measure isotope ratios is generally equipped with a triple collector to simultaneously measure m/z = 44, 45 and 46 intensities. The isotope ratio mass spectrometry must either be equipped with a double introduction system to alternately measure the unknown sample and a reference sample, or use an integrated system that carries out quantitative combustion on samples and separates the carbon dioxide from the other combustion products before measuring the mass spectrum.

6.2. Combustion apparatus

Combustion apparatus able to quantitatively convert ethanol into carbon dioxide and capable of eliminating all other combustion products including water, without any isotopic fractionation. The apparatus can be either an integrated continuous flow system integrated with mass spectrometry (6.2.1), of an autonomous combustion system (6.2.2). The apparatus must be as precise as indicated in (11).

 

6.2.1.    Continuous flow systems 

These consist of either an elemental analyser, or a gas chromatograph equipped with an online combustion system.

The following laboratory material is used for systems equipped for the introduction of samples contained in metallic capsules :

• volumetric micropipette with appropriate cones
• balance with  1 μg accuracy or better
• tool for capsule sealing
• tin capsules for liquid samples
• tin capsules for solid samples

The following laboratory material is needed when using an elemental analyser equipped with a liquid injector or in the case of a preparation system for combustion chromatography:

• syringe for liquids
• flasks equipped with sealed closing system and inert septa

The laboratory materials indicated in the lists are examples that are susceptible of being replaced by other equivalent performance material depending on the type of combustion apparatus and of mass spectrometry used by the laboratory.

6.2.2.    Separate preparation systems

In this case the samples of carbon dioxide resulting from the combustion of samples to be analyzed and the reference sample are collected in ampoules which are then put in a double entry spectrometer system to carry out isotopic analyses. Several types of combustion apparatus described in the literature can be used:

• Closed combustion system filled with circulating oxygen gas
• Elemental analyser with helium and oxygen flows
• Sealed glass ampoule filled with copper oxide (II) used as an oxidation agent

7. Preparation of samples for tests

Ethanol must be extracted from the spirit drink before isotopic testing. This is carried out by distilling the beverage as described in §3.1 of the SNIF-NMR method for the determination by NMR of the deuterium distribution in the ethanol of spirit drinks of vitivinicultural origin.

8. Procedure

All preparation steps must be carried out without any significant ethanol loss through evaporation, which would change the isotopic composition of the sample.

The description that follows makes reference to the procedure generally used for ethanol sample combustion using commercial automatic combustion systems. All other methods, ensuring that ethanol samples are converted quantitatively into carbon dioxide without the evaporation of ethanol, can use the preparation of carbon dioxide for isotopic analyses.  An experimental procedure based on the use of an elemental analyser:

a)      Placing the samples in capsules

• use capsules, tweezers and a clean preparation tray
• take an appropriate sized capsule using tweezers
• introduce an appropriate amount of liquid into the capsule using a micropipette

 

Note: 3.84 mg of absolute ethanol or 4.17 mg of distillate with an alcohol content of 92 % m/m are necessary to obtain 2 mg of carbon. The appropriate quantity of distillate must be calculated in the same way according to the quantity of carbon necessary based on the mass spectrometer’s sensitivity.

• close the capsule with the sealing tool.
• each capsule must be completely sealed. If not, it must be discarded and a new  capsule must be prepared.
• two capsules must be prepared for every sample
• place the capsules in an appropriate place on the elemental analyser sample tray. Every capsule must be carefully identified in order by number.
• systematically place capsules containing working references at the beginning and the end of  the sample series
• regularly insert a check sample in the sample series.

b)      check and adjust the elemental analysis and mass spectometry instrumentation

• adjust the temperature of the elemental analyzer ovens and the helium and oxygen gas flow for an optimal combustion of the sample;
• check the elemental analysis system and the mass spectometry system for leaks (for example by checking the ion current where m/z = 28 corresponds to N₂);
• adjust the mass spectrometer to measure the ion current intensities for m/z = 44, 45 and 46;
• check the system using known reference samples before starting to measure the samples.

c)      To carry out a series of measurements

The samples that are placed on the autosampler of the elemental analyser or chromatographare introduced successively. The carbon dioxide for each sample combustion is eluted into the mass spectrometer which measures the ion current. The data system records the ion current intensities and calculates the  values for each sample (9).

9. Calculation

The objective of the method is to measure the ¹³C/¹²Cisotopic ratio of the ethanol extracted from spirit drinks. The ¹³C/¹²Cisotopic ratio can be expressed by its deviation compared to the reference work. The carbon 13 (δ ¹³C) isotopic ratio is calculated on a delta scale per thousand by comparing the results obtained for the sample to be measured to the working reference calibrated previously based on the primary international reference (V-PDB).  The  ¹³C values are expressed compared to the working reference:

where R_ech and R_ref are respectively the isotopic ratio¹³C/¹²C of the sample and the working reference.

The δ ¹³C values are thus expressed using V-PDB:

where δ¹³C_ref/V-PDB is the isotopic deviation determined beforehand for the working reference to V-PDB.

Small variations may occur while measuring on line due to changes in the instrumental conditions. In this case the  ¹³C samples must be corrected according to the difference in the ¹³C value from the working reference and the real value, which was calibrated beforehand against V-PDB by comparison with one of the international reference materials.Between two measurements of the working reference, the variation and therefore the correction applied to the sample results may be assumed to be linear. The working reference must be measured at the beginning and at the end of all sample series. A correction can then be calculated for each sample using linear interpolation between the two values (the difference between the assigned value of the working reference and the measurement values obtained).

10. Quality assurance and control

Check that the ¹³C value for the working reference does not differ by more than 0.5‰ of the accepted value. If not, the spectrometer must be checked and possibly readjusted.

For each sample, verify that the difference in the results between the 2 capsules measured successively is under 0.3 ‰. The final result for a given sample is the average value of the 2 capsules. If the deviation is higher than 0.3 ‰ the measurement should be repeated.

Measurement condition monitoring can be based on the ion current intensity for m/z = 44 and is proportional to the quantity of carbon injected in the elemental analyzer. Under standard conditions, the ion current intensity should be almost constant for the samples analysed. A significant deviation could be indicative of ethanol evaporation (an imperfect seal on a capsule), an instability of the elemental analyser, or the mass spectrometer.

 

11. Method performance characteristics (precision)

One collaborative analysis (11.1) was carried out on distillates containing alcohol of vinous origin, and cane and beet alcohol, in addition to different mixtures of these three origins. This study did not take into account the distillation step, and further information from other joint laboratory studies on wine (11.2) and in particular proficiency testing (11.3) for isotopic measurements have also been considered. The results show that different distillation systems under satisfactory conditions, and in particular those used for SNIF-NMR measurements, do not have significant variability for determining the δ¹³C of ethanol in wine. It is reasonable to suppose that this would likewise be true for the ethanol of spirit drinks. The precision parameters observed for wine are almost identical to those obtained in the joint study on distillates (11.1).

11.1.       Joint study on distillates

Year of inter laboratory study	1996
Number of laboratories	20
Number of samples	6 samples in double-blind comparison
Analysis	ethanol  13C

Sample code	Vinous origin alcohol	Beet alcohol	Sugar cane alcohol
A & G	80%	10%	10%
B & C	90%	10%	0%
D & F	0%	100%	0%
E & I	90%	0%	10%
H & K	100%	0%	0%
J & L	0%	0%	100%

Samples	A / G	B / C	D / F	E / I	H / K	J / L
Number of laboratories retained after eliminating  anomalous results	19	18	17	19	19	19
Number of results accepted	38	36	34	38	38	38
Average value (δ 13C) ‰	-25.32	-26.75	-27.79	-25.26	-26.63	-12.54
Sr2	0.0064	0.0077	0.0031	0.0127	0.0069	0.0041
Repeatability standard deviation (Sr) ‰	0.08	0.09	0.06	0.11	0.08	0.06
Repeatability limit r (2.8×Sr) ‰	0.22	0.25	0.16	0.32	0.23	0.18
SR2	0.0389	0.0309	0.0382	0.0459	0.0316	0.0584
Reproducibility standard deviation (SR) ‰	0.20	0.18	0.20	0.21	0.18	0.24
Reproducibility limit R (2,8× SR) ‰	0.55	0.9	0.55	0.60	0.50	0.68

11.2.       Inter laboratory study on two wines and one alcohol

Year of inter laboratory trial:	1996
Number of laboratories	14 for distillation of wine and 7 for also measuring the  13C of ethanol in wine 8 for measuring the δ 13C in the alcohol sample
Number of samples	3 (White wine ABV 9.3 % vol., white wine ABV 9.6 % and alcohol of strength 93% m/m)
Analysis	ethanol δ13C

Samples	Red wine	White wine	Alcohol
Number of laboratories	7	7	8
Number of accepted results	7	7	8
Average value (δ 13C) ‰	-26.20	-26.20	-25.08
Reproducibility variance SR2	0.0525	0.0740	0.0962
Reproducibility standard deviation (SR) ‰	0.23	0.27	0.31
Reproducibility limit R (2.8× SR) ‰	0.64	0.76	0.87

Different distillation systems were used by the participating laboratories. The  ¹³C isotopic determinations carried out in one laboratory on all of the distillates

returned by the participants, did not reveal any anomalous values or significantly distinct average values. The variation in results (S² = 0.0059) is comparable to repeatability variances Sr² from the collaborative study on distillates (11.1).

11.3.       Results from proficiency-testing studies

Since December 1994 international proficiency testing to determine the isotopic measurements for wine and alcohol (ABV of distillates 96 % vol.) have been organized regularly. The results enable participating laboratories to check the quality of their analyses. Statistical results enable an appreciation of the variability of derterminations under reproducibility conditions. This enables an estimation  of the variance parameters and the reproducibility limit. The results obtained for the wine and ethanol distillate  ¹³C determinations are summarized in the table below:

Wines					Distillates
Date	N	SR	S2R	R	N	SR	S2R	R
Dec. 1994	6	0,210	0,044	0,59	6	0,151	0,023	0,42
June 1995	8	0,133	0,018	0,37	8	0,147	0,021	0,41
Dec. 1995	7	0,075	0,006	0,21	8	0,115	0,013	0,32
March 1996	9	0,249	0,062	0,70	11	0,278	0,077	0,78
June 1996	8	0,127	0,016	0,36	8	0,189	0,036	0,53
Sept. 1996	10	0,147	0,022	0,41	11	0,224	0,050	0,63
Dec. 1996	10	0,330	0,109	0,92	9	0,057	0,003	0,16
March 1997	10	0,069	0,005	0,19	8	0,059	0,003	0,16
June 1997	11	0,280	0,079	0,78	11	0,175	0,031	0,49
Sept 1997	12	0,237	0,056	0,66	11	0,203	0,041	0,57
Dec. 1997	11	0,127	0,016	0,36	12	0,156	0,024	0,44
March 1998	12	0,285	0,081	0,80	13	0,245	0,060	0,69
June 1998	12	0,182	0,033	0,51	12	0,263	0,069	0,74
Sept 1998	11	0,264	0,070	0,74	12	0,327	0,107	0,91
Weighted average		0,215	0,046	0,60		0,209	0,044	0,59

N: number of participating laboratorie

12. Bibliography

 

• Determination by NMR of the distribution of deuterium in ethanol of spirit drinks of vitivinicultural origin
• OIV Compendium of international methods of analysis of spirit drinks of vitivinicultural origin.
• Determination by isotopic mass spectrometry of the ¹³C/ ¹²C isotopic ratio of wine ethanol or ethanol obtained from fermentation of musts, concentrated musts or grape sugar
• OIV Compendium of International Methods of Analysis of Wine and Musts. Detecting enrichment of musts, concentrated musts, grape and wine sugars by application of nuclear magnetic resonance of deuterium  (RMN-FINS/SNIF-NMR)
• E.C. Regulation. Community analytical methods which can be applied in the wine sector, N°.2676/90.  Detecting enrichment of grape musts, concentrated grape musts, rectified concentrated grape musts and wines by application of nuclear magnetic resonance of deuterium (SNIF-NMR)
• Official Journal of the European Communities, NoL 272, Vol 33, 64-73, 3 October 1990
• Inter-laboratory study about the determination of ¹³C in wine ethanol OIV FV No 1051
• Fidelité de la determination du rapport isotopique ¹³C/¹²C de l’éthanol du vin OIV FV No 1116.
• Stable carbon isotope content in ethanol of EC data bank wines from Italy, France and Germany. A Rossmann ; H-L Schmidt ; F. Reniero ; G. Versini ; I. Moussa ; M.- H. Merle. Z. Lebensm. Unters. Forsch., 1996, 203, PP. 293-301.

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OIV-MA-BS-06 Density of alcohols and alcoholic beverages method for determining electronic densimetry (principle based on measuring the period of oscillation)

 

Type IV method

 

1. Introduction

This method for determining the density of neutral alcohols and alcoholic beverages is based on the change in oscillation frequency in relation to the change in mass based on calibration with two fluids of known density.

Electronic densimeters with digital displays are commercially available to perform this determination.

2. Object and scope of application

The purpose of this document is to describe a method for determining the density of alcohols and alcoholic beverages at atmospheric pressure.

The application of the method is restricted to products with a vapour pressure of less than 800 hectoPascal (600 mmHg) and a viscosity of less than approximately 15,000 m2/s (I m/s = 1 cSt) at the test temperature.

With reference to the currently applicable regulations, the test temperature is set to: 20°C.

3. Density

The density of a liquid at a given temperature is equal to its mass divided by its volume:

It is expressed in kilograms per cubic meter (kg/m³) at a temperature of 20 degrees Celsius (°C) for alcohols and alcoholic beverages.

Note: electronic densimeters display results expressed in grams per cubic centimetre which may be converted into kilograms per cubic meter.

4. Principle

4.1. A liquid sample of a few millilitres is introduced into a vibrating measuring tube.

Measuring the period of oscillation of the tube containing the sample determines the density of the sample at the test temperature, using a previously calibrated apparatus.

4.2. Principle of vibrating measuring tube.

Figure 1: Vibrating measuring tube

Electronic densimeters operate according to the vibrating measuring tube principle (fig. 1): the fluid is introduced into a U-shaped tube and subjected to electromagnetic excitation (fig. 2 and fig. 3).

 

Figure 2: Reactive forces exerted by the fluid

 

The induced period of oscillation is thus proportional to the total mass subject to vibration and can be used to determine the density of the sample based on the following equation:

Figure 3: Resulting torsion

• where T = induced period of vibration
• M = mass of the empty tube
• V = volume of the oscillated sample
• C = spring constant
• p = density of the sample

4.3. Detailed principle.

The density of the liquids is determined by the electronic measurement of the oscillations of a vibrating U-shaped tube.

To carry out this measurement, the sample is introduced into an oscillating system, whose specific frequency is thus modified by the mass of the substance introduced.

The system comprises an undamped U-shaped vibration tube, subject to electronic excitation. The two straight sections of the U-shaped tube act like a spring mechanism. The oscillatory movements occur perpendicular to the U. The filling capacity, V, is delimited by the two fastening points. If the oscillator contains the volume established as V, the latter vibrates within and with the tube. It is accepted that the mass is proportional to the density. Since filling the tube beyond the fastening point does not affect the measurement, it is possible to perform a continuous flow measurement.

By maintaining a constant temperature over the entire system, the density will be calculated based on the period assuming a hollow container having mass M suspended by a spring, with a spring constant c. The hollow container will be filled with a volume of liquid of density p. The natural frequency of this vibratory system is:

F=1/2

• A = (c/4)²  V
• et B=M/V
• which gives p = A T2 - B
• (p = rho).

Constants A and B are the oscillator's spring constants, i.e. the mass of the empty tube and the tube's filling capacity. A and B are therefore system constants specific to each oscillator. They can be deduced from the measurement of two periods when the oscillator is filled with substances of known densities.

5. Apparatus

5.1. Digital display densimeter.

This appliance comprises the following elements:

• a glass measuring cell containing the measuring tube, a constant temperature chamber to be connected to an external circulating thermostatic bath, and a thermowell. The chamber can also be thermostated using an integrated device with a semiconductor element which uses the PELTIER effect,
• a system for oscillating the measuring tube and for measuring the period of oscillation,
• a clock,
• a calculator and digital display.

5.2. Temperature control.

The densimeter's performance standards can only be met if the measuring cell is connected to a thermostatic bath, ensuring a temperature stability better than ± 0.02 °C, or if the densimeter has an integrated thermal control device which can achieve the same temperature stability.

5.3. Sample injection syringes.

At least 2 ml polypropylene or glass syringes with tips that fit to the cell inlet. An adapter with PTFE cones is required in order to avoid the deterioration of the tip of the measuring cell.

The electronic densimeter can also be equipped with the appropriate autosampler for the apparatus.

5.4. Temperature measurement.

Temperature measurement is carried out on the cell with a temperature probe whose sensing device (a platinum resistance probe compliant with class A of standard NF C 42.330), which is mounted with 4 wires, is introduced into the thermowell provided for this purpose in the cell. The probe is combined with an electronic temperature transmitter whose readout has a resolution of 0.01 °C. The probe and transmitter must first have been be calibrated in an approved calibration centre in order to ensure temperature measurement with an uncertainty less than or equal to ± 0.05°C.

The probe and transmitter must be periodically checked.

6. Products
   1. Reference fluids.

During tests, the fluids must maintain their density characteristics; therefore, they must not be made of mixtures of products with different vapour pressures; their molecular composition and purity must be known. Their viscosity must be lower than 2 mm²/s.

Reference fluids must be chosen so that the densities encompass those of the products to be measured. The difference in density between the 2 reference fluids at the same temperature must be higher than 0.01 g/m³.

The reference fluid densities determined at a temperature of 20 °C with an uncertainty of less than ± 0.05 °C must be known with an uncertainty of less than ± 0.05 kg/m³.

When measuring the density of alcohols and alcoholic beverages, the following must be used, under the conditions previously described:

• hydro-alcoholic solutions whose density is exclusively determined using the pycnometric method (reference method).
• recently prepared, degassed double distilled water, or water of equivalent analytical purity,
• dry air.

6.2. Cleaning products.

• chromic acid,
• organic solvents: ethanol 96 vol%, pure acetone.
  3. Drying.

• Pure acetone, dry air

7. Period measurements in ambient air

Prior to the commissioning and calibration of the densimeter, it is essential to ensure the reproducibility of the measurement in the ambient air so that this measurement can be used to quickly check the cleanliness of the cell and consistency of the densimeter before every density measurement.

It should be possible to perform measurements of periods in the ambient air with a reproducibility of ± 10^-5 in relative values over the period for the same barometric pressure and the same temperature.

With some densimeters, the resonant period in the ambient air varies depending on the position of the temperature probe in the thermowell. For these densimeters, either the measuring cell must be replaced, or the temperature probe must be permanently attached, or its position in the thermowell must be accurately determined in order to achieve the reproducibility conditions described above.

 

NOTE: The use of polluted or excessively humid air may negatively influence the measurements. When these characteristics are combined in the test room, it is advisable to make the drying air flow through a purifier/dryer.

8. Apparatus calibration
   1. General.

The apparatus must be calibrated upon initial commissioning. It must be recalibrated if a deviation in the air measurement is observed (see section 9.20) and, in any case, every three months.

8.2. During initial calibration, it is necessary to calculate the values of constants A and B, determined by measuring the periods of oscillation (T1 and T2) respectively obtained using two reference fluids.

8.2.1.    Place the display selector on the period measurement (T) position. Rinse the cell with acetone. Dry it with dry air generated by the pump that is integrated to the densimeter. When the reading is almost stable, stop the air supply, wait for thermal equilibrium and record the period of oscillation (Ta) obtained with an ambient air temperature of 20 °C. This process helps to check the cleanliness of the cell and stability of the apparatus at every calibration or determination of sample density.

8.2.2.    Calibration measurement using the first reference fluid. Use a syringe to fill the cell through its bottom port with the standard liquid until it comes flush with the top port. Leave the syringe in place. While performing this, check the filling quality by visually checking for any air bubbles, even tiny ones. When thermal equilibrium has been reached, record the reading for the period of oscillation (T1). If the thermal control is compliant with the required accuracy, the value of T1 must not vary by more than ± 20 nanoseconds (2 resolution points).

8.2.3.    Calibration measurement using the second reference fluid. Empty the cell with the syringe by drawing from the bottom port. Rinse the cell with acetone. Dry it with dry air generated by the pump that is integrated to the densimeter. To do so, connect the air outlet to the top port of the cell, start the pump and allow it to operate until the reading for T2 is almost constant; stop the pump, and when thermal equilibrium is reached, record the reading for the period of oscillation (T2) which corresponds to the air. If the reading for T2 matches the value obtained during previous tests carried out with a properly cleaned cell and at the same temperature, the cell can be considered clean and dry.

Carry out calibration using the second standard by repeating the steps in paragraph 8.22 and record the reading for the period of oscillation (T2) corresponding to the second reference fluid.

8.2.4.    Based on the T1 and T2 values measured and the known values for the densities of both reference fluids, calculate constants A and B using the following equations:

• A = T1² - T2² / p1 – p2
• B= T2² – Ap2

where

• T1 is the observed period of oscillation with the cell containing the first reference fluid (in ms).
• T2 is the observed period of oscillation with the cell containing the second reference fluid (in ms).
• p1 is the density of the first reference fluid at the test temperature (in g/cm³),
• p2 is the density of the second reference fluid at the test temperature (in g/cm³).

Depending on the procedure for the densimeter being used:

8.2.5.    Enter constants A and B using the digital display at the top of the apparatus. In order to make sure they have been correctly memorised, display the values by placing the selector on the "A" and "B" positions.

8.2.6.    Place the selector on the measurement position. The densimeter should immediately display the densities of the samples introduced into the measuring cell.

NOTE: Some electronic densimeter models automatically calculate the calibration constants.

8.3. Checking the calibration.

In order to validate the operation, measure a reference solution whose density value is within the calibration range used.

Reference substances, verified by a metrology agency, are commercially available.

The calibration is validated if the result of the measurement of the reference substance density complies with the accuracy class of the electronic densimeter being used.

9. Procedure
   1. Preparation of test apparatus.

• Place the densimeter on a perfectly stable support, isolated from any vibrations.
• Connect the densimeter to the circulating constant temperature bath using flexible rubber pipes or insulating tubes. Fill the water bath according to the manufacturer's instructions and add a product to prevent the formation of algae.

Set the bath temperature to reach and maintain the requisite test temperature on the densimeter.

• Accurately setting and controlling the temperature in the measuring cell are very important parameters, as a 0.1 °C error can result in a variation in density in the order of 0.1 kg/m³.
• The following rules must be observed:
• the measuring cell must be maintained at a constant temperature for 6 hours before the test.
• the maximum temperature variation measured by the temperature probe of the measuring cell must not exceed ± 0.02 °C.
• the pipe flow, length and insulation between the thermostatic bath and the cell are to be adjusted to ensure the stability of the cell temperature.

9.2. Checking period measurements in the ambient air.

• Clean, rinse and dry the cell.
• Carry out a measurement in the ambient air. Check that the period measured does not deviate by more than i0- in relative values from the period determined under the conditions described in section 7. If deviation occurs, clean the cell again with a lukewarm chromatic acid solution (warning: this product can cause serious burns), which is the most effective cleaning agent. If the deviation persists after several cleaning operations, repeat the calibration process.

9.3. Density measurement.

• Filter the sample first, if necessary.
• Illuminate the cell.

If only a small quantity of sample is available, use the syringe to introduce the quantity needed so that the liquid to be measured reaches the top port of the clean and dry cell. While filling the cell, make sure all air bubbles are completely removed; the sample must be homogeneous and must not contain any solid particulates.

• Leave the syringe in place on the bottom port of the cell.

NOTE: Introducing dark coloured samples into the cell does not help to establish the absence of air bubbles or solid particulates with certainty.

Switch off the lamp immediately after introducing the sample, as the heat it produces influences the measurement temperature.

9.4. Calculation and expression of results.

9.4.1.    Densimeter with an integrated calculator.

After a few minutes, the density value stabilises, indicating that the equilibrium temperature of the measurement has been reached. If the measurement temperature does not differ by more than ± 0.01 °C from a temperature of 20 °C, record the reading.

If needed, convert the obtained result into kg/m³.

9.4.2.    Densimeter without a calculator.

Allow the reading for the period of oscillation (T) to stabilise within one unit from the fourth decimal place. If the measurement temperature does not differ by more than ± 0.01 °C from a temperature of 20 °C, record the reading.

Calculate the density of the sample in kg/m3 using the following formula:

where

• T is the period of oscillation for the sample measured (in ms).
• A and B are the constants defined during the calibration prescribed in paragraph 8.

9.4.3.    Viscosity correction.

If the liquid whose density is being measured has a viscosity higher than 2 mm²/s, correction is required to take the viscosity into account, using the formula provided by the manufacturer of the densimeter.

10. Test report

The test report must indicate:

• the method used,
• the result and mode of expression of results,
• the specific details and any unforeseen events recorded during the measurement,
• operations not included in the method.

 

APPENDIX A

TABLE 1

AIR DENSITY

Air density, expressed in g/cm³, varies with the pressure P expressed in mbar and the temperature expressed in °C.

A t °C and p Ton-, calculate the density using the following formula:

Values are given for contents of 0.03 vol% of CO₂ in the air; values change by ± 1/19000 with each variation of ± 0.0001 of the CO₂ volume.

Composition of dry air at ground level:

	N2	O2	A	CO2	Ne	He	Kr	X	H2
Volume in %	78.09	20.95	0.93	0,03	0.0018	0.0005	0.041	0.068	0.045
Mass in %	75.52	23.15	1.28	0.05	0.0013	0.047	0.043	0.044	0.084

Method OIV-MA-BS-15 : R2009

Type II method

Anethole. Gas chromatography determination of trans-anethole in spirit drinks of viti-vinicultural origin

(OIV/OENO 379/2009)

1.                Scope

This method is suitable for the determination of trans-anethole in aniseed-flavoured spirit drinks using capillary gas chromatography.

2.                Normative references

ISO 3696: 1987 Water for analytical laboratory use - Specifications and test methods.

3.                Principle

The trans-anethole concentration of the spirit is determined by gas chromatography (GC). The same quantity of an internal standard, e.g. 4‑allylanisole (estragole) when estragole is not naturally present in the sample, is added to the test sample and to a trans‑anethole reference solution of known concentration, both of which are then diluted with a 45% ethanol solution and injected directly into the GC system.

An extraction is necessary before sample preparation and analysis for liqueurs that contain large amounts of sugars.

4.                Reagents and materials

During the analysis use only reagents of a purity of at least 98 %.  Water of at least grade 3 as defined by ISO 3696 should be used.

Reference chemicals should be stored cold (ca. 4°C), away from light, in aluminium containers or in tinted (amber) glass reagent bottles.  The stoppers should preferably be fitted with an aluminium seal. Trans-anethole will need to be "thawed" from its crystalline state before use, but in this case its temperature should never exceed 35°C.

4.1.      Ethanol 96 % vol.  (CAS 64-17-5)

4.2.      1-methoxy-4- (1-propenyl) benzene; (trans-anethole) (CAS 4180-23-8)

4.3.      4-allylanisole, (estragole) (CAS 140-67-0), suggested internal standard (IS)

4.4.      Ethanol 45 % vol.

Add 560 g of distilled water to 378 g of ethanol 96 % vol.

4.5.      Preparation of standard solutions

All standard solutions should be stored at room temperature (15-35°C) away from light in aluminium containers or in tinted (amber) glass reagent bottles.  The stopper should preferably be fitted with an aluminium seal.

Trans-anethole and 4-allylanisole are practically insoluble in water, and it is therefore necessary to dissolve the trans-anethole and 4-allylanisole in some 96 % ethanol (4.1) before the addition of 45 % ethanol (4.4).

The stock solutions must be freshly prepared each week.

4.5.1.                    Standard solution A

Stock solution of trans‑anethole (concentration: 2 g/L)

Weigh 40 mg of trans-anethole (4.2) in a 20 mL volumetric flask (or 400 mg in 200 mL, etc.).  Add some 96 % ethanol (4.1) and make up to volume with 45 % vol. ethanol (4.4), mix thoroughly.

4.5.2.                    Internal standard solution B

Stock solution of internal standard, e.g. estragole (concentration: 2 g/L)

Weigh 40 mg of estragole (4.3) in a 20 mL volumetric flask (400 mg in 200 mL etc.).  Add some 96 % vol. ethanol (4.1) make up to volume with 45 % vol. ethanol (4.4), mix thoroughly.

4.5.3.                    Solutions used to check the linearity response of the FID

The linearity response of the FID must be checked for the analysis taking into account a range of concentrations of trans-anethole in spirits from 0 g/L up to 2.5 g/L. In the procedure of analysis, the unknown samples of spirits to be analysed are diluted 10 times (8.3). For the conditions of the analysis described in the method, stock solutions corresponding to concentrations of 0, 0.05, 0.1, 0.15, 0.2, and 0.25 g/L of trans-anethole in the sample to be analysed are prepared as follows: take 0.5, 1, 1.5, 2, and 2.5 mL of stock solution A (4.5.1) and pipette in separate 20 mL volumetric flasks; pipette into each flask 2 mL of internal standard solution B (4.5.2) and make up to volume with 45 % vol. ethanol (4.4), mix thoroughly.

The blank solutions (8.4) is used as the 0 g/L solution.

4.5.4.                    Standard solution C

Take 2 mL of standard solution A (4.5.1) and pipette into a 20 mL volumetric flask then add 2 mL of internal standard solution B (4.5.2) and make up to volume with 45% vol. ethanol (4.4), mix thoroughly.

5.                Apparatus and equipment

5.1.      A capillary gas chromatograph fitted with a flame ionisation detector (FID) and integrator or other data handling system capable of measuring peak areas, and with an automatic sampler or the necessary equipment for manual sample injection.

5.2.      Split/splitless injector

5.3.      Capillary column, for example:

Length:  50 m

Internal diameter: 0.32 mm

Film thickness: 0.2 µm

Stationary phase: FFAP ‑ modified TPA polyethylene glycol cross‑linked porous polymer

Common laboratory equipment: A grade volumetric glassware, analytical balance (precision:  ±0.1 mg).

6.                Chromatography conditions

The column type and dimensions, and the GC conditions, should be such that anethole and the internal standard are separated from each other and from any interfering substances.  Typical conditions for the column given as an example in 5.3 are:

6.1.      Carrier gas: analytical helium.

6.2.      Flow rate: 2 mL/min

6.3.      Injector temperature: 250°C.

6.4.      Detector temperature: 250°C.

6.5.      Oven temperature conditions: isothermal, 180°C, run time 10 minutes

6.6.      Injection volume: 1µL, split 1:40

7.                Samples

Samples should be stored at room temperature, away from light and cold.

8.                Procedure

8.1.      Sample screening for estragole

To ensure that there is no estragole naturally present in the sample, a blank analysis should be carried out without the addition of any internal standard.  If estragole is naturally present then another internal standard must be chosen (for instance menthol).

Pipette 2 mL sample into a 20 mL volumetric flask and make up to volume with 45% vol. ethanol (4.4), mix thoroughly.

8.2.      Preparation of unknown samples

Pipette 2 mL sample into a 20 mL volumetric flask then add 2 mL of internal standard solution B (4.5.2) and make up to volume with 45 % vol. ethanol (4.4), mix thoroughly.

8.3.      Blank

Pipette 2 mL of internal standard solution B (4.5.2) into a 20 mL volumetric flask and make up to volume with 45 % vol. ethanol (4.4), mix thoroughly.

8.4.      Linearity test

Prior to the commencement of the analysis the linearity of the response of the FID should be checked by successively analysing in triplicate each of the linearity standard solutions (4.5.3).

From the integrator peak areas for each injection plot a graph of their mother solution concentration in g/L versus the ratio R for each.

R = trans-anethole peak area divided by the estragole peak area.

A linear plot should be obtained.

8.5.      Determination

Inject the blank solution (8.3), followed by standard solution C (4.5.4), followed by one of the linearity standards (4.5.3) which will act as a quality control sample (this may be chosen with reference to the probable concentration of trans-anethole in the unknown), followed by 5 unknowns (8.2); insert a linearity (quality control) sample after every 5 unknown samples, to ensure analytical stability.

9.                Calculation of response factor

Measure peak areas (using an integrator or other data system) for trans-anethole and internal standard peaks.

9.1.      Response factor (RF_i) calculation

The response factor is calculated as follows

Where:

• is the concentration of trans-anethole in the standard solution A (4.5.1.)
• is the concentration of internal standard in the standard solution B (4.5.2.)
• is the area of the trans-anethole peak
•  is the area of the internal standard peak
• is calculated from the 5 samples of solution C (4.5.4)

9.2.      Analysis of the linearity response test solutions

Inject the linearity response test solutions  (4.5.3).

9.3.      Analysis of the sample

Inject the unknown sample solution (8.2)

10.         Calculation of results

The formula for the calculation of the concentration of trans-anethole is the following:

where:

• is the unknown trans-anethole concentration
• is the concentration of internal standard in the unknown (4.5.2)
• is the area of the trans-anethole peak
• is the area of the internal standard peak
• is the response coefficient (calculated as in 9.1)

The trans-anethole concentration is expressed as grams per litre, to one decimal place.

11.         Quality assurance and control

The chromatograms should be such that anethole and the internal standard are separated from each other and from any interfering substances.  The RF_i value is calculated from the results for the 5 injections of solution C (4.5.4).  If the coefficient of variation (CV % = (standard deviation/mean)*100)) is within plus or minus 1 %, the RF_i average value is acceptable.

The calculation above should be used to calculate the concentration of trans-anethole in the sample selected for the quality control from the linearity control solutions (4.5.3).

If the mean calculated results from analysis of the linearity solution selected for Internal Quality Control sample (IQC) are within plus or minus 2.5 % of their theoretical value, then the results for the unknown samples can be accepted.

12.         Treatment of spirits sample containing large amount of sugar and of liqueur sample prior to GC analysis

Extraction of alcohol from spirit drink containing a large amount of sugar, in order to be able to determine the trans-anethole concentration using capillary gas chromatography.

12.1. Principle

An aliquot of the liqueur sample is taken and to this is added the internal standard, at a concentration similar to that of the analyte (trans-anethole) in the liqueur. To this are added sodium phosphate dodecahydrate and anhydrous ammonium sulphate. The resulting mixture is well shaken and chilled, two layers develop, and the upper alcohol layer is removed. An aliquot of this alcohol layer is taken and diluted with 45 % ethanol solution (4.4) (Note: no internal standard is added at this stage, because it has already been added). The resulting solution is analysed in gas chromatography.

12.2. Reagents and materials

During the extraction use only reagents of a purity greater than 99 %.

12.2.1.               Ammonium sulphate, anhydrous, (CAS 7783-20-2)

12.2.2.               Sodium phosphate, dibasic, dodecahydrate, (CAS 10039-32-4)

12.3. Apparatus and equipment

Conical flasks, separating flasks, refrigerator.

12.4. Procedure

12.4.1.               Sample screening for estragole

To ensure that there is no estragole naturally present in the sample, a blank extraction (12.6.2) and analysis should be carried out without the addition of any internal standard.  If estragole is naturally present then another internal standard must be chosen.

12.4.2.               Extraction

Pipette 5 mL of 96 % ethanol (4.1) into a conical flask, weigh into this flask 50 mg of internal standard (4.3), and add 50 mL of the sample.  Add 12 g of ammonium sulphate, anhydrous (12.2.1), and 8.6 g of dibasic sodium phosphate, dodecahydrate (12.2.2).  Stopper the conical flask.

Shake the flask for at least 30 minutes.  A mechanical shaking device may be used, but not a Teflon coated magnetic stirring bar, as the Teflon will absorb some of the analyte.  Note that the added salts will not dissolve completely.

Place the stoppered flask in a refrigerator  (T< 5^oC) for at least two hours.

After this time, there should be two distinct liquid layers and a solid residue.  The alcohol layer should be clear; if not replace in the refrigerator until a clear separation is achieved.

When the alcohol layer is clear, carefully take an aliquot (e.g. 10 mL), without disturbing the aqueous layer, place in an amber vial and close securely.

12.4.3.               Preparation of the extracted sample to be analysed

Allow extract (12.4.2) to reach room temperature.

Take 2 mL of the alcohol layer of the attemperated extracted sample and pipette into a 20 mL volumetric flask, make up to volume with 45 % ethanol (4.4), mix thoroughly.

12.5. Determination

Follow the procedure as outlined in 8.5.

12.6. Calculation of results

Use the following formula to calculate the results

Where:

• is the weight of internal standard (4.3.) taken (12.4.2) (in milligrams)
• V is the volume of unknown sample (50 mL)
• is the response factor (9.1.)
• isthe area of the trans-anethole peak
•   is the area of the internal standard peak

The results are expressed in grams per litre, to one decimal place.

12.7. Quality control and assurance

Follow the procedure as outlined in 11 above.

13.         Method performance characteristics (precision)

Statistical results of the interlaboratory test: the following tables give the values for anethole.

The following data were obtained from an international method performance study carried out on a variety of spirit drinks to internationally agreed procedures.

Year of interlaboratory test	1998
Number of laboratories	16
Number of samples	10
Analyte	Anethole

Pastis :

Samples	A	B	C	D	E	F
Number of laboratories retained after eliminating outliers	15	15	15	13	16	16
Number of outlirs (laboratories)	1	1	1	3	-	-
Number of accepted results	30	30	30	26	16	16
Mean value g/l	1,477	1,955	1,940	1,833	1,741	1,754
Repeatability standard deviation (Sr) g/l	0,022	0,033	0,034	0,017	-	-
Repeatability relative Standard deviation (RSDr) (%)	1,5	1,7	1,8	0,9	-	-
Repeatability limit (r)  g/l	0,062	0,093	0,096	0,047	-	-
Reproducibility standard deviation (sR) g/l	0,034	0,045	0,063	0,037	0,058	0,042
Reproducibility relative standard deviation (RSDR) (%)	2,3	2,3	3,2	2,0	3,3	2,4
Reproducibility limit (R) g/l	0,094	0,125	0,176	0,103	0,163	0,119

Sample types:

A pastis, blind duplicates

B pastis, blind duplicates

C pastis, blind duplicates

D pastis, blind duplicates

E pastis, single sample

F, single sample

Other aniseed-flavoured spirit drinks:

Samples	G	H	I	J
Number of laboratories retained after eliminating outliers	16	14	14	14
Number of outliers (laboratories)	-	2	1	1
Number of accepted results	32	28	28	28
Mean value g/l	0,778 0,530*	1,742	0,351	0,599
Repeatability standard deviation (Sr) g/l	0,020	0,012	0,013	0,014
Repeatability relative standard deviation (RSDr) (%)	3,1	0,7	3,8	2,3
Repeatability limit (r) g/l	0,056	0,033	0,038	0,038
Reproducibility standard deviation (SR) g/l	0,031	0,029	0,021	0,030
Reproducibility relative standard deviation (RSDR) (%)	4,8	1,6	5,9	5,0
Reproducibility limit (R) g/l	0,088	0,080	0,058	0,084

Sample types:

G ouzo, split levels (*)

H anis, blind duplicates

I aniseed-flavoured liqueur, duplicates

J aniseed-flavoured liqueur, duplicates

14.         Bibliography

1. Commission Regulation (EC) N° 2091/2002 of 26 November 2002 amending Regulation (EC) No 2870/2000 laying down Community reference methods for the analysis of spirits drinks, OJEC of 27 November 2002, L322/11
2. P. Brereton, S. Hasnip, A. Bertrand, R. Wittkowski, C. Guillou, Analytical methods for the determination of spirit drinks, Trends in Analytical Chemistry, Vol. 22, No. 1, 19-25, 2003

OIV-MA-BS-10 Determination of total dry extract usual method by calculation

Type IV method

1. Principle

 

The total dry extract can be calculated indirectly based on the value of the density of the "residue without alcohol" or the alcoholic beverage from which the alcohol has been removed and has been returned to the original volume by adding water. This dry extract is expressed as the amount of sucrose which, dissolved in one litre of solution, has the same density.

This quantity is given by the Plato table (table 1).

2. Procedure

Density 20/20, dr, of the "residue without alcohol" is calculated by Tabarie's Formula:

• where ds = density of the alcoholic beverage at 20°C compared with water at 20°C
• da = density at 20°C of the same hydroalcoholic mixture as the alcoholic beverage, relative to water at 20°C.

dr can also be calculated based on the densities at 20°C ρv of the alcoholic beverage ρa the hydroalcoholic mixture of the same degree by the formula

Record the density dr of the de-alcoholised medium in Table 1 to obtain the weight of total dry extract in grams per litre.

Table 1 for the calculation of solids content

Relative
density	Third decimal point of relative density
to 2 decimal points	0	1	2	3	4	5	6	7	8	9
	Grams of extract per litre
1,00	0,0	2,6	5,1	7,7	10,3	12,9	15,4	18,0	20,6	23,2
1,01	25,8	28,4	31,0	33,6	36,2	38,8	41,3	43,9	46,5	49,1
1,02	51,7	54,3	56,9	59,5	62,1	64,7	67,3	69,9	72,5	75,1
1,03	77,7	80,3	82,9	85,5	88,1	90,7	93,3	95,9	98,5	101,1
1,04	103,7	106,3	109,0	111,6	114,2	116,8	119,4	122,0	124,6	127,2
1,05	129,8	132,4	135,0	137,6	140,3	142,9	145,5	148,1	150,7	153,3
1,06	155,9	158,6	161,2	163,8	166,4	169,0	171,6	174,3	176,9	179,5
1,07	182,1	184,8	187,4	190,0	192,6	195,2	197,8	200,5	203,1	205,8
1,08	208,4	211,0	213,6	216,2	218,9	221,5	224,1	226,8	229,4	232,0
1,09	234,7	237,3	239,9	242,5	245,2	247,8	250,4	253,1	255,7	258,4
1,10	261,0	263,6	266,3	268,9	271,5	274,2	276,8	279,5	282,1	284,8
1,11	287,4	290,0	292,7	295,3	298,0	300,6	303,3	305,9	308,6	311,2
1,12	313,9	316,5	319,2	321,8	324,5	327,1	329,8	332,4	335,1	337,8
1,13	340,4	343,0	345,7	348,3	351,0	353,7	356,3	359,0	361,6	364,3
1,14	366,9	369,6	372,3	375,0	377,6	380,3	382,9	385,6	388,3	390,9
1,15	393,6	396,2	398,9	401,6	404,3	406,9	409,6	412,3	415,0	417,6
1,16	420,3	423,0	425,7	428,3	431,0	433,7	436,4	439,0	441,7	444,4
1,17	447,1	449,8	452,4	455,2	457,8	460,5	463,2	465,9	468,6	471,3
1,18	473,9	476,6	479,3	482,0	484,7	487,4	490,1	492,8	495,5	498,2
1,19	500,9	503,5	506,2	508,9	511,6	514,3	517,0	519,7	522,4	525,1
1,20	527,8	-	-	-	-	-	-	-	-	-

Interpolation table

Fourth decimal point of relative density	Grams of extract per litre	Fourth decimal point of relative density	Grams of extract per litre	Fourth decimal point of relative density	Grams of extract per litre
1	0,3	4	1,0	7	1,8
2	0,5	5	1,3	8	2,1
3	0,8	6	1,6	9	2,3

OIV-MA-BS-13 Determination of pH

Type IV method

1. Presentation

The pH is closely related to the concentration of hydrogen ions (H+) present in alcoholic beverages (the pH characteristics of alcoholic beverages depend on various parameters, such as the quality of the reducing water, the duration of maturation in casks, the nature of the aromatic raw materials, and of any additives).

Due to the presence of ethyl alcohol in alcoholic beverages, the pH should be measured according to specific procedures.

2. Purpose

The purpose of the present document is to describe the measurement of pH in alcoholic beverages by the potentiometric method, using a glass electrode.

On the one hand it specifies the essential characteristics required of the appliance in order to obtain comparable results, and on the other, standardises the operating instructions for the glass electrode and the techniques to follow in order to obtain satisfactory results.

3. Scope

The method is applicable in the case of measurements on beverages with an alcoholic strength by volume ranging between 15 and 50% vol.

4. Principle of the method

4.1. Definition of pH

The pH of a solution is the decimal cologarithm of the solution activity in hydrogen ions and is measured in pH units.

4.2. General principle

The potential difference between a glass electrode and reference electrode immersed in the same solution is a linear function of its pH. According to the laws of Nernst, the electrode potential is related to the activity of the H+ ions present as indicated by the relationship

H = k + RT Loa (H+l F

where

• R is the gas constant, in joules / degrees
• T is the absolute temperature (°K)
• F is the Faraday symbol (96,500 coulombs)
• (H+) is the activity of the H+ ions,
• k is a constant depending on the nature of the glass electrode and the measuring device.

Determining the pH is therefore equivalent to the accurate measurement of potential difference. This measurement is made using a potentiometric apparatus with amplifiers. The assembly is required because of the high resistance of the electrical circuit and, in particular, that of the glass electrode.

Given the influence of temperature on the measurement result, the electrometer used must be equipped with an apparatus for temperature compensation and the exact conversion of the electromotive force in pH units, at a temperature of the sample.

The asymmetry potential of the glass membrane and the junction and diffusion potentials between the reference electrode and the liquid being tested will be eliminated by calibrating the system using standard solutions of known pH. One these standard solutions will be considered as the primary standard.

4.3. Principle applied to alcoholic beverages

4.3.1.    The measurement of pH in organic media

The traditional pH range extending from 0 to 14 is determined by the dissociation of water. If the water content of a solution is gradually reduced or the water is replaced by another solvent, it is the dissociation equilibrium, i.e. the latter’s ionic product which is taken into account instead of that of the water. This results in totally different concentration ranges for the "free" H+ ions (i.e. which are not chemically bound).

In non-aqueous media, it is not possible to carry out absolute measurements of pH. Only relative measurements can be made. In addition, partially aqueous media are often low-ion.

However, from a water content of at least 5%, the classic definition of pH can be used, i.e. expressed in terms of absolute values and not just relative values.

Under these operating conditions, at the interface between the electrolyte and solution to be measured a phase separation is often formed which makes the signal unstable.  There is also a risk of precipitation at the membrane level. The same problem is also encountered when using concentrated solutions of KCl as the reference electrolyte.

4.3.2.    Specific measurement conditions

To avoid the problems described above, the basic requirement is that the electrolyte solution to measure and form a homogeneous solution without phase separation or precipitation. This condition can be met using lithium chloride (LiCl) in an ethanol medium.

A second condition is the use of an electrode with cylindrical membrane and a ground-in diaphragm, to ensure optimum contact between the reference electrolyte and the solution to be measured.

5. Apparatus
   1. pHmeter

pH meter calibrated in pH units, enabling measurements to a minimum accuracy of: 0.01 pH i.e. 1 mV.

The instrument is preferably to be equipped with an electronic device for the automatic compensation of the temperature to a minimum accuracy of 0.5°C.

The pH meter should be used in a place sheltered from pollutants, acid or alkaline vapours in particular, hydrogen sulphide (H2S) and ammonia (NH3).

5.2. Electrodes

5.2.1.    Combined electrode

The electrodes marketed for this specific purpose are generally of the type: combined electrode.

The useful part of the electrode consists of a cylindrical membrane and a ground-in diaphragm made of Teflon.

The reference electrolyte is an ethanol solution at 95% vol. of lithium chloride (LiCl) to 1 mol/L. Its alcoholic strength should be close to that of the alcoholic beverage to be analysed.

5.2.2.    Immerse the electrode tip when not used continuously, in an ethanol solution of lithium chloride to 1 mol/1, unless otherwise specified by the manufacturer of the electrode.

5.3. Small laboratory equipment

5.3.1.    Common glassware: beakers, crystallizers, etc.

5.3.2.    Stirring device: magnetic stirrer and bar, for example.

5.3.3.    Cleaning supplies: Joseph paper, etc.

6. Reagents
   1. Deionised or distilled water.

Free from carbon dioxide and metal ions, with a maximum conductivity of 20°C 200 µS/m.

6.2. Standard buffer solution.

With reference to standard NFT 01012 "pH measurement - standard solutions for calibration of a pH meter”

6.2.1.    pH buffer solution: 3.57 at 20°C

 Saturated solution of potassium acid tartrate. Solution containing at least 5.7 g/1 of potassium acid tartrate (HOOC C₂H₄O₂ COOK) at 20°C. This solution can be kept for two months in the presence of 0.1 g of thymol per 200 ml.

pH	3.57 at 20°C
	3.56 at 25°C
	3.55 at 30°C

6.2.2.    pH buffer solution: 4.00 at 20°C

• 0.05 M solution of potassium hydrogen phthalate. Solution containing 10.211 g/1 of potassium hydrogen phthalate (HOOC C₂ H₄ COOK) at 20°C (maximum storage time: 2 months).

pH	3.999 at 15°C
	4.003 at 20°C
	4.008 at 25°C
	4.015 at 30°C

6.2.3.    pH buffer solution: 6.88 at 20°C

• Solution containing
• Dihydrogen phosphate, KH₂PO₄:  3.402 g
• Dipotassium phosphate, K₂HPO₄: 4.354 g
• Water q.s.p 1 L
• (Shelf life: 2 months)

pH	6.90 at 15°C
	6.88 at 20°C
	6.86 at 25°C
	6.85 at 30°C

6.2.4.    pH buffer solution: 9.22 at 20°C Solution containing

• Decahydrated Borax, B₄O₇Na₂.10 H₂O...: 3.810 g
• Water q.s.p: 1 L

(Basic buffer solutions are quickly altered by the carbon dioxide in the surrounding air, and it is therefore necessary to renew the solution for each calibration).

pH: 9.22 at 20°C

Note: market-available reference buffer solutions can also be used (according to the DIN 19266 standard and NBS, for example).

7. Procedure
   1. Calibration of the measurement chain
      1.     Two standard solutions are needed to calibrate the pH meter. Their pH should, if possible, be located on either side of the presumed pH value of the test solution; if this is not possible, one of them must not differ by more than one unit pH from the presumed value.

7.1.2.    Zero setting the measurement chain (pH)

Operate in accordance with the instructions provided with the apparatus used.

Rinse the electrodes with the first standard buffer solution by pouring the liquid along them.

Introducing a sufficient volume of the same standard solution into the measuring vessel, which should be clean and dry, and immerse the electrodes.

Adjust the indication of the pH meter on the pH value of the standard solution taking into account its temperature (if necessary).

Remove the electrodes and discard the standard solution contained in the measuring vessel.

7.1.3.    Setting the slope of the electrode

Rinse the electrodes with distilled or deionised water and then with the second standard buffer solution

Introduce a sufficient volume of the same standard buffer solution and immerse the electrodes.

If the result matches the known value of the pH of the standard solution, the unit is in working condition and is properly calibrated.

7.1.4.    Calibration Check

Use a buffer solution with an intermediate pH value in relation those used for calibration.

7.2. pH measurements

Once the device has been calibrated, rinse the electrodes and the measuring vessel, first with deionised or distilled water, then with the test solution by proceeding as above. Homogenize the test solution, introduce a sufficient volume in the measuring vessel and immerse the electrodes.

Lightly stir the test solution.

Verify that the indication given by the pH meter is stable and record it.

8. Expression of results

 

In the operating conditions described above, the accuracy of the determination is ± 0.02 pH units

The results are expressed in units of pH, at a temperature of: 20°C, in the form

pH at 20 °C = xx, xx

9. Test report

Indicate in the test report:

• The method used,
• The specific details and any unforeseen events recorded during the measurement,
• Operations that were not scheduled or were optional.

10. Bibliography

• Method written with reference to the standards
• NFTO1-013 Mesure électrométrique du pH au moyen d'une électrode de verre - Vocabulaire et méthode de mesure –
• NFTO1-012 pH-métrie - Solutions étalons pour l'étalonnage d'un pH-mètre

Other sources

• Norme NF T 90-008 - Essais des Eaux. Mesure électrométrique du pH avec l'électrode de verre.
• Utilisation et entretien des instruments de mesure - Cahier technique - Fondation de l'eau - Ministère de l'Environnement –
• Théorie der Glaselektrode - K. Schwabe et H.D. Suschke-Angeur - Chem.76 (1964) 39-49

La pratique et la théorie de la Mesure du pH - Ingold Messtechnik AG.Compendium of International Methods of Analysis of Wines and Musts - International Office of Vine and Wine (OIV): Mesure du pH des vins et des moûts.