SECTION 3.1.6 - MULTIELEMENT ORGANIC COMPOUNDS

Codified File

Quantitation of glucose, malic acid, acetic acid, fumaric acid, shikimic acid and sorbic acid in wine using quantitative nuclear magnetic resonance spectrometry (1H NMR) (Type-IV)

OIV-MA-AS316-01 Quantitation of glucose, malic acid, acetic acid, fumaric acid; shikimic acid and sorbic acid in wine using quantitative nuclear magnetic resonance spectrometry ()

Type IV method

 

  1. Introduction

NMR spectroscopy is a so called primary quantitative analytical technique with broad linear ranges (5-6 orders of magnitude). Multiple suppression of water and ethanol signals can significantly increase the sensitivity for matrices containing water and ethanol (such as wine) during automated measurements. Various compounds in wine can be identified and quantified by specific signals in only one analytical run.

  1. Scope

 

The described method is suitable for the quantitative determination of glucose, malic acid, acetic acid, fumaric acid, shikimic acid at their natural concentrations in wine and in addition for the preserving agent sorbic acid.

Working range mg/L:

Glucose

600-50000

Malic acid

300-5000

Acetic acid

30-2000

Fumaric acid

20-300

Shikimic acid

20-500

Sorbic acid

20-800

  1. Abbreviations

NMR: Nuclear Magnetic Resonance

NMR :Proton Nuclear Magnetic Resonance

TSP :3 - (trimethylsilyl) propionic acid sodium salt

PULCON: PULse length based CONcentration determination

  1. Principle

The wine sample is diluted with 10% buffer in D2O. TSP is used as an internal standard to adjust the chemical shift (δ (0 ppm).  After that the sample is measured by 1H NMR. At least single water suppression has to be applied. To increase sensitivity, also suppress the signal from the ethanol. The selected wine analytes are evaluated and quantified using appropriate signals (see 11.1 Annex Table 1).

  1. Reagents and materials

The reagents used and the water (5.8) must be free from the analytes to be determined. Unless otherwise stated, solution means an aqueous solution.

5.1.   (99.9 atom % D) CAS 7789-20-0

5.2.   (trimethylsilyl) propionic acid 2,2,3,3-d4 sodium salt (TSP) (98 atom % D) CAS 24493-21-8

5.3.   Buffer-Solution pH 2.9 – 3.3 to adjust the pH of wine

For example: 1 M KH2PO4 (Potassium dihydrogen phosphate, CAS 7778-77-0, 0.1 % TSP (3 - (trimethylsilyl) propionic acid sodium salt) (5.2),

3 mM Na (sodium azide, CAS 26628-22-8) in (5.1), pH 3.10

5.4.   1 M hydrochloric acid, CAS 7647-01-0

5.5.   1 M sodium hydroxide, CAS 1310-73-2

5.6.   Buffer solutions for the calibration of electrodes

pH 4.00 and pH 2.00

(certified Reference Material, e. g. Certipur®)

5.7.   Citric acid monohydrate, CAS 5949-29-1

5.8.   Agua ultrapura, ISO 3696.

  1. Apparatus

The membrane filters (6.8) must be free from the analytes to be determined.

6.1.   5 mm NMR tubes, max. 1 % inner diameter deviation

6.2.   Spinner with template for adjustment of NMR tubes

6.3.   Device for pH measurement (0.01 pH units)

6.4.   Automatic titration system (adjustment of the pH to 0.01 pH units) alternativ manual adjustment

6.5.   NMR spectrometer, for example, 400 MHz with 5 mm probe (z-Gradient) and temperature stabilization 0.2K

6.6.   100 - 1000 μl pipettes

6.7.   1.5 ml reaction vials

6.8.   Polyvinylidene Fluoride (PVDF) membrane filter, 0.2 μm pore size, 15 mm diameter

  1. Sampling

Wine samples must be clear and have to be filtered (6.8) otherwise. For the sample preparation, wines are diluted with 10% buffer in O. TSP is used as an internal standard for referencing the chemical shift to δ 0 ppm. The final pH of the sample solutions should be 3.10 0.02.

For example, 900 μl of wine is mixed with 100 μl buffer (5.3) and the pH adjusted exactly to 3.10 (+/- 0.02 pH units) with hydrochloric acid (5.4) or sodium hydroxide (5.5) in order to use the quantification parameters given in 11.1 Annex Table 1. For this purpose, suitable automatic titration systems or manual adjustment with a sensitive pH meter should be used. From this mixture 600 μl is transferred in a 5 mm NMR tube and is directly measured.

  1. Procedure

8.1.   NMR Spectrometer and Measurement

The measurements have to be performed with water and ethanol multipresaturation suppression schemes. Several techniques for suppressing unwanted signals, such as selective multi-presaging and watergate, are available. To properly suppress the water signal, spectrometers are equipped with appropriate pulse sequences. 

The signal-to-noise ratio of the selected signals for quantification of the analytes shall be more than 10:1.

In principle, the essential parameters are as follows:

The recycling delay has to be at least 6 sec.

The measurements have to be performed at 300 K (27 °C) with temperature stability of 0.2 K without rotation.

Resolution equal or better 16 points/Hz

The sweep width (SW) must be equal or greater than 18 ppm.

The calibration and measurements of wine samples must be carried out under the same pulse angle.

8.2.   Quantification of compounds

The quantification is performed on the recommended signal areas/intensities of the analytes (see 11.1 Annex Table 1). It can be done by internal or external (PULCON) standardization and calibration. The signals of appropriate analytes have to be assigned (see 11.1 Annex Table 1). Pure standards in comparable concentrations have to be measured under the same conditions as samples in order to obtain the additional response correction factor for the analyte in question (e.g. by spiking experiments). Suitable signals of the target substances are listed in 11.1 Annex Table 1.

  1. Calculations

9.1.   Calculation with internal standard

For the quantification, appropriate signals of analytes can be evaluated according to the following formula (internal standard):

and

Masses of analyte and standard [g]

 

and

Molecular weights of analyte and standard [g/mol]

 

  and

Numbers of protons of analyte and standard

 

and

Areas for the selected peaks of analyte and standard

x

Analyte

std

Reference standard, internal standard (e.g. TSP 5.2)

CF

Correction factor – see 11.1 Annex Table 1 (if needed, obtained by spiking experiments of the analyte in question)

9.2.   Calculation with external standard, PULCON method

For the quantification, appropriate signals of analytes can be evaluated according to the PULCON method by the following formula F1. For quantification an external sample with known concentration of suitable substances for calibration is used each run, Quantref sample (citric acid 20 g/L).  The resulting quantification factor is part of the data of each sample. The Quantref sample is used to calculate qf according to formula F2. The PULCON method is based on the following formula:

F. 1

with:

  • γAn = searched analyte mass concentration (in mg/L)
  • IAn = absolute integral of analyte in sample
  • SWAn = spectral width (e.g. 20.55 ppm)
  • MAn = molar mass of the analyte  (g/mol)
  • PAn = excitation pulse length used for the sample (in μs)
  • kAn = correction factor (if needed, obtained by spiking experiments of the analyte in question)
  • SIAn = Size (e.g. 131072)
  • qf = mean value quantification factor from QuantRef
  • PRef = excitation pulse length used for the QuantRef (in μs)
  • NH, An = number of protons per analyte molecule giving this resonance
  • dAn = inner diameter of the analyte tube
  • NSAn = number of acquired FIDs for the analyte tube

F. 2

With:

  • IRef = absolute integral of the reference signal
  • SWRef = spectral width (e.g. 20.55 ppm)
  • MRef = molar mass of the reference substance  (g/mol)
  • SIRef = size (e.g. 131072 = 128k = 217)
  • γRef = mass concentration of the reference substance
  • NH, Ref  = number of protons per reference molecule giving this resonance
  • dRef  = inner diameter of sample tube for the reference tube
  • NSRef = number of acquired FIDs for the reference tube

Furthermore, it is mandatory to acquire both reference and analyte spectra respectively with the same setting for receiver sensitivity (receiver gain). It is also advisable to keep all

measurement parameters the same (temperature, the type of sample tube, SI, SW, NS) when determining qf or yAn respectively.

9.3.   Expression of results

Results should be expressed in mg/L with one decimal for minor constituents (<1 g/L) and without decimals for major constituents (>1 g/L).

  1. Precision

A ring trial was conducted to provide a realistic indication of the method performance. Details are given in Godelmann et al. 2016.

10.1.         Repeatability and reproducibility

Table 1 summarizes the relative standard deviations of the repeatability and reproducibility for the different analytes (Godelmann et al. 2016).

Table 1: Relative standard deviations of the repeatability and reproducibility, taken from the proficiency test (Godelmann et al. 2016) for the different analytes.

Glucose

Malic acid

Acetic acid

Fumaric acid

Shikimic acid

Sorbic acid

NMRP01 (Model wine)

Number of laboratories

15

14

15

14

13

14

Mean mg/L

9903

2628

1056

82.1

103.6

126.1*

RSDr %

1.5

1.7

1.4

1.5

1.8

7.5

RSDR %

5.5

4.3

7.5

12.5

5

11.9

NMRP02 (white wine)

Number of laboratories

15

14

15

14

13

15

Mean mg/L

28304

3528

868

12.1 (<LOQ)

45.8

164.6

RSDr %

1.3

1.7

1.6

4

2.1

RSDR %

4.6

14.3

9

18.3

5.1

NMRP03 (red wine)

Number of laboratories

14

9

14

13

13

14

Mean mg/L

11505

240 (<LOQ)

544

29.1

34.6

149.7

RSDr %

2.2

3.6

3.1

14.7

2.7

RSDR %

4.3

7.6

9.1

20

5.4

NMRP04 (red wine)

Number of laboratories

14

11

14

13

5

Mean mg/L

12538

251

627

n.d.

61.8

10.9 (<LOQ)

RSDr %

1.7

6.6

2.7

9.4

RSDR %

3.9

11.4

5.8

15.3

NMRP05 (white wine)

Number of laboratories

14

13

14

13

13

15

Mean mg/L

30303

2615

1011

27.1

29.3

191.8

RSDr %

3.2

4.6

2.7

3

8.8

3.9

RSDR %

5

13.7

7

5.3

15.6

7

NMRP06 (red wine)

Number of laboratories

14

11

14

4

12

14

Mean mg/L

6090

267

630

n.d.

30

158.5

RSDr %

3

6.1

2.1

9.6

4.3

RSDR %

5.3

10.2

4.9

12.6

6.3

NMRP07 (white wine)

Number of laboratories

13

10

14

14

13

4

Mean mg/L

5297

8036

794

n.d.

36.2

3.2 (<LOQ)

RSDr %

1.5

3.7

2.6

11.5

RSDR %

6.3

5.9

7.4

14.7

NMRP08 (white wine)

Number of laboratories

14

14

14

13

13

6

Mean mg/L

16518

5254

301

n.d.

68.4

5.4 (<LOQ)

RSDr %

1

2.2

3

4.2

RSDR %

4.5

8.6

7.1

6.4

NMRP09 (white wine)

Number of laboratories

14

12

14

14

13

15

Mean mg/L

2091

2390

176

45.9

44.1

98

RSDr %

3.1

2.6

4.6

2.2

4.3

1.8

RSDR %

6.6

5.7

12

4.6

8.4

5.1

NMRP10 (red wine)

Number of laboratories

9

7

14

15

13

15

Mean mg/L

442 (<LOQ)

178 (<LOQ)

502

90.6

58

200.3

RSDr %

2.4

2.5

5.2

2.9

RSDR %

11.7

7.7

16.4

6.8

10.2.         Limit of detection and limit of quantification

The limit of detection (LOD) and the limit of quantification (LOQ) need to be estimated individually by the laboratories and depend on the NMR system used (particularly on the field strength). Nevertheless to give an indication the LODs and LOQs listed in Table 2 were calculated according to the instructions of the resolution OENO 7-2000 (E-AS1-10-LIMDET) on basis of sample preparation and parameters of NMR measurement previously (400 MHz, and using ethanol suppression).

Table 2: Limit of detection and limit of quantification

Analyte

LOD mg/L

LOQ mg/L

Glucose

150

600

Malic acid

90

300

Acetic acid

10

30

Fumaric acid

5

20

Shikimic acid

5

20

Sorbic acid

5

20

  1. Annex

11.1.         Table 1 Quantification Parameters, according 400 MHz, pH 3.10

Une image contenant table

Description générée automatiquement

11.2.         Trueness/Recovery

The recovery was determined for the ring test samples by comparing the mean values of the NMR method with respective analysis of the relevant parameter by the OIV method (for acetic acid enzymatic/HPLC methods and fumaric acid HPLC method were used)

The calculated recoveries are for glucose 100.3 % (n=9, 95.2 106.4), for acetic acid 108.9

% (n=10, 99.9 123), for malic acid 104.1 % (n=7, 91.4 124.1), for shikimic acid 105.2 % (n=10, 91.2 122.3), for sorbic acid 100.2 % (n=8, 97.9 102.5) and for fumaric acid 96.8 % (n=6, 80.5 104.1). Only for the parameter acetic acid were yielded always findings of above

100% with a total mean of 109%. For these findings, the correction factor of 1.28 could be the reason see 11.1 Annex Table 1. The recoveries are calculated on the basis of analysis of reference values originating from OIV methods.

Table 2 Recoveries of analytes

Analyte

Mean recovery %

n: number of ring test samples calculated

Variation %

Glucose

100.0 (n=9)

95.2 – 106.4

Malic acid

104.1 (n=7)

91.4 – 124.1

Acetic acid

108.9 (n=10)

99.9 123

Fumaric acid

96.8 (n=6)

80.5 – 104.1

Shikimic acid

105.2 (n=10)

91.2 – 122.3

Sorbic acid

100.2 (n=8)

97.9 – 102.5

11.3.         Horrat values of all compounds

Table 4

Parameter

Horrat value

Samples <LOQ

0,5-1,5

1,6-2,0

>2,0

Acetic acid

7 (0,8-1,3)

3 (1,6;1,6;1,9)

0

0

Malic acid

4 (0,9-1,5)

2 (1,6;2,0)

2 (2,8;3,1)

2

Glucose

9 (1,0-1,5)

0

0

1

Sorbic acid

7 (0,6-1,5)

0

0

3

Fumaric acid

6 (0,5-1,5)

0

0

4

Shikimic acid

5 (0,6-1,3)

5 (1.6:1.6;1.8;1.9;2,0

1 (2,1)

0

11.4.         Example for an NMR spectra

  1. Literature
  • 1.Godelmann R., Fang Fang,  Humpfer E., Schütz B., Bansbach M., Schäfer H., Spraul M., (2013), Targeted and Nontargeted Wine Analysis by 1H NMR Spectroscopy Combined with Multivariate Statistical Analysis. Differentiation of Important Parameters: Grape Variety, Geographical Origin, Year of Vintage, J. Agric. Food Chem. 61, 5610−5619
  • 2.Monakhova Y.B., Schäfer H., Humpfer E., Spraul M., Kuballa T., Lachenmeier D., (2011), Application of automated eightfold suppression of water and ethanol signals in 1H NMR to provide sensitivity for analyzing alcoholic beverages, Magn. Reson. Chem. 49,734-739
  • 3. G. Wider, L. Dreier: Measuring Protein Concentrations by NMR Spectroscopy, J. Am. Chem. Soc. 2006, 128, 2571-2576
  • 4. Godelmann R., Kost C., Patz C., Ristow R., Wachter H., (2016), Quantitation of compounds in wine using 1H NMR spectroscopy – Description of the method and collaborative study,  Journal of AOAC International Vol. 99, No. 5, 1295-1304
  • 5. Horwitz W. (1995) Protocol for the design, conduct and interpretation of method- performance studies, Pure and Applied Chemistry 67, 331-343
  • 6. Horwitz, W. (1982) Anal. Chem. 54, 67A-76A
  • 7. Peeler, J.T., Horwitz W., & Albert R. (1989) J. Assoc. Off. Anal. Chem. 72, 784-806
  • 8. Herbert-Pucheta, J.E., Mejía-Fonseca, I., Zepeda-Vallejo, L.G., Milmo-Brittingham, D., Maya, G.P. The “Wine-T1” NMR experiment of novel wine-metabolome fingerprinting with nuclear-spin relaxation DOI: 10.1051/bioconf/20191202029
  • 9. Herbert-Pucheta, J.E., Pino-Villar, C., Rodríguez, González, F., Padilla-Mata, G., Milmo-Brittingham, D., Zepeda-Vallejo, L.G. “One-shot” analysis of wine parameters in non-Saccharomyces large-scale alcohol reduction processes with one- and two-dimensional nuclear magnetic resonance, DOI: 10.1051/bioconf/20191502016
  • 10. Resolución OENO 7-2000 (E-AS1-10-LIMDET), “Estimación del límite de detección y de cuantificación de un método de análisis”
  • 11. ISO 3696.