Annex F - Specific Methods for the Analysis of Grape Sugar

Codified File

Conductivity (Type-IV)

OIV-MA-F1-01 Conductivity

Type IV method

  1. Principle

The electrical conductivity of a column of liquid defined by two parallel platinum electrodes at its ends is measured by incorporating it in one arm of a Wheatstone bridge.

The conductivity varies with temperature and it is therefore expressed at 20°C.

  1. Reagents

 

Use only reagent grade chemicals

2.1.  Purified water for laboratories, with specific conductivity below 2 μS cm-1 at 20°C, for example EN ISO 3696 type II water.

2.2.  Reference solution of potassium chloride.

Dissolve 0.581 g of potassium chloride, KCl previously dried to constant mass at a temperature of 105°C, in demineralised water (2.1). Make up to one litre with demineralised water (2.1). This solution has a conductivity of 1 000 μS cm-1 at 20°C. It should not be kept for more than three months.

A commercial preparation can be used.

  1. Apparatus

3.1.  Conductivity meter enabling measurements of conductivity to be made over a range from 1 to 1 000 microsiemens per cm (μS cm-1).

3.2.  Water bath for bringing the temperature of samples to be analysed to approximately 20°C (20 2°C).

  1. Procedure
    1.   Preparation of the sample to be analysed

Use a solution with a total sugar concentration of 25 0.5 % (m/m) (25° Brix): weigh a mass equal to 2500/P and make up to 100 g with water (2.1),

P = percentage (m/m) of total sugars in the rectified concentrated must.

4.2.  Determination of conductivity

Bring the sample to be analysed to 20°C by immersion in a water bath. Maintain the temperature to within ± 0.1°C.

Rinse the conductivity cell twice with the solution to be examined.

Measure the conductivity and express the result in μS cm-1.

  1. Expression of the Results

The result is expressed in microsiemens per cm (μScm−1) at 20°C to the nearest whole number for the 25% (m/m) (25° Brix) solution of rectified concentrated must.

5.1.  Calculations

If the apparatus does not have temperature compensation, correct the measured conductivity using Table I. If the temperature is below 20°C, add the correction; if the temperature is above 20°C, subtract the correction.

 

  1. Characteristics of the method

Repeatability (r)

  • r = 3 μS/cm

Reproducibility (R)

  • R = 16 μS/cm

Table I

Corrections to be made to the conductivity for temperatures different from 20°C (μS cm−1)

Conductivity

Temperature (°C)

20.2

19.8

20.4

19.6

20.6

19.4

20.8

19.2

21.

19.0

21.2

18.8

21.4
18.6

21.6
18.4

21.8

18.2

22,0(1)

18.0(2)

0

0

0

0

0

0

0

0

0

0

0

50

0

0

1

1

1

1

1

2

2

2

100

0

1

1

2

2

3

3

3

4

4

150

1

1

2

3

3

4

5

5

6

7

200

1

2

3

3

4

5

6

7

8

9

250

1

2

3

4

6

7

8

9

10

11

300

1

3

4

5

7

8

9

11

12

13

350

1

3

5

6

8

9

11

12

14

15

400

2

3

5

7

9

11

12

14

16

18

450

2

3

6

8

10

12

14

16

18

20

500

2

4

7

9

11

13

15

18

20

22

550

2

5

7

10

12

14

17

19

22

24

600

3

5

8

11

13

16

18

21

24

26

(1)Subtract the correction.

(2)Add the correction.

 

Hydroxymethylfurfural (HMF) by High-Performance Liquid Chromatography (Type-IV)

OIV-MA-F1-02 Hydroxymethylfurfural (HMF) by High-Performance Liquid Chromatography

Type IV method

 

  1. Principle of the Method

High-performance liquid chromatography (HPLC)

Separation through a column by reversed-phase chromatography and determination at 280 nm.

  1. Reagents

2.1.  Purified water for laboratory use and of quality standard EN ISO 3696

2.2.  Methanol, OH, distilled or HPLC quality. – CAS Number 67-59-1

2.3.  Acetic acid, CH3COOH, (ρ20 = 1.05 g/ml). – CAS Number 64-19-7

2.4.  Mobile phase: water (2.1) -methanol (2.2)-acetic acid (2.3) previously filtered through a membrane filter (0.45 μm), (40:9:1 v/v).

This mobile phase must be prepared daily and degassed before use.

2.5.  Reference solution of hydroxymethylfurfural, 25 mg/l (m/v).

Into a 100 ml volumetric flask, place 25 mg of hydroxymethylfurfural, C6H3O6, accurately weighed, and make up to the mark with methanol ( 2.2). Dilute this solution 1/10 with methanol (2.2) and filter through a membrane filter (0.45 μm).

If kept in a hermetically sealed brown glass bottle in a refrigerator, this solution will keep for two to three months.

(The concentration of the reference solution is given for guidance)

  1. Equipment

3.1.  Apparatus

High-performance liquid chromatograph equipped with:

  • a loop injector, 5 or 10 μl, (as an example),
  • spectrophotometric detector for making measurements at 280 nm,
  • column of octadecyl-bonded silica (e.g.: Bondapak C18 — Corasil, Waters Ass.),
  • a recorder and, if required, an integrator,

Flow rate of mobile phase: 1.5 ml/minute (as an example).

3.2.  Membrane filtration apparatus, pore diameter 0.45 μm.

  1. Procedure
    1.   Preparation of sample

Use the solution obtained by diluting the rectified concentrated must to 40% (m/v) (introduce 200 g of accurately weighed rectified concentrated must into a 500 ml volumetric flask. Make up to the mark with water and homogenise) and filter it through a membrane filter (0.45μm).

4.2.  Chromatographic determination

Inject 5 (or 10) μl of the sample prepared as described in paragraph 4.1. and 5 (or 10) μl of the reference hydroxymethylfurfural solution (2.5) into the chromatograph. Record the chromatogram.

The retention time of hydroxymethylfurfural is approximately six to seven minutes.

The volume injected and the sequence are given for guidance. The chromatographic determination can also be done with a calibration curve

  1. Expression of results

The hydroxymethylfurfural concentration in rectified concentrated musts is expressed in milligrams per kilogram of total sugars.

5.1.  Method of calculation

Let the hydroxymethylfurfural concentration in the 40% (m/v) solution of the rectified concentrated must be C mg/l.

The hydroxymethylfurfural concentration in milligrams per kilogram of total sugars is given by:

P = percentage (m/m) concentration of total sugars in the rectified concentrated must.

  1. Characteristics of the method

 

Repeatability (r)

  • r = 0.5 mg/kg total sugars

Reproducibility (R)

  • R = 3.0 mg/kg total sugars

Determination of the acquired alcoholic strength by volume (ASV) of concentrated musts (CM) and grape sugar (or rectified concentrated musts, RCM) (Oeno 419A-2011) (Type-IV)

OIV-MA-F1-03 Determination of the acquired alcoholic strength by volume (ASV) of concentrated musts (CM) and grape sugar (or rectified concentrated musts, RCM)

Type IV method

 

  1. Introduction

Concentrated musts (CM) and grape sugar (RCM) are viscous products with low alcohol contents; to determine their acquired ASV, a method must be used, the characteristics of which (linearity, repeatability, reproducibility, specificity, and detection and quantification limits) must be such that it is possible to measure alcohol contents of less than 1% vol.

  1. Field of application

The method applies to concentrated musts and grape sugar.

  1. Principle

A known mass of concentrated must (CM) or grape sugar is made alkaline by a suspension of calcium hydroxide and then distilled. The alcoholic strength by volume of the distillate is determined by electronic densitometry or by densitometry using a hydrostatic balance.

  1. Reagents
  • Suspension of 2M calcium hydroxide of analytical quality obtained by carefully pouring one litre of hot water (60°C to 70°C) on to about 120 g of unslaked lime (CaO).
  • Antifoam solution obtained by dilution of 2 ml of concentrated silicone antifoam in 100 ml of water.
  • Purified water for laboratory use and of quality EN ISO 3696.
  1. Equipment
  • Standard laboratory equipment including volumetric flasks 
  • Analytic balance capable of weighing to within 0.1 g.
  • Any type of distillation or steam distillation apparatus may be used provided that it satisfies the following test:
  • Distil an ethanol‑water mixture with an alcoholic strength of 10% vol. five times in succession.  The distillate should have an alcoholic strength of at least 9.9% vol. after the fifth distillation; i.e. the loss of alcohol during each distillation should not be more than 0.02% vol.
  • Electronic density meter or hydrostatic balance.
  1. Procedure
  • Homogenise the test sample by inverting the flask several times.
  • In a 500 ml volumetric flask, weigh about 200 g of concentrated must or rectified concentrated must (to within 0.1 g). Note the weight (TS) of this test sample. Fill up to the mark with deionised water. This solution is about 40% m/v in must.

Obtaining the distillate

  • Transfer 250 ml of the 40% solution to the distillation flask, add to the flask about 10 ml of calcium hydroxide in suspension, about 5 ml of antifoam solution and, where applicable, a boiling regulator (e.g. pieces of porcelain).
  • Gently bring to the boil.
  • Recover the distillate in a 100 ml volumetric flask (about 90 ml).
  • Leave the distillate to return to ambient temperature, then fill up to the mark with deionised water.

Measurement of ASV

This is performed by electronic densitometry or by hydrostatic balance.

  1. Calculation

  • ASV measured = alcohol content given by the density meter, as % vol.
  • TS = test sample of concentrated must or grape sugar, in weight.
  • MV= density of concentrated must or rectified concentrated must, in g/ml

The results are expressed to 2 decimal places and rounded to within 0.05 %vol.

  1. Characteristics of the method

8.1.  Linearity of response

The linearity of the density meter for low ASV values is one of the critical parameters of this method. A standard range of 10 aqueous-alcoholic solutions of ASV ranging between 0 and 5%vol. was prepared. Each solution was analysed 3 times.

The response of the density meter is perfectly linear within this range as shown by the calibration line in Figure 1.

Figure 1: Linearity of determination of the ASV by electronic densitometry between 0 and 5% level

8.2.  Specificity of the method

The second critical point of this method is the distillation of viscous musts containing small quantities of alcohol. In order to verify the specificity, known quantities of ethanol (from 0.25% vol to 5% vol) were added to CMs and grape sugar. The supplemented test specimens were distilled in the conditions defined earlier, then the distillates were analysed by electronic densitometry or by hydrostatic balance.

The results are shown in Table 1. The recovery rate is satisfactory, ranging between 88% and 99%. As shown by the line in Figure 2, the method is specific (slope in the vicinity of 1, intercept point in the vicinity of 0).

Table 1: Recovery rate for determination of the acquired ASV of CMs and Grape Sugar

Test specimen

Initial content (%vol.)

Added content (%vol.)

Recovered content (%vol.)

Recovery rate (%)

CM 1

0.00

0.25

0.22

88

CM 1

0.00

1.00

0.98

98

Grape Sugar (RCM) 1

0.00

1.00

0.94

94

Grape Sugar (RCM) 1

0.00

2.00

1.97

99

CM 2

0.00

0.50

0.44

88

Grape Sugar (RCM)2

0.00

5.00

4.94

99

 

Figure 2 : Specificity of determination of the acquired ASV of CMs and Grape Sugar

8.3.  Repeatability

The repeatability of the method was determined using 20 test specimens of CM or grape sugar supplemented with alcohol or not. Each CM or RCM test specimen was analysed 3 times, in order to ensure identical conditions. The repeatability limits obtained are as follows:

Table 2: Repeatability of determination of the acquired ASV of CMs and Grape Sugar

Repeatability for electronic densitometry

Calculated value

Standard deviation

0.009

CV or RSD as %

0.9%

r limit

0.024 %vol.

r limit as %

3%

Repeatability for Hydrostatic balance

Calculated value

Standard deviation

0.013

CV or RSD as %

1.7%

r limit

0.038 %vol.

r limit as %

5,3%

8.4.  Reproducibility

The reproducibility of the results is determined by analysing the same must twice, at different dates during a given period of time. The results are given in Table 3.

Table 3 - Reproducibility of determination of the acquired ASV of CMs and grape sugar

Reproducibility for electronic densitometry

Calculated value

Standard deviation

0.043

CV or RSD as %

3%

R limit

0.12%vol.

R limit as %

9%

Reproducibility for Hydrostatic balance

Calculated value

Standard deviation

0.026

CV or RSD as %

3.4%

R limit

0.076%vol.

R limit as %

10.6%

8.5.  Detection and quantification limits

The limits of detection (LD) and quantification (LQ) estimated based on the linearity study are as follows:

  • LD = 0.01%vol.
  • LQ = 0.05%vol.

The quantification limit was verified by analysis of musts having an ASV at a concentration level of 0.05%vol.

8.6.  Uncertainty

Uncertainty, evaluated based on the reproducibility standard deviation, is 0.10%vol.

Sucrose by high-performance liquid chromatography (Type-IV)

OIV-MA-F1-04 Sucrose by High-Performance Liquid Chromatography

Type IV method

 

  1. Principle

For testing and determination by high-performance liquid chromatography: the sucrose is separated in a column of alkylamine-bonded silica and detected by refractometry. The result is quantified by reference to an external standard analysed under the same conditions.

Note: Authentication of a must or of a wine may be checked by the method using NMR of deuterium described for detecting the enrichment of musts, rectified concentrated musts and wines.

The chromatographic conditions are given for guidance.

  1. Reagents

2.1.  Purified water for laboratory use and of quality EN ISO 3696..

2.2.  HPLC quality acetonitrile ( CN) – CAS Number 75-05-8

2.3.  Sucrose – CAS Number 57-50-1

2.4.  Mobile phase: acetonitrile-water (80:20 v/v)., previously subjected to membrane filtration (0.45 μm); the composition of the mobile phase is given as an example.

This mobile phase must be degassed before being used.

2.5.  Standard solution: 1.2 g/l aqueous sucrose solution. Filter using a 0.45 μm membrane filter. (The concentration of the standard solution is given as an example.)

  1. Equipment
    1.   High-performance liquid chromatograph equipped with:
  • 10 μl loop injector (as an example)
  • a detector: a differential refractometer or an interferometer refractometer
  • an alkylamine-bonded silica column, length 25 cm, internal diameter 4 mm (as an example)
  • a guard column filled with the same phase (as an example)
  • an arrangement for insulating the guard column and analytical columns or for maintaining their temperature (30 ° C),
  • a recorder and, if required, an integrator,
  • mobile phase flow rate: 1 ml/min (as an example).
    1.   Equipment for membrane filtration (0.45 μm).
  1. Procedure

4.1.  Preparation of sample:

Use the solution obtained by diluting the rectified concentrated must to 40 % (m/v) as described in Annex H 'Total acidity', section 5.1., and filtering it using a 0.45 μm membrane filter.

4.2.  Chromatographic determination

Inject in turn into the chromatograph 10 μl of the standard solution and 10 μl of the sample prepared as described in 4.1.

Repeat these injections in the same order.

Record the chromatogram.

The retention time of the sucrose is approximately 10 minutes.

The sample volume and sequence are given for guidance. The chromatographic determination can also be done with a calibration curve

  1. Calculations

 

For the calculation, use the average of two results for the standard solution and the sample.

Let C be the sucrose concentration in g/l of the 40 % (m/v) solution of rectified concentrated must.

The sucrose concentration in g/kg of the rectified concentrated must is then:

  1. Expression of results

 

The sucrose concentration is expressed in grams per kilogram, to one decimal place.

  1. Characteristics of the method

Repeatability (r)

  • r = 1.1 g/kg must

Total acidity (Type-IV)

OIV-MA-F1-05 Total acidity

Type IV method

 

  1. Definition

The total acidity of the rectified concentrated must is the sum of its titrable acidities when it is titrated to pH 7 against a standard alkaline solution.

Carbon dioxide is not included in the total acidity.

  1. Principle of the method

2.1.  Potentiometric titration or titration with bromothymol blue as an indicator and comparison with an end-point colour standard.

  1. Reagents

3.1.  Buffer solutions

3.1.1.      pH 7.0:

monopotassium phosphate, (

107.3 g

1 M sodium hydroxide (NaOH) solution

500 ml

Water to

1000 ml

3.1.2.      pH 4.0

Solution of potassium hydrogen phthalate, 0.05 M, containing 10.211 g of potassium hydrogen phthalate (C8H5KO4) per litre at 20 °C.

Note: commercial reference buffer solutions traceable to the SI may be used.

For example:

  • pH 1.679 0.01 at 25°C
  • pH 4.005 0.01 at 25°C
  • pH 7.000 0.01 at 25°C
    1.   0,1 M sodium hydroxide (NaOH) solution.
    2.   4 g/l bromothymol blue indicator solution:

Bromothymol blue (

4 g

Neutral ethanol 96 % vol

200 ml

Dissolve and add:

Water free of

200 ml

1 M sodium hydroxide solution sufficient to produce blue-green colour (pH 7) approximately

7.5 ml

Water to:

1000 ml

  1. Apparatus

 

4.1.  Potentiometer with scale graduated in pH values, and electrodes.

As a reminder, the glass electrode must be kept in distilled water. The calomel/saturated potassium chloride electrode must be kept in a saturated potassium chloride solution. A combined electrode is most frequently used: it should be kept in distilled water.

4.2.  Conical flask 100 ml.

  1. Procedure

5.1.  Preparation of sample:

Introduce 200 g of accurately weighed rectified concentrated must. Make up to the mark with 500 ml water. Homogenize.

5.2.  Potentiometric titration

5.2.1.      Zeroing of the apparatus

Zeroing is carried out before any measurement is made, according to the instructions provided with the apparatus used.

5.2.2.      Calibration of the pH meter

The pH meter must be calibrated at 20°C using standard buffer solutions traceable to the SI. The pH values selected must encompass the range of values that may be encountered in musts. If the pH meter used is not compatible with calibration at sufficiently low values, a verification using a standard buffer solution linked to the SI and which has a pH value close to the values encountered in the musts may be used.

5.2.3.      Method of measurement

Into a conical flask (4.4), introduce a 50 ml of the sample, prepared as described in 5.1.

Add about 10 ml of distilled water and then add the 0.1 M sodium hydroxide solution (3.2) from the burette until the pH is equal to 7 at 20 °C. The sodium hydroxide must be added slowly and the solution stirred continuously.

Let n ml be the volume of 0.1 M NaOH added.

5.3.  Titration with indicator (bromothymol blue)

5.3.1.      Preliminary test: end-point colour determination.

Into a conical flask (4.4) place 25 ml of boiled distilled water, 1 ml of bromothymol blue solution (3.3) and 50 ml of the sample prepared as in (5.1).

Add the 0.1 M sodium hydroxide solution (3.2) until the colour changes to blue-green.

Then add 5 ml of the pH 7 buffer solution (3.1)

5.3.2.      Measurement

Into a conical flask (4.4) place 30 ml of boiled distilled water, 1 ml of bromothymol blue solution (3.3) and 50 ml of the sample, prepared as described in 5.1.

Add 0.1 M sodium hydroxide solution (3.2) until the same colour is obtained as in the preliminary test above (5.3.1).

Let n ml be the volume of 0.1 M sodium hydroxide added.

  1. Expression of results

6.1.  Method of calculation

The total acidity expressed in milliequivalents per kilogram of rectified concentrated must is given by:

The total acidity expressed in milliequivalents per kilogram of total sugars is given by:

P = % concentration (m/m) of total sugars.

It is recorded to one decimal place.

  1. Characteristics of the method

Repeatability (r)

  • r = 0.4 meq /kg total sugars

Reproducibility (R)

  • R = 2.4 meq /kg total sugars

pH (Type-IV)

OIV-MA-F1-06 pH

Type IV method

 

  1. Principle

The difference in potential between two electrodes immersed in the liquid under test is measured. One of these two electrodes has a potential which is a function of the pH of the liquid, while the other has a fixed and known potential and constitutes the reference electrode.

  1. Reagents

2.1.  Buffer solutions

2.1.1.      Saturated solution of potassium hydrogen tartrate, containing at least 5.7 g of potassium hydrogen tartrate per litre () at 20 °C. (This solution may be kept for up to two months by adding 0.1 g of thymol per 200 ml.) pH/temperature

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

2.1.2.      Solution of potassium hydrogen phthalate, 0.05 M, containing 10.211 g of potassium hydrogen phthalate () per litre at 20 °C.

(Maximum keeping period, two months.)

pH/temperature

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

2.1.3.      Solution containing:

monopotassium phosphate,

3.402 g

dipotassium phosphate,

4.354 g

Water to

1000 ml

(maximum keeping period, two months)

pH/temperature

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

Note: commercial reference buffer solutions traceable to the SI may be used.

For example:

  • pH 1.679 0.01 at 25°C
  • pH 4.005 0.01 at 25°C
  • pH 7.000 0.01 at 25°C
  1. Apparatus
    1.   pH meter with a scale calibrated in pH units and enabling measurements to be made to at least 0.01.
    2.   Electrodes:
      1.       Glass electrode.
      2.       Calomel-saturated potassium chloride reference electrode
      3.       Or a combined electrode.
  1. Procedure
    1.   Preparation of the sample for analysis

Dilute the rectified concentrated must with water to produce a concentration of 25 0.5 % (m/m) of total sugars (25° Brix).

If P is the percentage concentration (m/m) of total sugars in the rectified concentrated must, weigh a mass of:

2500/P

and make up to 100 g with water.

The water used must have a conductivity below 2 microsiemens per cm.

4.2.  Zeroing of the apparatus

Zeroing is carried out before any measurement is made, according to the instructions provided with the apparatus used.

4.3.  Calibration of the pH meter

The pH meter must be calibrated at 20°C using standard buffer solutions traceable to the SI. The pH values selected must encompass the range of values that may be encountered in musts. If the pH meter used is not compatible with calibration at sufficiently low values, a verification using a standard buffer solution linked to the SI and which has a pH value close to the values encountered in the musts may be used.

4.4.  Determination

Dip the electrode into the sample to be analysed, the temperature of which should be between 20 and 25 °C and as close as possible to 20 °C.

Read the pH value directly off the scale.

Carry out at least two determinations on the same sample.

The final result is taken to be the arithmetic mean of two determinations.

  1. Expression of results

The pH of the 25 % (m/m) (25 ° Brix) solution of rectified concentrated must is quoted to two decimal places.

  1. Characteristics of the method

Repeatability (r)

  • r = 0.07

Reproducibility (R)

  • R = 0.07

Sulphur dioxide (Type-IV)

OIV-MA-F1-07 Sulphur dioxide

Type IV method

 

  1. Definitions

Free sulphur dioxide is defined as the sulphur dioxide present in the must in the following forms:

The equilibrium between these forms is a function of pH and temperature:

represents molecular sulphur dioxide.

Total sulphur dioxide is defined as the total of all the various forms of sulphur dioxide present in the must, either in the free state or combined with its constituents.

  1. Materials

Total sulphur dioxide is extracted from the previously diluted rectified concentrated must by entrainment at high temperature (approximately 100 °C).

2.1.  Reagents

2.1.1.      Phosphoric acid, 85 % (H3PO4) (ρ20 = 1.71 g/ml).

2.1.2.      Hydrogen peroxide solution, 9.1 g H2O2/litre (three volumes).

2.1.3.      Indicator reagent:

methyl red

100 mg

methylene blue

50 mg

alcohol 50 % vol

100 ml

2.1.4.      Sodium hydroxide solution (NaOH), 0.01 M.

2.2.  Apparatus

2.2.1.      The apparatus used should conform to the diagram shown below, particularly with regard to the condenser.

Fig. 1 The dimensions given are in millimetres. The internal diameters of the four concentric tubes forming the condenser are 45, 34, 27 and 10 mm.

 

The gas feed tube to the bubbler B ends in a small sphere of 1 cm diameter with 20 0.2-mm diameter holes around its largest horizontal circumference. Alternatively, this tube may end in a frit glass plate which produces a large number of very small bubbles and thus ensures good contact between the liquid and gaseous phases.

The gas flow through the apparatus should be approximately 40 litres per hour. The bottle on the right of the diagram is intended to restrict the pressure reduction produced by the water pump to 20 to 30 cm of water. To regulate the vacuum to its correct value, a flowmeter with a semi-capillary tube should be installed between the bubbler and the bottle.

2.2.2.      A microburette.

  1. Procedure
    1.   For rectified concentrated musts, use the solution obtained by diluting the sample to be analysed to 40 % (m/v) as indicated in the chapter 'Total acidity', section 5.1. Introduce 50 ml of this solution and 5 ml of phosphoric acid (2.2.1) into the 250 ml flask A of the entrainment apparatus. Connect the flask to the apparatus.
    2.   Place 2 to 3 ml of hydrogen peroxide solution (2.2.2) in the bubbler B, neutralize with the 0.01 M sodium hydroxide solution (2.2.4) and bring the must in the flask A to the boil using a small flame of 4 to 5 cm height which should directly touch the bottom of the flask. Do not put the flask on a metal plate but on a disc with a hole of approximately 30 mm diameter in it. This is to avoid overheating substances extracted from the sample that are deposited on the walls of the flask.

Maintain boiling while passing a current of air (or nitrogen). Within 15 minutes the total sulphur dioxide has been carried over and oxidized. Determine the sulphuric acid which has formed by titration with the 0.01 M sodium hydroxide solution (2.2.4).

Let n ml be the volume used.

  1. Calculation

Total sulphur dioxide in milligrams per kilogram of total sugars (50 ml prepared test sample (3.1):

(where P = percentage concentration (m/m) of total sugars

  1. Expression of results

 

Total sulphur dioxide is expressed in mg/kg of total sugars.

  1. Characteristics of the method

 

Repeatability (r)

  • 50 ml test sample < 50 mg/l; r = 1 x 250/P mg/kg of total sugars

Reproducibility (R)

  • 50 ml test sample < 50 mg/l; R = 9 x 250/P mg/kg of total sugars

Chromatic properties (Type-IV)

OIV-MA-F1-08 Chromatic properties

Type IV method

 

  1. Principle of the method

The absorbance of the rectified concentrated must is measured at 425 nm through a pathlength of 1 cm after dilution to bring the sugar concentration to 25 % (m/m) (25° Brix)

  1. Apparatus

 

2.1.   Spectrophotometer enabling measurements to be made between 300  and 700 nm.

2.2.   Glass cells with optical paths of 1 cm.

2.3.   Membrane filter of pore diameter 0.45 μm.

  1. Procedure

3.1.   Preparation of the sample

Use the solution with a sugar concentration of 25 % (m/m) (25° Brix) prepared as described in the chapter 'pH', section 4.1. Filter through a membrane filter of pore diameter 0.45 μm.

3.2.   Determination of absorbance

Zero the absorbance scale at a wavelength of 425 nm using a cell with an optical path of 1 cm containing distilled water.

Measure the absorbance A at the same wavelength of the solution containing 25 % sugar (25° Brix) prepared as in 3.1 and placed in a cell with an optical path of 1 cm.

  1. Expression of results

 

The absorbance at 425 nm of the rectified concentrated must in a solution with 25 % sugar (25° Brix) is quoted to two decimal places.

Repeatability (r)

  • r =  0.01 AU at 25°Brix

Total cations (Type-I)

OIV-MA-F1-09 Specific methods for the analysis of grape sugar

Type I method

ANNEX A: TOTAL CATIONS

  1. Principle

The test sample is treated by a strongly acid cation exchanger. The cations are exchanged with H+. Total cations are expressed by the difference between the total acidity of the effluent and that of the test sample.

  1. Apparatus

2.1.  Glass column of internal diameter 10 to 11 mm and length approximately 300 mm, fitted with a drain tap.

2.2.  pH meter with a scale graduated at least in 0.1 pH units.

2.3.  Electrodes:

  • glass electrode, kept in distilled water,
  • calomel/saturated potassium chloride reference electrode, kept in a saturated solution of potassium chloride,
  • or a combined electrode, kept in distilled water.
  1. Reagents

3.1.  Strongly acid cation exchange resin in H+ form pre-swollen by soaking in water overnight.

3.2.  Sodium hydroxide solution, 0.1 M.

3.3.  Paper pH indicator.

The water used must be purified water for laboratories, with specific conductivity below 2 μS cm-1 at 20°C, for example EN ISO 3696 type II water.

  1. Procedure

The pH meter must be calibrated according to the method OIV MA AS313-15

4.1.  Preparation of sample

Use the solution obtained by diluting the rectified concentrated must to 40% (m/v). Introduce 200 g of accurately weighed rectified concentrated must. Make up to the mark with 500 ml water. Homogenize.

4.2.  Total acidity of the rectified concentrated must

Titrate the acidity of the concentrated must in 100 ml of sample prepared as in 4.1 with the 0.1M sodium hydroxide solution until the pH is equal to 7 at 20 °C. The alkaline solution should be added slowly and the solution continuously shaken. Let n1 ml be the volume of 0.1 M sodium hydroxide solution used.

4.3.  Preparation of the ion exchange column

Introduce into the column approximately 10 ml pre-swollen ion exchanger in H+ form. Rinse the column with distilled water until all acidity has been removed, using the paper indicator to monitor this.

4.4.  Ion exchange

Pass 100 ml of the rectified concentrated must solution prepared as in paragraph 4.1 through the column at the rate of one drop every second. Collect the effluent in a beaker. Rinse the column with 50 ml of distilled water. Titrate the acidity in the effluent (including the rinse water) with the 0.1 M sodium hydroxide solution until the pH is 7 at 20°C. The alkaline solution should be added slowly and the solution continuously shaken. Let n2 ml be the volume of 0.1 M sodium hydroxide solution used.

  1. Expression of the results

The total cations are expressed in milliequivalents per kilogram of total sugar to one decimal place.

5.1.  Calculations

Total acidity of the rectified concentrated must in milliequivalents per kilogram:

  • a=2.5 n1

Acidity of the effluent expressed in milliequivalents per kilogram of rectified concentrated must:

  • E= 2.5 n2.

Total cations in milliequivalents per kilogram of total sugars:

  • P=percentage concentration (m/m) of total sugars.

5.2.  Repeatability (r)

  • r = 0.3

Heavy metals by ETAAS (Type-IV)

OIV-MA-F1-10 Specific methods for the analysis of grape sugar

Type IV method

Annex D: Heavy metals

D.1 Determination of lead level by ETAAS

Heavy metals are described in detail in the steps for preparing grape sugar samples (concentrated musts and MCR rectified concentrated musts) for determining lead content.

The instrumentation and computer tools used in the testing laboratories vary and change.

As a result, general criteria for calibration and metrics are given.

  1. Warning

Security precautions – Operators must protect their hands and eyes when handling acids. Acids must be handled under an appropriate fume hood.

  1. Scope

This method specifies an electrothermal atomic absorption spectrometry method (ETAAS) for determining the lead content of rectified concentrated musts between 10 µg/kg to 200 μg/kg.

  1. Normative references

ISO 3696, Water for analytical laboratory use - Specification and test methods

  1. Principle

In Electrothermal Atomic Absorption Spectrometry (ETAAS), a sample volume is inserted into a graphite tube which may be heated to over 2800°C. When the temperature is gradually increased, the sample matrix dries and thermal decomposition and dissociation occur. For most elements, the peak height is proportional to the concentration of the element in the solution, although in a very large number of cases, it is preferable to work with the peak area.

  1. Reagents and solutions

Unless otherwise indicated, only use lead-free reagents of recognised analytical quality.

5.1.   Demineralised, ultra-pure water with resistivity above 18 MΩ, following ISO 3696.

5.2.   Nitric acid of a concentration above 60% (Normapur quality).

5.3.   Ammonium dihydrogen phosphate

5.4.   Matrix modifier: , 6% solution

Pour 3g of into a 50 ml volumetric flask. Dissolve and bring to volume with demineralised water.

5.5.   Magnesium nitrate Mg( to 6 molecules of water

5.6.   0.5% magnesium nitrate solution (keep refrigerated).

Pour 0.5g of magnesium nitrate into a 100 ml volumetric flask. Dissolve and bring to volume with demineralised water. Keep this solution refrigerated for a maximum of 15-20 days.

5.7.   Certified mono element lead solution(s) (at 1000 mg/l)

5.8.   10 mg/l lead solution

Place 1 ml of the stock solution (5.7) and 10 ml of nitric acid (5.2) in a 100 ml flask. Bring to volume with ultra-pure water (5.1).

5.9.   100 μg/l lead solution

Place 1 ml of the stock solution (5.8) in a 100 ml flask. Add 10 ml of nitric acid (5.2). Bring to volume with ultra-pure water (5.1).

5.10.         Triton X-100 (1% v/v)

5.11.         Blank test: 10% nitric acid

Preparation of the calibration range

The number of calibration solutions depends on the required precision. At least five standards are required. The precision and accuracy of the results may be verified by analysing a control sample.

It should be stressed that the linearity of the calibration curve is often limited.

Correct the absorbance values of the calibration solutions by subtracting the absorbance value of the blank test. To plot a calibration curve or calculate the calibration function, use the values obtained as well as the analyte concentration of the calibration solutions.

Depending on the type of apparatus, it is possible to work with an autosampler to direct inject predetermined volumes from the 100 μg/l solution in order to have a calibration range of 0 to 100 μg/l (e.g. 0, 10, 25, 50, 100 µg/l). It is also possible to prepare calibration solutions separately.

Note 1: A smaller volume of test sample may be used to determine lead content greater than 100 μg/l.

 

  1. Apparatus and equipment

6.1.   Atomic absorption spectrometer equipped with an electrothermal atomiser, a hollow-cathode lamp adapted for lead functioning with the manufacturer-recommended current, an automatic correction device for background noise and a computer reading system or high-speed graphic recorder. A correction of background noise should be used with electrothermal atomic absorption spectrometry. The minimum acceptable technical specification is based on deuterium. A correction of the Zeeman background noise is preferable if the signal from background noise is high. To increase the analyte signal-to-noise ratio, the use of a graphite tube with a pyrolytic platform is recommended.

Note 2: a wavelength of 217.0 nm can be used for lead. The sensitivity is about two times higher than that obtained at 283.3 nm. However, since the noise and risk of interference are greater, it is necessary to work with a Zeeman background noise correction system.

 

6.2.   Precision balance accurate to 0.1 mg

6.3.   Class A graduated pipettes: 0.5 ml, 1 ml, 5 ml

6.4.   Class A volumetric flasks: 50 ml and 100 ml

Note 3: the material in contact with the sample must remain in a 10% nitric acid solution (5.2) for at least 12 hours and must be subsequently rinsed several times with demineralised water (5.1).

  1. Sampling

 

Preparation of the sample for testing

In a 50 ml flask (6.4), pour 10 g of the sample accurate to 0.1 mg, 5 ml of nitric acid (5.2), and 0.5 ml of triton X-100 (1% v/v) (5.10). Bring to 50 ml with the demineralised water (5.1) and homogenise.

  1. Procedure

Adjust the instrumental parameters and align the electrothermal atomiser following the manufacturer's instructions in order to derive maximum benefit from the background noise correction system. Adjust the sampler in the same way. Determine the optimal parameters for the electrothermal atomiser for the particular type of atomiser and sample volume, as recommended by the apparatus manufacturer, in order to cover the optimal measuring range. Adjust the baseline of the apparatus to zero. Verify the stability of zero in the atomisation system by executing the predefined temperature programme for the white heating of the graphite atomiser. The following furnace settings may be used:

phase

temperature

 level-off

 rise (ramp)

 type of gas

 gas speed

 reading

(°C)

 (s)

 (°C/s)

(l/mn)

1

130

 15

 10

 argon

0.2

no

2

350

 5

 25

 argon

 0.2

no

3

500

 5

 50

 argon

 0.2

 no

4

750

 10

 100

 argon

 0.2

 no

5

1900

 3

 0

 argon

 stopped

yes

6

2500

 3

 0

 argon

 0.2

no

7

100

 10

 0

 argon

 0.2

no

Using an autosampler, inject a set volume of the solution. Add a set volume of modifier solution and atomise the blank test (5.11), the calibration solutions and the diluted test sample solutions  by order of increasing response of the apparatus. If the peak height (or the peak area) of the test sample is greater than the value of the calibration solution with the highest concentration, a lower test sample volume must be used.

External calibration

The following programme for the sampler is given as an example (volume in µl) to determine the lead content through external calibration.

blank test

sample

standard 1

 standard 2

 standard 3

 standard 4

10 μg/l

 25 μg/l

50 μg/l

100 μg/l

 blank (HNO3 10%)

5.0

 thinner (HNO, 10%)

4.5

3.7

2.5

0

 sample

5.0

 stock solution

(Pb 100 μg/l)

0.5

1.3

2.5

5.0

  6%

4.0

4.0

4.0

4.0

4.0

4.0

Mg( 0.5%

2.0

2.0

2.0

2.0

2.0

2.0

 total volume

11.0

11.0

11.0

11.0

11.0

11.0

Atomise each solution at least two times and, if the reproducibility is acceptable in compliance with the quality control system used in the laboratory, calculate the average of readings. If necessary, reset the baseline to zero.

Addition method

It is also possible to use the addition method to reduce the effect of non-spectral interferences between the standards and the samples, as long as the calibration curve is linear in the absorbance range used.

Transfer identical volumes of the testing sample in three receptacles (for example, autosampler cups). Add a small quantity of standard solution to two of the receptacles, calculated in order to obtain a concentration for the samples, respectively, of between 100% and 200% higher than the concentration in the original sample. Add the same quantity of water in the third receptacle. Carefully mix the solutions. Measure the integrated absorbance of each solution and plot a curve with the added concentration on the x-axis and the measured absorbance on the y-axis. Determine the analyte concentration of the reagent blank solution or the test blank solution in the same manner.

The following programme for the sampler is given as an example (volume in μl) to determine the lead content using the addition method.

blank test

sample

addition 1

addition 2

25 μg/l

50 μg/l

blank (HNO3 10%)

5.0

thinner (HNO, 10%)

2.5

2.5

1.2

0

sample

5.0

5.0

5.0

stock solution

(Pb 100 μg/l)

1.3

2.5

6 %

1.0

1.0

1.0

1.0

Mg( 0.5%

2.0

2.0

2.0

2.0

total volume

10.5

10.5

10.5

10.5

  1. Calculation

The apparatus software establishes the calibration graph (absorbance as a function of lead concentration in μg/l). It gives the lead concentration of the samples. Take into account any dilution, if applicable.

  1. Precision parameters

For a lead concentration inferior to 150 μG/kg:

r (Repetability) = 15 μg/kg

R (Reproducibility) = 25 μg/kg

  1. Bibliography
  • Laboratoire SCL33. Détermination du plomb dans le vin par atomic absorption spectrometry (four-graphite). Manuel d’instructions, 2010.
  • Laboratoire SCL33. Détermination du plomb dans les aliments solides par atomic absorption spectrometry (four-graphite). Manuel d’instructions, 2010.
  • Rodriguez Garcia J.C. Desarrollo de metodologías para la determinación de metales en miel mediante ETAAS y estudio quimiométrico de su empleo como bioindicador. Universidad de Santiago de Compostela, Facultad de Ciencias, Campus de Lugo, 2006.

Heavy metals by ICP-MS (Type-IV)

OIV-MA-F1-11 Specific methods for the analysis of grape sugar

Type IV method

 

ANNEX D.2: HEAVY METALS

 

Determination of lead content by Inductively Coupled Plasma Mass Spectrometry (ICP-MS).

The analysis of Pb in rectified concentrated grape musts can also be performed applying the method OIV/OENO 344/2010 (Multielemental Analysis Using ICP-MS), with the following modification added at the end of point N°5 (Sample preparation):

5.      Sample preparation

This method can also be applied to the analysis of Pb in rectified concentrated grape musts. For this purpose, a prior mineralisation of the sample is required. A digestion of the samples in a close vessel microwave system is recommended. The following procedure is given as a way of example:

 

Ad 1 g of must, 2 ml of nitric acid (3.4) and 8 ml of water (3.1) in a microwave vessel, and apply the following microwave digestion programme:

Stage

ramp

°C

Hold

1

20 min

200

20 min

Once the samples have been digested, transfer them to a 50 ml plastic tube (4.6), dilute with water (3.1) to 30g and homogenize.

Determination of meso-inositol, scyllo-inositol and sucrose (Type-II)

OIV-MA-F1-12 Specific methods for the analysis of grape sugar

Type II method

Determination of meso-inositol, scyllo-inositol and sucrose

 

  1. Principle

Rectified Concentrated Must (RCM) is mainly composed of sugars, polyalcohols and water contained in grapes. All the other organic and mineral components are removed during the rectification process.

Meso-inositol, scyllo-inositol and sucrose are determined through gas chromatography (GC) following silanisation.

The sucrose possibly found in small amounts in the RCM is stable for some months since hydrolysis is greatly slowed down due to the absence of organic and mineral acids, which are removed during the rectification process, to a very low water content, and to a high level of glucose and fructose.

  1. Reagents

2.1.  Xylitol (CAS no. 87-99-0)

Internal standard: (aqueous solution of at a precisely known concentration of about 10 g/L prepared at the time).

2.2.  Meso-inositol () (CAS no. 87-89-8)

2.3.  Scyllo-inositol () (CAS no. 488-59-5)

2.4.  Glucose (), fructose (), sucrose ()

2.5.  Bis(trimethylsilyl)trifluoroacetamide - (BSTFA) – () (CAS no. 25561-30-2)

Warning: This is a dangerous and inflammable product. Inflammable liquids and vapours may provoke serious skin burns and serious eye lesions. Wear gloves/protective clothing. Protect your eyes/face.

2.6.  Trimethylchlorosilane () – TMCS – (CAS no. 75-77-4)

Warning: This is a dangerous and inflammable product. Harmful to the skin. Provokes serious skin burns and serious ocular lesions. Toxic when inhaled. May irritate the respiratory tract. Keep away from sources of heat/sparks/free flames /heated surfaces. Do not smoke. Avoid inhaling the vapours. Wear gloves/protective clothing. Protect your eyes/face.

2.7.  Pyridine p.a. () (CAS no. 110-86-1)

Warning: This is a dangerous and inflammable product. Noxious when inhaled, in contact with the skin and when swallowed.

2.8.  Absolute ethanol () (CAS no. 64-17-5)

Warning: This is an inflammable product. Liquid and vapours easily inflammable. Keep away from sources of heat/sparks/free flames /heated surfaces. Do not smoke.

2.9.  Type 1 Water in conformity with ISO 3696 standard or deionised water with resistivity 18M cm

2.10.        The silanising reagent is also available in ready to use kits (e.g. HMDS+TMSCl+Pyridine 3:1:9 Supelco cod. 33038)

2.11.        Technical gases: nitrogen, hydrogen, helium and air for gas chromatography and for the dehydration phases

  1. Apparatus

3.1.  Gas chromatograph

3.2.  Capillary column able to guarantee a minimum efficiency of N=250,000 plates/column for sucrose at 1 g/L

For example, OV-1 (25 m x 0.30 mm x 0.15 µm) or DB-5 (60 m x 0.25 mm x 0.10 μm).

Operating conditions (only as an example):

carrier gas: pure hydrogen or helium, for gas chromatography,

Hydrogen: Warning: This is an extremely inflammable gas. Store the container in a well-ventilated place and far from flames and sparks. – Do not smoke. Avoid the piling up of electrostatic loads.

carrier gas flow rate: about 2 mL/min,

injector temperature: 250 °C,

temperature of flame ionisation detector (FID): 300 °C,

programming of temperature: 1 minute at 160 °C, 4 °C/minute up to 260 °C, constant temperature of 260 ° C for 15 minutes,

splitter ratio: about 1:20,

auxiliary gases: pure hydrogen and air for gas chromatography

3.3.  Integrator

3.4.  Microsyringe: 10 μL

3.5.  Micropipettes: 10, 100, 400 and 1000 μ

3.6.  2 mL flasks with Teflon stopper

3.7.  Oven

3.8.  Technical balance, analytical balance able to ensure an accuracy of ± 0.1 mg

3.9.  Flasks of 50 and 100 mL

3.10.        Dryer

  1. Procedure

4.1.  Preparation of the sample

In a 50 mL flask, weigh a quantity “p” of rectified concentrated must ranging between 4.9 and 5.1 g, noting the weight of the substance with the precision of 0.1 mg.

Then add 1 mL of xylitol standard solution (2.1) and bring to volume with water (2.9).

4.2.  Dehydration of the sample

After mixing, 100 μL of solution is taken and placed in a flask (3.6) where it is dried under a gentle stream of nitrogen.

100 μL of absolute ethanol (2.8) may be added to facilitate evaporation.

Note 1: In case a precise dose of sucrose is desired, the diluted solution should be prepared just before the silanisation, in order to limit hydrolysis of the sucrose in the diluted acqueous solution.

Note 2: The repeated measurements of the sucrose content have to be performed on diluted solutions prepared every time before every silanisation.

4.3.  Derivatization

The residue is carefully dissolved in 100 μL of pyridine (2.7) and 100 μL of bis (trimethylsilyl)trifluoroacetamide (2.5) and 10 μL of trimethylchlorosilane (2.6) are added. The flask is closed with the Teflon stopper and placed in the oven at 70 °C for 70 minutes.

Take the sealed flasks out of the oven and leave to cool in the dryer in the dark at room temperature for an hour before injecting into the gas chromatograph.

The substance conserved in the sealed flask and kept in the dryer in the dark at room temperature is stable for three days.

Note 3: If working with a silanisation kit, 400 μL of reagent should be used per 100 μL of the dehydrated and diluted sample, as described in 4.1.

Note 4: The silanisation is considered successful if the solution, after a sole phase, has a clear appearance or leaves a slight, white residue. There should not be a dark residue since this would indicate an excess of non-derivatised sugar or an aged silanising substance.

Note 5: Should there be a white suspension, wait until the solid matter deposits on the bottom without centrifuging.

4.4.  Gas chromatographic analysis

1 μL is taken with a syringe (3.4) and injected into the chromatograph with the aforementioned splitter.

The chromatogramme should not show a confluence of peaks (sign of a badly performed silanisation), but characteristic peaks as shown in the attached figures. (Fig.9-Fig.12).

4.5.  Peak integration criteria

Integrate the gas chromatographic peaks with respect to the horizontal baseline. In case of peaks that are not perfectly resolved, trace the horizontal baseline starting from the deeper valleys that delimit the peak in question. Trace a vertical line downwards starting from the valleys of the peaks up to the baseline to identify the peak area.

Do not use the valley-valley integration method.

An example of the application of these criteria is given in Figure 10 for the internal standard, in Figure 11 for the inositols and in Figure 12 for the sucrose.

Note 6: In case a precise dose of sucrose is desired, it is important to respect the integration criteria explained in paragraph 4.4. and shown in Figure 4.

  1. Calculations

5.1.  Calculation of response factors

 Note: instead of the calculation of response factors a calibration curve can be used

5.1.1.     A solution is prepared containing:

  • 60 g/L of glucose,
  • 60 g/L of fructose,
  • 1 g/L of meso-inositol,
  • 1 g/L of sucrose,

(weigh 60 g of glucose and 60 g of fructose with precision 1 g; then 1 g of meso-inositol and 1 g of sucrose with precision 0.1 mg) and lastly bring to volume of 1 litre with water.

5.1.2.     Silanisation of the reference solution

Carry out the operations described in paragraph 4.1 starting with  5 mL of said solution in place of the 5 g of RMC

Take 5 mL of the solution and proceed as in paragraph 4.

5.1.3.     Gaschromatographic response factors

The results for meso-inositol and sucrose with respect to xylitol are calculated from the chromatogram.

In the case of scyllo-inositol, which has a retention time lying between the last peak of the anomeric form of glucose and the peak for meso-inositol (see Figure 11), use the same response factors achieved for meso-inositol.

Where: = area of the meso-inositol peak; = area of the sucrose peak; = area of the internal standard peak; = concentration of meso-inositol in mg/L; = concentration of sucrose in mg/L; = concentration of internal standard in mg/L, the following formula is true:

The solution for the calculation of the response factors has to be prepared and analysed on the same day (see note 1 of paragraph 4.1).

5.2.  Formulation of the results

Meso-inositol, scyllo-inositol and sucrose are expressed in mg/kg of Total Sugars (mg/kg TS) without decimals.

5.2.1.     Concentrations expressed in mg/L for the 10% (w/v) solution of RCM (4.1):

5.2.2.     Concentrations expressed in mg/kg of Total Sugars (mg/kg TS) for the meso-inositol and the scyllo-inositol, and for the sucrose in the RCM.

Indicating with “i” any of the three compounds:

Where “w” is the weighed amount in g of the RCM and “G” is the percentage of sugar of the RCM expressed in °Brix [or % (m/m) of sucrose]. The sugar percentage of the RCM sample should be measured using the OIV-MA-AS2-02 method.

  1. Characteristics of the method

6.1.  Critical points

The method regards the analysis of sugars and polyalcohols found in extremely small quantities in a matrix of glucose and fructose in very high concentrations. It is thus necessary to verify the method’s capacity to furnish linear responses in the range of concentrations proposed and that are sufficiently accurate compared with known values.

Furthermore, the method provides for gas chromatographic analysis of the silanised compounds obtained through derivatisation of the sugars. These compounds are sensitive to humidity and tend to deteriorate with time. It is therefore important to verify the adequacy of the instructions regarding conservation and handling of these compounds.

Lastly, sucrose is subject to hydrolysis due to the quantity of residual water in the RCM (from 30 to 45%). However, the low acidity of the matrix and the high concentration of glucose and fructose slow down the hydrolysis process and allow accurate measurements to be carried out. It is therefore important to check that the analysis timeframes are fast compared to the hydrolysis in order to allow repeatable measurements of the sucrose.

6.2.  Linearity

A series of six synthetic samples were prepared (including the blank) containing a matrix of glucose and fructose obtained by weighing equal quantities of the two sugars in relation to a 60% (w/w) content of total sugars in the initial RCM.

To five of these synthetic samples, precise amounts in increasing quantities of meso-inositol and sucrose were added so as to achieve the concentrations shown in the following table:

concentration added

No.

meso-inositol

sucrose

(mg/kg TS)

(mg/kg TS)

1

0 (blank)

0 (blank)

2

214.7

427.3

3

420.0

857.7

4

840.2

1675.8

5

1727.0

3338.0

6

2514.0

6719.0

The samples were then diluted (4.1), the diluted solution was dehydrated (4.2), silanised (4.3) and analysed with the GC (4.4-4.5).

The samples were then silanised and analysed using GC. The results were verified in order of linearity, showing on the graph the ratio between the peak areas of the meso-inositol peaks and that of the internal standard (), and the ratio between the concentration of meso-inositol and of the internal standard (in mg/L), indicated by The GC analysis was conducted twice and the following data refer to the mean of the two values.

The same treatment was applied to the sucrose as follows

Fig. 1 Linearity of meso-inositol

The linearity of the meso-inositol is highly satisfactory (R>0.998) in the entire range of concentration studied.

Fig. 2 Linearity of sucrose

In relation to sucrose, the linear relationship hypothesised over the entire range of concentrations studied did not lead to a satisfactory correlation (R=0.967) but, by narrowing down the linearity field to the synthetic sample no. 5, the correlation became comparable to that of meso-inositol (R>0.997).

Following the instructions in par. 5.1, the following response factors were obtained:

RF rel. Meso-inositol/Xylitol I.S.

RF rel. Sucrose/Xylitol I.S.

1.04 0.03 (mean σ; n=4)

0.36 0.06 (mean σ; n=4)

6.3.  Specificity

The relationship between the added meso-inositol and that determined by GC is linear in the entire measurement range studied, and the slope of the line is very close to one and intercept is very close to zero.

Fig. 3 Specificity of meso-inositol

Also, the recovery is satisfactory at between 95 and 105%, as seen in the following table:

added

(mg/kg TS)

determined by GC ±σ (n=2)

(mg/kg TS)

Recovery (%)

0

0

-

214.7

213 2

99%

420.0

419 3

100%

840.2

852 20

102%

1727.0

1668 214

100%

2514.0

2587 36

99%

As to the specificity of the sucrose, the concentrations obtained from the calculation of the added sucrose and that determined by GC conform and are in a linear relationship with each other, with a slope of one and intercept of almost zero, on the condition, however, that the concentration range is more restricted compared to that studied.

The following graph shows that the linear relationship does not extend up to the last concentration level of about 6700 mg/kg TS

Fig. 4 Specificity of sucrose

Also, the recovery is satisfactory, at between 90 and 110%, excluding the higher concentration levels, as seen in the following table:

added

(mg/kg TS)

determined by GC

σ (n=2)

(mg/kg TS)

Recovery (%)

0

0

-

427.3

423 16

99%

857.7

913 37

107%

1675.8

1852 344

111%

3338.0

3297 284

99%

6719.0

9220 19

137%

6.4.  Stability of sucrose in rectified concentrated must

A sample of the RCM with added sucrose was kept at room temperature and analysed at regular time intervals in order to see the incidence of the hydrolysis phenomenon of sucrose in RCM.              The results are summarised in the following table:

t = 0 days

t=9 days

t=53 days

Meso-inositol (mg/kg TS)

2227

2100

2052

Scyllo-inositol (mg/kg TS)

424

430

394

Sucrose (mg/kg TS)

4631

5108

4969

Both the meso-inositol and the scyllo-inositol, as well as the sucrose, do not show significant variations in concentration compared to the initial value up to 53 days after the preparation.

This fact appears to be evident in the following graph

Fig. 5 Stability over time

6.5.  Stability of the silanised sample

The silanised product obtained as described in point 4.2 was conserved as described in the same paragraph. At 24-hour intervals the silanised sample was analysed with the gas chromatograph following the procedure set out in point 4.3 and the succeeding points.

The results are described in the following table:

t=0

mean ± SD (n=3)

t=24 h

mean SD (n=3)

t=48 h

mean SD (n=3)

t=72 h

mean SD (n=3)

t=96 h

mean SD (n=3)

Meso-inositol

(mg/kg TS)

2424 109

2347 44

2358 17

2453 39

2478 15

Scyllo-inositol

(mg/kg TS)

261 7

254 2

256 4

257 3

264 1

Sucrose

(mg/kg TS)

6233 971

6500 200

6633 58

6733 321

6600 436

There are no significant differences between the results obtained from the same silanised sample up to 4 days after silanisation, adopting the measures for the conservation of the silanised sample described in point 4.2.

This fact is evident in the following graphs:

Fig. 6 Stability of Meso-inositol

Fig. 7 Stability of Scyllo-inosito

Fig. 8 Stability of Sucrose

6.6.  Precision

Precision parameters obtained in the interlaboratory test conducted in April 2014 between 8 Italian laboratories. The Ring Test was performed on a sample with added sucrose at a concentration of 1 g of sucrose / 1 kg RCM

sucrose

meso-inositol

scyllo-inositol

Number of participating laboratories

8

8

8

Number of accepted test results

23

23

23

Mean values (mg/kg TS)

1665

954

145

Repeatability

Repeatability standard deviation (Sr)

78

52

11

Relative repeatability standard deviation (%RSDr)

4.7

5.4

7.3

Repeatability limit (r)

219

146

29

HORRAT r = / RSD(R) Horwitz

0.9

1.0

1.0

Reproducibility

Reproducibility standard deviation (SR)

122

76

19

Relative reproducibility standard deviation (%RSDR)

7.4

8.0

13

Reproducibility limit (R)

343

213

55

RSD(R) Horwitz %

5.2

5.7

7.6

HORRAT R = / RSD(R) Horwitz

1.4

1.4

1.8

/

0.64

0.68

0.58

  1. Bibliography
  • Versini G., Dalla Serra A. and Margheri G. (1984). Polialcooli e zuccheri minori nei mosti concentrati rettificati. Possibili parametri di genuinità? Vignevini, 11(3), 41-47
  • Monetti A., Versini G., Dalpiaz G. and Raniero F. (1996). Sugar adulterations control in concentrated rectified grape musts by finite mixture distribution analysis of the myo-inositol and scyllo-insitol content and the D/H methyl ratio of fermentative ethanol. Journal of Agricultural and Food Chemistry, 44-8: 2194-2210.

Figures

 

Fig. 9 Chromatogram of the reference solution for the calculation of response factors

 

Fig. 10 Chromatogram of an RCM sample – Internal Standard ZONE

 

Fig. 11 Chromatogram of an RCM sample - “Inositol” ZONE

capture2.jpg

Fig. 12 Chromatogram of an RCM sample –with 0.5 g/kg sucrose added

 

Folin-Ciocalteu Index (Type-IV)

OIV-MA-F1-13 Specific methods for the analysis of grape sugar- Folin-Ciocalteu Index

Type IV method

  1. Definition

The Folin-Ciocalteu Index is (IFC) the result obtained from the application of the method described below.

This method applies to rectified concentrated must (RCM).

  1. Principle of the method

All phenolic compounds contained in RCM are oxidized by the Folin-Ciocalteu reagent. In RCM other reducing substances can interfere such as, for example, sugars and sulfur dioxide. This interference can be evaluated by measuring a "blank" devoid of phenolic substances, prepared by treating the corresponding sample with activated charcoal.

The Folin-Ciocalteu reagent is formed from a mixture of phosphotungstic acid (H3PW12O40) and phosphomolybdic acid () which, after oxidation of the reducing substances present in the RCM, is reduced to a mixture of the blue oxides of tungsten () and molybdenum (). The blue coloration produced has a maximum absorption in the region of 750 nm.

  1. Reagents

These must be of analytical reagent quality.

The water used must be distilled or water of equivalent purity.

3.1.  Chemicals

3.1.1.      Sodium tungstate dihydrate, (CAS Number: 10213-10-2);

3.1.2.      3.1.2 Sodium molybdate dihydrate, (CAS Number: 10102-40-6);

3.1.3.      Phosphoric acid solution 85 wt. % in , , ρ 20 = 1.71 g/ml (CAS Number 7664-38-2);

3.1.4.      Hydrochloric acid, HCl, ρ 20 = 1.2 g/ml (CAS Number 7647-01-0);

3.1.5.      Lithium sulfate monohydrate, (CAS Number: 10102-25-7);

3.1.6.      Bromine, (CAS Number: 7726-95-6);

3.1.7.      Sodium carbonate anhydrous, (CAS Number: 497-19-8);

3.1.8.      Activated charcoal decolorizing (CAS Number 7440-44-0).

3.2.  Folin-Ciocalteu reagent

This reagent is available commercially in a form ready for use.

It may be prepared as follows: dissolve 100 g of sodium tungstate (· 2) and 25 g of sodium molybdate (· 2) in 700 ml of distilled water. Add 50 ml of 85 % phosphoric acid (ρ 20 = 1.71 g/ml) and 100 ml of concentrated hydrochloric acid (ρ 20 = 1.19 g/ml). Bring to the boil and boil for 10 hours under reflux conditions. Then add 150 g of  lithium sulphate () and a few drops of bromine and boil once more for 15 minutes. Allow to cool and make up to one liter with distilled water.

3.3.  Anhydrous sodium carbonate, Na2CO3, made up into a 20 % w/v solution.

  1. Apparatus

Normal laboratory apparatus, particularly:

4.1.  100 ml volumetric flasks.

4.2.  Spectrophotometer capable of operating at 750 nm.

4.3.  Technical balance ( 0.01 g)

4.4.  50 ml graduated cylinder;

4.5.  50 ml beaker;

4.6.  Magnetic stirrer;

4.7.  Rapid-filtration filter papers;

4.8.  5 ml calibrated pipette;

4.9.  Optical-glass cuvette;

4.10.        Ultrasonic bath

  1. Procedure

Good repeatability of results is achieved by using scrupulously clean apparatus (volumetric flasks and spectrophotometer cells).

5.1.  Preparation of sample

Let P = percentage (m/m) of total sugars in the rectified concentrated must.

Dilute the RCM with distilled water until a total sugar concentration of  the solution equal to 25 0.5 % (m/m) (25° Brix): weigh a mass in g equal to 2500/P into a volumetric flask (4.1) and make up to 100 g with water.

5.2.  Preparation of a blank sample

Take 10 ml from solution 5.1 using the graduated cylinder (4.4), put into a 50 ml beaker (4.5) and add 0,5g of activated carbon (3.1.8).

Leave in contact for 15 minutes with the aid of a magnetic stirrer (4.6), and then filter the solution thought a rapid-filtration paper (4.7).

5.3.  Color reaction

5.3.1.      Color development in the sample

Introduce the following reagents or solutions into a 100 ml volumetric flask (4.1) strictly in the order given below:

  • 5 ml of the sample (5.1) using a pipette (4.8),
  • 50 ml of distilled water by means of a graduated cylinder (4.4) ,
  • 5 ml of Folin-Ciocalteu reagent (3.2) using a pipette (4.8),
  • 20 ml of sodium carbonate solution (3.2) by means of a graduated cylinder (4.4).

Make up to 100 ml with distilled water. Stir to homogenize. Wait 30 minutes for the reaction to stabilize.

During this period the flasks should be put in an ultrasonic bath (4.10) for 15 minutes to remove any bubbles that may interfere in the spectrophotometric measurement.

5.3.2.      Color development in blank

Proceed as described in (5.3.1) by replacing the sample (5.1) with a blank (5.2).

5.4.  Measurement

Determine the absorbance at 750 nm through an optical-glass cuvette with a path length of 1 cm, with respect to a blank (5.2).

If the absorbance is not around 0.3 an appropriate dilution should be made until the measured absorbance falls to around 0.3.

  1. Expression of results

 

6.1.  Method of calculation

The result is expressed in the form of an index obtained by multiplying the absorbance by 16, with one decimal point.

The FCI value calculated should be corrected for the blank according to the following formula:

FCI measured at 25°Brix = 16 d (A – )

where:

  • A = absorbance at 750 nm measured on the sample at 25 ± 0.5 % (m/m) (5.1)
  • = absorbance at 750 nm measured on the blank (5.2)
  • d = an appropriate factor if a dilution has been done (5.4)
  1. Method performance

The method was checked in the ICQRF laboratory in Conegliano (Italy) analyzing two RCM samples. Each sample was further enriched in SO2 at a concentration 5 mg/Kg TS (mg per Kg of total sugar). The samples were analyzed three times:

Samples

FC index at 25°Brix

Media

SD

r=2.8xSD

RCM 1

5.4

4.9

5.3

5.2

0.3

0.8

RCM 2

2.2

2.4

1.9

2.2

0.2

0.7

Further data was provided from the ASAE laboratory (Portugal):

Number of samples

Concentration range

Sr

r

SR

R

21

From 1 to 5.3

0.25

0.7

21

From 1 to 5.0

0.91

2.5