5-(hydroxymethyl)furfural- Determination
COEI-2-HMF Determination of 5-(hydroxymethyl) furfural
- Principle
The 5-(hydroxymethyl)furfural (HMF) is determined by HPLC (sharing liquid chromatography in reverse phase).
- Apparatus and solutions
2.1. Instrumental parameters (for example)
- Chromatograph in liquid phase
- UV/visible detector
- column: octadecyl type grafted silica (C18), (length: 20 cm; internal diameter: 4.6 mm; granulometry of phase: 5 μm)
- mobile phase: ultra filtered demineralised water - methanol - acetic acid (80, 10, 3: v/v/v)
- flow: 0.5 ml/mn
- detection wave length: 280 nm
- injected volume: 20 μl
- Preparation of calibration solutions
Solution HMF at 20 mg/l:
- In a 100 ml graduated flask, introduce 20 mg of HMF weighed within 0.1 mg and complete to the graduated line with ultra filtered demineralised water,
- introduce 10 ml of this solution in a 100ml graduated flask and complete with ultra filtered demineralised water;
- the solution HMF at 20 mg/l is to be prepared each day.
- Preparation of samples
The samples and the calibration solution HMF are injected after filtration on a 0.45 μm membrane.
- Procedure
The chromatographic column is stabilised with the mobile phase for about 30 min.
Calculate the concentration of HMF of the sample from the peak surfaces.
ANALYSE ET CONTROLE DES GAZ PAR CPG
COEI-2-CONGAZ Analyses of gas control by gaseous chromatography
- Principle
The gases are controlled by chromatography in gaseous phase using a "molecular sieve" type column and detection by catharometer or flame ionisation.
- Sampling
Either use
- a stainless steel flask for sampling gas
- a Teflon sampling bag for gas.
- Injection method
Use of a unheated gas valve with a 250 μl ring.
- Separation of light cases
4.1. Column (for example)
Phase: Molecular sieve Chromosorb 101, Porapak Q
- diameter of particles 5 μm
- granulometry: 80 to 100 mesh
Dimensions: length: 2 m, internal diameter: 2 mm.
4.2. Vector Gas
-
Helium (He), flow: 3 ml/mn
- Oven temperature: 40°C isotherm
- Detector: Catharometer, Intensity 190 μA
- Separation of light hydrocarbons
5.1. Column (for example)
Wide bore
Phase: apolar, diameter of particles: 5 μm
Length: 30 m, internal diameter: 0.53 mm
5.2. Vector gas
Nature: Helium, Flow: 3 ml/mn
Oven temperature 35°C to 200°C rise: 10°C/mn
5.3. Detector: Flame ionisation, temperature 220°C.
Detection of biogenic amines by TLC
COEI-2-AMIBIO Qualitative method for detection of biogenic amines produced by lactic acid bacteria by thin-layer chromatography (TLC)
- Principle
This method determines the ability to produce biogenic amines (BA) by bacteria in liquid culture media containing the corresponding amino-acid precursor. The method permits the separation and identification of the amines histamine (HIS), tyramine (TYR), putrescine (PUT), cadaverine (CAD) and phenylethylamine (PEA) using thin layer chromatography (TLC).
- Reagents
2.1. Amino acids: L-histidine monohydrochloride, L-tyrosine di-sodium salt, L-ornithine hydrochloride, L-lysine monohydrate and L-phenylalanine;
2.2. Amines: histamine dihydrochloride, tyramine hydrochloride, 1,4-diaminobutane dihydrochloride , 1,5-diaminopentane dihydrochloride, β-phenylethylamine hydrochloride;
2.3. Dansyl chloride
2.4. Acetone
2.5. Chloroform
2.6. Triethylamine
2.7. Isopropanol
2.8. Triethanolamine
2.9. Thin-layer chromatography (TLC) plates (10 x 20 precoated plates with 0.20 mm silica gel 60 F254)
- Standard solutions
A stock of standard solutions is prepared by dissolving 0.2 g of each amine (HIS, TYR, PUT, CAD and PEA) in 10mL of 40% ethanol. The working standard solution is prepared by mixing 1 ml of each of these solutions and bringing it to a final volume of 10 mL with water.
Amines are converted to their fluorescent dansyl derivatives as follows: one volume of 250 mM Na2HPO4, 0.1 volume of 4N NaOH and 2 volumes of dansyl chloride solution (5 mg/mL dansyl chloride in acetone) are added to one volume of the sample. The mixture is homogenized with a Vortex mixer and incubated at 55° C for 1 hour in the dark.
- Microorganisms and growth conditions
O. oeni strains are cultured in pH 4.8 MRS broth (Merck), supplemented with 10% tomato juice. Strains of the genera Lactobacillus and Pediococcus are cultured in pH 6.3 MRS broth. All the bacteria are incubated at 30° C.
The broths are supplemented with biogenic-amine precursor amino acids such as histidine (5 mg/mL), tyrosine (5 mg/mL), ornithine (5 mg/mL), lysine (5 mg/mL), and phenylalanine (5 mg/mL). Samples are analysed after 9-12 days of growth.
- TLC conditions
The amines are fractionated on silica gel plates (silica gel 60 F254s). Amine-derivative extracts (10 μl) are applied 2 cm from the base of the plates with capillary pipettes. The dansylated compounds are separated by ascending development for 17 cm in chloroform:triethylamine (4:1). The spots are visualized under UV by using a transilluminator with a system for image acquisition. If a similar instrument is not available, the plate can be sprayed with isopropanol:triethanolamine (8:2) to enhance the fluorescence and visualized under a classical UV source.
The detection limit for the amines TYR, PUT, CAD and PEA is 0.01 mg/ml and the detection limit for HIS is 1 mg/mL. The method showed less sensitivity to HIS, however this detection level in the TLC method described is also adequate to detect HIS production when the bacteria is growing in a culture media supplemented with 5 mg/mL of histidine, as previously described.
- Analysis of biogenic amines from bacterial cultures
Bacterial strains are grown as described in section 4. After incubation, the broth media are centrifuged and the supernatants are analysed for BA content. Analysis of amines produced by bacterial strains is performed directly on bacterial supernatants as described above.
The separation order of the resulting amine spots from the top to the bottom of the plate are: PEA, TYR, HIS, CAD, PUT.
- Bibliography
- CostantiniA., CersosimoM., Del Prete V., Garcia-Moruno E. (2006). Production of biogenic amines by lactic acid bacteria: screening by PCR, TLC and HPLC of strains isolated from wine and must. Journal of food protection, 69 (2): 391-396.
- Garcia-MorunoE., Carrascosa A.V., Muñoz R. (2005). A rapid and inexpensive method for the determination of biogenic amines from bacterial cultures by thin-layer chromatography. Journal of food protection, 68 (3): 625-629.
- Garcia-MorunoE. A method for the determination of biogenic amines from bacterial cultures by thin-layer chromatography (TLC), 2007 OIV FV 1243
Arsenic- Determination by AAS
COEI-2-ARSENI Measuring arsenic by hydride generation and atomic absorption spectrometry
- Field of application
This method applies to the analysis of arsenic in the concentration range of 0 to 200 μg/l with prior mineralisation for oenological products.
- Description of the technique
2.1. Principle of the method
After reducing arsenic (V) into arsenic (III), arsenic is determined by hydride generation and atomic absorption spectrometry.
2.2. Principle of the analysis (figure n°1)
The peristaltic pump draws up the borohydride solution, hydrochloric acid solution and calibration or sample.
The hydride formed in the gas-liquid separator is entrained by a neutral gas (argon).
The gaseous current passes in a dessicator made up of calcium chloride.
The arsenic hydride is analysed in an quartz absorption cell in the flame of a air-acetylene burner.
The optical path of the hollow-cathode lamp of the atomic absorption spectrometer passes in the quartz cell.
- Reagents and preparation of reagent solutions
3.1. Ultra-pure demineralised water
3.2. Ultra-pure nitric acid at 65%
3.3. Potassium iodide KI
3.4. Potassium iodide at 10% (m/v)
3.5. Concentrated hydrochloric acid
3.6. Hydrochloric acid at 10% (m/v)
3.7. Sodium borohydride NaBH4
3.8. Sodium hydroxide NaOH in patches
3.9. Sodium borohydride solution at 0.6% (containing 0.5% of NaOH)
3.10. Calcium chloride CaCl2 (used as a dessicator)
3.11. Silicone antifoam
3.12. Arsenic calibration solution at 1 g/l containing 2% of nitric acid and prepared from the following acid: H3AsO4½ H20
3.13. Arsenic solution at 10 mg/l: place 1 ml of the calibration solution (3.12.) in a 100 ml flask; add 1% of nitric acid (3.2.); complete to volume with demineralised water (3.1.).
3.14. Arsenic solution at 100 μg/l: place 1 ml of the arsenic solution at 10 mg/l (3.13.) in a 100 ml flask; add 1% of nitric acid (3.2.); complete to volume with demineralised water (3.1.).
- Apparatus
4.1. Glassware:
4.1.1. graduated flasks 50 and 100 ml (class A)
4.1.2. graduated pipettes 1, 5, 10 and 25 ml (class A)
4.1.3. cylindrical vases 100 ml
4.2. Hot plate with thermostat
4.3. Ashless filter paper
4.4. Atomic absorption spectrophotometer:
4.4.1. air-acetylene burner
4.4.2. hollow-cathode lamp (arsenic)
4.4.3. deuterium lamp
4.5. Accessories:
4.5.1. vapour generator (or gas-liquid separator)
4.5.2. quartz absorption cell placed on the air-acetylene burner
4.5.3. bottle of neutral gas (argon)
- Preparation of the set of calibration solutions and samples
5.1. Set of calibration solutions 0, 5, 10, 25 μg/l
Place successively 0, 5, 10, 25 ml of the arsenic solution at 100 µg/l (3.14.) in 4, 100 ml flasks; add to each flask 10 ml potassium iodide at 10% (3.4.) and 10 ml of concentrated hydrochloric acid (3.5.); complete to volume with demineralised water (3.1.); allow to stand at room temperature for one hour.
5.2. Samples of oenological products
The sample is mineralised by wet process (cf. mineralisation methods of samples before determination by atomic absorption spectrometry) then filtered. Transfer 10 ml of filtered mineralisate to a 50 ml flask; add 5 ml of potassium iodide at 10% (3.4.) and 5 ml of concentrated hydrochloric acid (3.5.); add a drop of anti-foam (3.11.); adjust to volume with demineralised water (3.1.). Allow to stand at room temperature for one hour. Filter on an ashless filter paper.
- Procedure
6.1. Instrumental parameters of the atomic absorption spectrophotometer (given as an example)
6.1.1. oxidant air-acetylene flame
6.1.2. wave length: 193.7 nm
6.1.3. width of the monochromator’s slit: 1.0 nm
6.1.4. intensity of the hollow-cathode lamp: 7 mA
6.1.5. correction of the non specific absorption with a deuterium lamp
6.2. Analytical determination
The peristaltic pump draws up the reagent solutions (3.6.) and (3.9.) and the calibrations or samples (5.1.) or (5.2).
Present successively the calibration solutions (5.1.); wait long enough so that the hydride formed in the gas-liquid separator, passes in the absorption cell; perform an absorbance reading for 10 seconds; perform two measurements; the spectrometer’s computer software sets up the calibration curve (absorbance depending on the concentration of arsenic in μg/l).
Then present the samples (5.2.). Perform two measurements.
6.3. Self-check
Every five determinations, an analytical blank solution and a calibration are analysed in order to correct a possible deviation of the spectrometer.
- Expression of results
The results are directly printed by the printer connected to the computer.
The concentration of arsenic in oenological products is expressed in μg/kg while taking into account the test sample.
- Control pf results
The quality control is performed by placing, after the set of calibration solutions and every five samples, a reference material whose content in arsenic is known with certainty.
A control card is set up for each reference material used. The control limits were set at: +/- 2SR intra (SR intra: standard deviation of reproductibility).
- Bibliograhy
- PESQUE M., 1982. Dosage de l’arsenic dans le vin. Rapport de stage. Diplôme d’œnologue. Institut d’œnologie de Bordeaux.
- GAYE J., MEDINA B., 1998. Dosage de l’arsenic dans le vin par spectrométrie d’absorption atomique. Feuillet Vert de l’O.I.V. n°1069.
- GAYE J., MEDINA B., 1999. Arsenic dans les vins. Feuillet Vert de l’O.I.V. n°1087.
Total nitrogen- Determination
COEI-2-AZOTOT Determination of total nitrogen
- Apparatus
1.1. The apparatus used for separating NH3 is either a distillation apparatus with a rectifying column or a distillation apparatus under a current of steam (diagram) made up of:
- A 1 l flask A of borosilicate glass used as a boiler with a stopcock funnel for filling. It can be heated by a gas or electric furnace.
- An adapter C which gathers the spent liquid from the bubbler B.
- A bubbler B of 500 ml with an inclined neck; the supply tube must reach the lowest part of the flask. The out-going tube has an anti-entrainment ball that makes up the top part of the bubbler. A stop-cock funnel E allows to introduce the liquid to be treated and alkaline lye.
- A cooler 30 to 40 cm long, vertical, with a ball with fine dowel bush on the tip.
- A 250 ml conical flask for the distillate.
- Mineralisation flask, 300 ml ovoid-shaped flask with a long neck.
- Reagents
- Concentrated sulphuric acid (R).
- Mineralisation catalyser (R).
- Sodium hydroxide solution at 30% (m/m) (R).
- Boric acid solution at 4% (R).
- Hydrochloric acid solution 0.1 M.
- Mixed-based indicator with methyl red (R) and methylene blue.
- The boiler must contain acidulated water by 1 per 1 000 of sulphuric acid. It is advisable to boil this liquid before any operation, with the drain cock P open to let the CO2 escape.
- Procedure
In the mineralisation flask, introduce the test sample containing 4 to 50 mg of nitrogen. Add 5 g of mineralisation catalyser (R) and 10 ml of concentrated sulphuric acid (R), if the quantity of dry organic matter to be mineralised is below 500 mg. Increase these quantities if a higher quantity of organic matter must be used.
Heat in an open flame under a hood. The neck of the flask is maintained inclined until the solution becomes colourless and the walls of the flask are clear of carbonised products.
After cooling, dilute with 50 ml of water and cool; introduce this liquid in the bubbler B with the funnel E, then add 40 to 50 ml of sodium hydroxide solution at 30% (R) in order to obtain frank alkalinisation of the liquid. Entrain the ammoniac with the vapour by gathering the distillate in 5 ml of boric acid solution (R) placed beforehand in a receiving conical flask with 10 ml of water, with the tip of the ampoule plunged into the liquid. Add 1 or 2 drops of mixed-based indicator and gather 70 to 100 ml of distillate.
Titrate the distillate with the hydrochloric acid solution 0.1 M until the indicator turns pink violet.
1 ml of 0.1 M hydrochloric acid solution corresponds to 1.4 mg of nitrogen.
|
Apparatus for the distillation of ammoniac in a current of steam (PARNAS and WAGNER) The cocks P and E can be replaced by a plastic pipe fitting with a Mohr pinch-clamp cock. |
Benzo[a]pyrene- Determination
COEI-2-HYDCAR Aromatic polycyclic hydrocarbons
Determination of benzo(a)pyrene in oenological charbons by HPLC
- Principle
Polycyclic aromatic hydrocarbons including benzoapyrene are extracted by hexane; the solvent is evaporated and the residue is taken up by the methanol-tetrahydrofuran for analysis by HPLC.
- Apparatus and reagents
2.1. Reagents and calibrations
- Acetonitrile for HPLC
- Hexane for pesticide residues
- Tetrahydrofuran for HPLC (THF)
- Deionised and microfiltered water
- Benzo[a]pyrene for HPLC.
- Apparatus and chromatographic conditions
- octadecyl type HPLC column
- fluorimetric detector adjusted to the following detection conditions:
- excitation wave length: 300 nm,
- emission wave length: 416 nm.
Mobile phase:
- solvent A: Deionised and microfiltered water
- solvent B: acetonitrile
Variations in the composition of the solvent
|
||
TIME in min |
% solvent A |
% solvent B |
0 |
50 |
50 |
15 |
20 |
80 |
40 |
0 |
100 |
45 |
50 |
50 |
Flow 1.0 ml/mn
2.3. Preparation of reference solutions
Benzoapyrene reference solution at about 100 mg/l in a methanol/THF mixture (50/50) stored for 3 years maximum in cold conditions.
Daughter solution at about 20 μg/l, prepared extemporaneous (0.5 ml of reference solution in 50 ml of methanol/THF then 1 ml of this intermediate solution in 50 ml de methanol/THF).
2.4. Preparation of samples
2 g of oenological charbon are mixed in a 50 ml volumetric flask with 30 ml of hexane.
The polycyclic aromatic hydrocarbons are extracted for 5 min using a magnetic stirrer. The organic phase recovered by filtration is gathered in a evaporating flask and evaporated. The extract is taken up by 2 ml of a methanol/THF mixture (1/1, v/v) and injected.
- Results
The benzoapyrene content must not be higher than 1 μg/kg.
Remark: It is also possible to determine benzo[a]pyrene by chromatography in gaseous phase by an apolar capillary column with detection by mass spectrometry.
Bromine- Index
COEI-2-IBROME Bromine index
The bromine index is the quantity of bromine expressed in grammes, that 100 g of the substance can set.
- Apparatus
A graduated flask of 300 to 400 ml with an interior tube welded at the bottom, an emery stopper and a tube with a handle, compliant with the following diagram
Bromination flask 300 ml in borosilicate glass. Stopper with ground-glass joints standardised 24/40. |
- Solutions
2.1. Potassium bromate solution 0.016 M
This solution contains for 1000 ml:
Potassium bromate KBrO3 |
2.783 g |
Weigh exactly 2.783 g of potassium bromate and introduce into a 1000 ml graduated flask containing about 500 ml of distilled water; shake in order to dissolve and complete to 20°C with distilled water the volume of 1000 ml of solution. Mix and store in a flask with a glass stopper.
2.2. Iodine solution 0.05 M
Iodine I |
12.69 g |
Potassium iodide de KI |
18 g |
Water q.s.p |
1000 ml |
Weigh exactly 12.69 g of iodine, then 18 g of potassium iodide and introduce into a 1000 ml graduated flask with about 200 ml of distilled water. Allow the dissolution to operate in cold conditions with the flask being sealed. Add about 500 ml of distilled water, then shake to absorb the iodine in a vapour state and complete to 20°C with distilled water, the volume to 1000 ml of solution. Mix and store in a coloured glass flask with a glass stopper.
2.3. Sodium thiosulphate solution 0.1 M
The 0.1 M sodium thiosulphate solution contains for 1000 ml:
Sodium thiosulphate |
24.82 g |
Weigh exactly 24.82 g of sodium thiosulphate and introduce into a 1000 ml graduated flask containing about 600 ml of boiled distilled water. Shake to dissolve and complete to 20°C with boiled distilled water, the volume to 1000 ml of solution. Mix. Store away from light. Control the titre of this solution using the 0.05 M iodine solution.
- Technique
Using a tube with a handle, put about 0.50 g of potassium iodide in the recipient inside the flask; (it is convenient to make a circular mark on the tube corresponding to the salt’s weight so as not to have to weigh each dosage). Caution has to be taken so as not to introduce iodide on the external part of the flask. Then introduce the measured volume of the solution of the product to be measured, dissolved in neutral or alkaline water, in the external part of the flask, then 25 ml of potassium bromate solution 0.016 M measured with a pipette, and 2 g of pure potassium bromide. Rinse the sides with water to come to a total volume of about 100 ml, then add 5 ml of concentrated hydrochloric acid (R); quickly close the flask with the stopper, the joint being humid with distilled water; by a circular movement homogenise the content and allow to stand the prescribed time. Shake the flask vigorously so as to put the potassium iodide in contact with the liquid so as to enable the vapour bromine to react; open the flask while rinsing the joint and the stopper with a spray of distilled water, and determine iodine using 25 ml of sodium thiosulphate solution 0.1 M; titrate the excess of sodium thiosulphate with the iodine solution 0.05 M in the presence of starch paste;
Let n be the volume used:
Quantity of bromine (in mg) set by the substance to be dosed = n 0.008
Cadmium- Determination by AAS
COEI-2-CADMIU Determination of cadmium by atomic absorption spectrometry
- Principle
The cadmium is determined in solid oenological products after mineralisation by wet process or directly for liquid oenological products or put in a solution.
The determinations are performed by atomic absorption without a flame (electro-thermal atomisation in a graphite oven).
- Apparatus
2.1. Instrumental parameters (given as an example)
Spectrophotometer equipped with an atomiser with a graphite tube.
- wave length: 228.8 nm
- hollow-cathode lamp (cadmium)
- width of slit: 1 nm
- intensity of the lamp: 3 mA
- correction of continuum by the Zeeman effect
- graphite oven with a tantalised platform
- (tantalisation procedure of the platform described above)
- adjusting the oven for an analysis:
step |
temperature (°C) |
time (s) |
gas flow rate ( / mn |
type of gas |
reading of signal |
1 |
100 |
35 |
3.0 |
argon |
no |
2 |
500 |
10 |
3.0 |
argon |
no |
3 |
500 |
45 |
1.5 |
argon |
no |
4 |
500 |
1 |
0.0 |
argon |
no |
5 |
2250 |
1 |
0.0 |
argon |
yes |
6 |
2250 |
1 |
0.0 |
argon |
yes |
7 |
2500 |
2 |
1.5 |
argon |
no |
8 |
1250 |
10 |
3.0 |
argon |
no |
9 |
75 |
10 |
3.0 |
argon |
no |
2.2. Adjustments of the automatic sampler (given as an example)
volumes injected in µl |
|||
solution of Cd at 8 μg/l |
blank |
matrix modifier |
|
blank |
0 |
10 |
2 |
calibration N° 1 at 8 μg / l |
1 |
9 |
2 |
calibration N° 2 at 16 μg / l |
2 |
8 |
2 |
calibration N° 3 at 24 μg / l |
3 |
7 |
2 |
calibration N° 4 at 32 μg / l |
4 |
6 |
2 |
Sample to be dosed |
5 |
5 |
2 |
- Reagents
- Demineralised water
- Pure nitric acid for analysis at 65%
- Anhydrous palladous chloride (59% in Pd)
- Magnesium nitrate with 6 water molecules (ultra pure)
- Ammonium dihydrogenophosphate
Matrix modifier: palladous chloride and magnesium nitrate mixture (dissolve 0.25 g of PdCl2 and 0.1 g of Mg(NO3)2.6H2O in 50 ml of demineralised water) or ammonium dihydrogenophosphate at 6% (dissolve 3 g of NH4H2PO4 in 50 ml of demineralised water).
Cadmium reference solution at 1 g/l, commercial or prepared as follows: dissolve 2.7444 g Cd(NO3)2.4H2O in a solution of HNO3 0.5 M, adjust to 1 l with HNO3 0.5 M.
Cadmium solution at 10 mg/l: place 1 ml of the reference solution in a 100 ml graduated flask, add 5 ml of pure nitric acid and complete to volume with demineralised water.
Cadmium solution at 0.8 g/l: place 4 ml of the diluted solution in a 50 ml graduated flask, add 2.5 ml of pure nitric acid and complete to volume with demineralised water.
Calibration range at 0, 8, 16, 24 and 32 μg/l of cadmium.
- Preparation of samples
No preparation is necessary for liquid oenological products or in solution form; solid products are mineralised by wet process.
The blank solution is made up of a pure nitric acid solution for analysis at 1%.
- Procedure
Each calibration solution is passed right after the blank solution. Perform 2 successive absorbance readings and establish the calibration curve.
Calculate the cadmium content of the samples while taking into account the test sample of different dilutions.
Calcium- Determination by AAS
COEI-2-CALCIU Determination of calcium by atomic absorption spectrometry
- Principle
The calcium is directly determined in the liquid oenological product (or in the mineralisation solution) suitably diluted by atomic absorption spectrometry by air-acetylene flame after the addition of spectral buffer.
- Apparatus
Instrumental parameters (given as an example)
- Atomic absorption spectrophotometer
- Reducing air-acetylene flame
- Hollow-cathode lamp (calcium)
- wave length: 422.7 nm
- width of slit: 0.2 nm
- intensity of the lamp: 5 mA
- No correction of non specific absorption.
- Reagents
3.1. demineralised water
3.2. calcium reference solution at 1 g/l, commercial or prepared as follows: dissolve 5.8919 g of Ca(NO3)2.4H2O in a solution of HNO3 0.5 M, adjust at 1 l with HNO3 0.5 M.
3.3. calcium solution at 100 mg/l:
- place 10 ml of the reference solution in a 100 ml graduated flask and 1 ml of pure nitric acid.
- complete to volume with demineralised water
- concentrated hydrochloric acid (R): 35% minimum
- lanthanum solution at 25 g/l:
- weigh 65.9 g lanthanum chloride (LaCl3.6H2O) in a 250 ml cylindrical vase, transfer to a 1000 ml graduated flask with demineralised water; add to the test tube 50 ml of concentrated hydrochloric acid (R); after solubilisation, allow to cool, complete to volume with demineralised water.
- set of calibration solutions: 0, 2, 4, 6, 8 mg/l of calcium
- place successively 0, 1,0, 2,0, 3,0 and 4.0 ml of the solution at 100 mg/l of calcium in 5, 50 ml graduated flasks, add 10 ml of lanthanum solution at 25 g/l, complete to volume with demineralised water.
- Preparation of samples
4.1. Case of liquid or solution oenological products
In a 50 ml graduated flask place 10 ml of the lanthanum solution and a volume of sample as after having being completed to volume with demineralised water; the concentration is below 8 mg/l.
4.2. Case of solid oenological products
Proceed with mineralisation by dry process;
Put in each solution of the set the same quantity of acid used for putting cinders in solution or mineralisation (see chapter “Mineralisation”).
Take up cinders and 2 ml of concentrated hydrochloric acid (35% minimum) in a 100 ml flask; add 20 ml of lanthanum solution at 25 g/l and complete to volume with demineralised water.
Perform a blank test in the same conditions.
- Procedure
Pass each solution of the set in ascending order of the concentration of calcium.
For each solution, perform 2 absorbance readings when they are perfectly stabilised (integration time of signal: 10 seconds).
Pass each sample twice and calculate the calcium content.
Cinders sulfuric- Total
COEI-2-CENDRE Sulphuric cinders
The sulphuric cinders result from the calcination after being in contact with air after being attacked by sulphuric acid.
Heat a silica or platinum crucible of low form for 30 min until red; allow to cool in a vacuum dessicator and tare the crucible. Place the exactly weighed test sample in the crucible and wet it with a sufficient quantity of concentrated sulphuric acid (R) diluted beforehand by an equal volume of water. Heat until dry evaporation, then in a muffle oven, first carefully until red without exceeding the temperature of 600°C 25°C. Maintain calcination until the black particles disappear, allow to cool, add 5 drops of sulphuric acid diluted to half to the residue, then evaporate and calcinate as previously until constant weight; weigh after cooling in the desiccator.
Calculate the rate of sulphuric cinders referring to 100 g of substance.
Total cinders
The total cinders result from the calcination of the product after contact with air.
Heat a silica or platinum crucible of low form for 30 min until red. Allow to cool in a vacuum dessicator and tare the crucible. Dispose homogenously the exactly weighed test sample in the crucible. Desiccate for an hour in the incubator at 100°C-105°C. Incinerate in the muffle oven, first carefully to avoid that the sample catches fire, then until red at a temperature of 600°C 25°C. Maintain the calcination until the black particles disappear. For 30 min allow to cool in a vacuum desiccator. Weigh. Continue the calcination until constant mass.
If the black particles persist, take up the cinders in hot distilled water. Filter these cinders on an ashless filter paper (porosity 10 µm). Incinerate the filter and residue until constant mass. Group the new cinders with the filtrate. Evaporate the water. Incinerate the residue until constant mass.
Calculate the rate of total cinders by referring to 100 g of substance.
Chlorides- Reasearch
COEI-2-CHLORU Search for chlorides
In a 160 16 mm test tube, place the volume prescribed of the solution obtained by the means indicated in each monography; add 5 ml of diluted nitric acid (R); complete to 20 ml and add 0.5 ml of silver nitrate solution at 5% (R).
Compare the opalescence or any cloudiness to the control sample prepared with 0.5 ml of hydrochloric acid at 0.10 g per litre (0.05 mg of HCl) with 5 ml of diluted nitric acid (R), and adjust to 20 ml with distilled water. Add 0.5 ml of silver nitrate solution at 5% (R). This tube contains 50 µg of HCl.
Chrome- Determination by AAS
COEI-2-CHROME Determination of chrome by atomic absorption spectrometry
- Principle
The chrome is determined by atomic absorption spectrophotometer without flame.
- Apparatus
2.1. Experimental parameters (given as an example)
- Atomic absorption spectrophotometer
- wave length: 357.9 nm
- hollow-cathode lamp (Chrome)
- width of slit: 0.2 nm
- intensity of the lamp: 7 mA
- correction of continuum by the Zeeman effect
- introduction in hot conditions of the samples in the graphite oven
- measurement of the signal: peak height
- time of measurement: 1 second
- number of measurements per sample: 2
- pyrolytic graphite tube:
- pyrolytic graphite oven containing a platform L’Vov tantalised
- tantalisation of platform (see above) inert gas: argon - hydrogen mixture (95%; 5%)
- parameters for oven:
step |
temperature (°C) |
time (s) |
gas rate flow (l / mn) |
type of gas |
reading of signal |
1 |
85 |
5 |
3.0 |
argon + hydrogen |
no |
2 |
95 |
40 |
3.0 |
argon + hydrogen |
no |
3 |
120 |
10 |
3.0 |
argon + hydrogen |
no |
4 |
1000 |
5 |
3.0 |
argon + hydrogen |
no |
5 |
1000 |
1 |
3.0 |
argon + hydrogen |
no |
6 |
1000 |
2 |
0.0 |
argon + hydrogen |
no |
7 |
2600 |
1.2 |
0.0 |
argon + hydrogen |
yes |
8 |
2600 |
2 |
0.0 |
argon + hydrogen |
yes |
9 |
2600 |
2 |
3.0 |
argon + hydrogen |
no |
10 |
75 |
11 |
3.0 |
argon + hydrogen |
no |
2.2. Adjustments of the automatic sampler
(given as an example)
volumes injected in µl |
|||
chrome solution at 50 μg/l |
blank |
matrix modifier |
|
blank |
0 |
17 |
3 |
calibration N° 1 at 50 µg/l |
5 |
12 |
3 |
calibration N° 2 at 100 µg/l |
10 |
7 |
3 |
calibration N° 3 at 150 µg/l |
15 |
2 |
3 |
sample to be measured |
5 |
12 |
3 |
- Reagents
3.1. pure demineralised water for analysis
3.2. pure nitric acid for analysis at 65%
3.3. anhydrous palladous chloride (59% in Pd)
3.4. pure hexahydrated magnesium nitrate for analysis
3.5. ammonium dihydrogenophosphate
3.6. matrix modifier: mixture of palladium chloride and magnesium nitrate (dissolve 0.25 g of PdCl2 and 0.1 g of Mg(NO3)2.6H2O in 50 ml of demineralised water) ammonium dihydrogenophosphate at 6% (dissolve 3 g of NH4H2PO4 in 50 ml of demineralised water).
3.7. Reducing agent: L-ascorbic acid in solution at 1% m/v.
3.8. chrome reference solution at 1 g/l, commercial or prepared as follows: dissolve 7.6952 g of Cr(NO3)3.9H2O in a solution of HNO3 0.5 M, adjust at 1 l with HNO3 0.5 M
3.9. chrome solution at 10 mg/l: place 1 ml of the reference solution in a 100 ml graduated flask, add 5 ml of nitric acid at 65% and complete to volume with demineralised water.
3.10. set of calibration solutions: 0, 50, 100 and 150 µg/l of chrome (see table: adjustments of the automatic sampler).
- Preparation of samples
4.1. Case of liquid or solution oenological products
The preparations are performed manually or automatically by the diluter by following the data from the table “adjustments of the automatic sampler”.
4.2. Case of solid oenological products
Proceed with mineralisation by wet process. Do a blank test.
- Procedure
Pass each solution of the set in ascending order of the concentration of chrome;
Pass each sample twice and calculate the chrome content while taking into account the test sample.
Bacteriological control
COEI-2-CONBAC Methods of microbiological analysis
Bacteriological control
Analysis common to all monographies
- Preliminary rehydration of yeasts (Saccharomyces and non-Saccharomyces): ADY (Active Dry Yeasts), AFY (Active Frozen Yeasts), COY (Compressed Yeasts), CRY (Cream Yeast Preparations), ENY (Encapsulated [beads] or Immobilised Yeasts), “levain de tirage” (yeast starter for tirage)
Weigh approx. 10 g of the preparation under sterile conditions (note the exact weight for final calculation of the concentation).
Adjust to 100 mL with sterile peptone saline water* under sterile conditions at 20-37 °C or according to the manufacturer’s recommendations.
Slowly homogenise using a rod, a stomacher technique or a magnetic stirrer for 5 min.
Stop stirring and allow to stand for 20 min at room temperature of between 20-30 °C.
Homogenise again at room temperature for 5 min.
Under sterile conditions, prepare serial decimal dilutions in water or sterile peptone saline water* and proceed with microbiological controls on the homogenised stock solution.
In the case of “levains de tirage” used for sparkling wines, sample 1 mL under sterile conditions, prepare serial decimal dilutions in water or sterile peptone saline water* and proceed with microbiological controls on the homogenised stock solution
* Peptone salt solution: bacteriological peptone 1 g/L, sodium chloride 8.5 g/L, final pH 7.0
- Preliminary rehydration of preparations of lactic acid bacteria
Weigh approx. 10 g of preparation of lactic acid bacteria under sterile conditions (note the exact weight for final calculation of the concentation).
Adjust to 100 mL with sterile peptone saline water* under sterile conditions (25 °C).
Homogenise using a magnetic stirrer or a stomacher technique for 5 min.
Stop stirring and allow to stand for 20 min at room temperature of between 20-30 °C.
Homogenise again at room temperature for 5 min.
Under sterile conditions, prepare serial decimal dilutions using water or sterile peptone saline water* and proceed with microbiological controls.
* Peptone salt solution: bacteriological peptone 1 g/L, sodium chloride 8.5 g/L, final pH 7.0
- Microbiological control of other products in the International Oenological Codex
(products for which the control of yeasts, bacteria and/or moulds is requested)
Weigh approx. 10 g of the oenological product to control under sterile conditions (note the exact weight for final calculation of the concentration).
Adjust to 100 mL with sterile peptone saline water* under sterile conditions.
Homogenise using a magnetic stirrer or a stomacher technique for 5 min.
Under sterile conditions, prepare serial decimal dilutions in water or sterile peptone saline water* and proceed with microbiological controls.
* Peptone salt solution: bacteriological peptone 1 g/L, sodium chloride 8.5 g/L, final pH 7.0
- Enumeration of total yeasts
YM agar medium (malt wickerham)
Bacteriological agar |
15 g |
Yeast extract |
3 g |
Malt extract |
3 g |
Peptone |
5 g |
Glucose |
10 g |
Water |
q.s. 1000 mL |
YPD
Yeast extract |
10 g |
Peptone |
20 g |
Glucose |
20 g |
Agar |
10 g |
Water |
q.s. 1000 mL |
Just after preparation, autoclave the medium at 120 °C for 20 min.
In case of prolonged incubation time, add chloramphenicol to a 100 mg/L final concentration to prevent bacterial growth.
After inoculation with the appropriate dilutions of the sample in order to reach 30-300 colonies, incubate the dishes at 25-30 °C under aerobic conditions for 48 to 72 hours.
Count the number of CFU in the dishes containing 30-300 colonies and refer to the weight of the dry matter.
In addition to the media proposed, any equivalent medium internationally recognised for growth of these microorganisms may be used.
- Enumeration of non-Saccharomyces yeasts
5.1. Lysine medium
The yeasts are cultivated in the lysine medium whose composition is as follows:
Agar |
20 g |
L-lysine monohydrochloride |
5 g |
Glucose |
1 g |
Bromocresol purple |
0.015 g |
Water |
q.s 1000 mL |
Adjust to |
pH 6.80.2 |
Bring to the boil for 1 min to ensure complete dissolution, then autoclave at 120°C for 20 min.
In case of prolonged incubation time, add chloramphenicol to a 100 mg/L final concentration to prevent bacterial growth.
After inoculation with the dilutions of the sample, the dishes are incubated at 25°C or 30°C for 48 to 96 hours.
Count the number of CFU (dishes of 30-300 colonies) and refer to the weight of the dry matter.
In addition to the media proposed, any equivalent medium internationally recognised for growth of these microorganisms may be used.
5.2. YPD medium with addition of cycloheximide at 10 mg/L, and incubation for 6-7 days under aerobic conditions
In case of prolonged incubation time, add chloramphenicol to a 100 mg/L final concentration to prevent bacterial growth.
- Enumeration of viable lactic acid bacteria
Modified MRS (Man, Rogosa and Sharpe)
The bacteria are cultivated in a MRS medium (Man, Rogosa, Sharpe 1960), with addition of tomato juice, and the composition is as follows:
Agar agar |
15 g |
Bacto-peptone |
10 g |
Meat extract |
8 g |
Yeast extract |
4 g |
Sodium acetate |
5 g |
K2HPO4 |
2 g |
Trisodium citrate |
2 g |
MgSO4 at 100 mg/L |
2.5 mL |
MnSO4 at 20 mg/L |
2 mL |
Tween 80 |
1 mL |
DL malic acid |
5 g |
Tomato juice[1] |
200 mL |
Glucose |
20 g |
or glucose 10 g +fructose |
10 g+10 g |
Adjust (HCl or NaOH) |
q.s. pH 4.8 |
Distilled water |
q.s. 1000 mL |
(q.s. = quantity sufficient)
Autoclave at 110 °C for 20 min.
When pouring the medium into the Petri dish, add pimaricine to a 10 mg/L final concentration to inhibit the growth of yeast and mould.
Incubate at 25°C under anaerobic conditions for 8 to 10 days.
In addition to the media proposed, any equivalent medium internationally recognised for growth of these microorganisms may be used.
- Enumeration of mould
Czapeck-Dox/s agar medium Agar agar |
15 g |
Saccharose |
30 g |
NaNO3 |
3 g |
K2HPO4 |
1 g |
MgSO4 |
0.5 g |
KCl |
0.5 g |
FeSO4 |
0.01 g |
Water |
q.s. 1000 mL |
Adjust to |
pH 7 |
Autoclave at 120°C for 20 min.
Add chloramphenicol directly to the medium in the Petri dish to a 100 mg/L final concentration to inhibit the growth of bacteria.
Incubate at 20°C under aerobic conditions for 10 days.
In addition to the media proposed, any equivalent medium internationally recognised for growth of these microorganisms may be used.
- Enumeration of acetic bacteria
Bacteriological agar |
20 g |
Yeast extract |
5 g |
Casein amino acids |
5 g |
Glucose |
10 g |
Adjust to |
pH 4.5 |
Water |
q.s. 1000 mL |
Autoclave at 120°C for 20 min.
When pouring the medium into the Petri dish, add pimaricine to a 100 mg/L final concentration, to inhibit the growth of yeast and mould, and penicillin to a 12.5 mg/L final concentration to inhibit the growth of lactic acid bacteria.
Incubate at 25 °C under aerobic conditions for 4 days.
In addition to the media proposed, any equivalent medium internationally recognised for growth of these microorganisms may be used.
- Count of Salmonella
9.1. Principle
The sample undergoes a pre-enrichment phase in peptoned buffered water for 16 to 20 hours at 37°C. Then the aliquot part of this mixture is inoculated for culture. This contains a specific medium and 2 special tubes (made up of 2 parts) and is incubated 24 hours at 41°C. Salmonella migrates from the bottom (selective medium) to the top part of the tube (indicator medium). The presence of Salmonella is indicated by a change in colour of this solution.
9.2. Apparatus and analytical conditions
Preparation for culture is carried out in the sterile zone ensured by the Bunsen burner. The soiled material is submitted for destruction by autoclave for 1 hour at 120°C or by total immersion in a bleaching agent for at least 18 hours (See cleaning procedure).
- Sterile glass test tube in 125 ml
- sterile stomacher bag
- Closing barrette
- stomacher
- Sterile glass tubes 16x160 mm.
- Cottoned glass test tubes 20x220
- 2 ml sterile plastic pipettes graduated by 0.1 ml
- 10 ml sterile plastic pipettes graduated by 0.1 ml
- Tube shaker
- Method for culture to be rehydrated.
- 2 ml sterile needle with plastic sterile syringe.
- Tweezer forceps
- Wrench for unscrewing tubes A and B for culture method
- Clean glass slide
- Sterile cottoned Pasteur pipettes
- Monosaccharide
- Oven at 41°C 1°C
- Oven at 37°C 1°C
- Bunsen burner
9.3. Reagents
- Sterile peptoned water (SPW)
- Sterile distilled water (SDW)
- Sterile 500 ml sealed flask filled with 125 ml of SPW
- Sterile 500 ml sealed flask filled with 225 ml of SPW
- Special medium for Salmonella: SRTEM
- Novobiocin disk (1.8 mg of novobiocin)
- Hektoën agar agar (see DOMIC-08)
- API 20E gallery
- Agar agar tubes TSAYE inclined
- Sterile NaCl at 8.5 g/l solution
- Anti-Salmonella serum
9.4. Procedure
9.4.1. Preparation of reference suspension
This differs according to nature of products and dilution rate.
Add a test portion of 25 grams or millilitres of the product in a stomacher bag to a nine fold greater amount of peptoned water.
Close the bag by heat welding or using a barrette.
Grind in a stomacher for 1 minute.
9.4.1.1. Pre-enrichment phase in a non selective liquid medium:
- Incubate the reference suspension for 16 to 20 hours at 37°C ± 1°C.
- Enrichment in selected liquid mediums
Preparation of culture measures
- unscrew the lid of the culture container;
- add SDW up to line 1 as marked on the container.
Note: The base of tubes A and B must be located under water
level.
- adjust the needle to the syringe and check that the syringe plunger is pushed in (absence of air);
- vertically introduce the needle to the syringe in the rubber disc in the centre of the stopper in tube A (blue stopper). Check that the needle is visible under the stopper;
- carefully withdraw the syringe up until the liquid reaches line 3 on the container.
Note: Do not draw up liquid into the syringe.
This operation should take approximately 5 seconds.
- Repeat this operation with tube B (red stopper);
- Close the stopper from the culture container tightly;
- Press the side of the recipient on a tube shaker and maintain at least 5 seconds.
Note: the liquid in tubes A and B must be shaken vigorously.
- Let the culture at least 5 minutes;
- Unscrew the culture container’s stopper and pour in the SRTEM medium until the level reaches line 2 as marked on the container;
- Add a novobiocin disc using a tweezer forceps;
- Remove the stoppers from tubes A (blue) and B (red) using a wrench, then dispose of the stoppers.
Note: avoid touching the tubes and the inside wall of the
container. Inoculation of culture container
- Homogenise the pre-enriched culture;
- Identify the culture container. Write down the analysis number on the lid.
- Unscrew the lid.
- Using a 2 ml pipette introduce 1 ml of pre-enriched culture in the culture container.
- Tighten the lid on the culture container.
- Write down the incubation time and date.
- Incubate 24 hours 30 min at 41°C 1°C in a strictly vertical position.
- Reading and interpretation
This is carried out by observing the top part of tubes A and B through the container walls.
Reaction |
Tube A |
Tube B |
Positive |
All degrees of black colouring |
All degrees of red or black colouring |
Negative |
Absence of black colouring |
Absence of ref or black colouring |
The possible presence of Salmonella is characterised by modifications in indicator medium colour located in one or both of the top parts of the tubes:
Tubes showing a positive reaction are subjected to selective agar isolation.
- Dry boxes of Hektoën agar in an incubator at 46°C 1°C until the drops on the surface of the medium disappear completely (lid removed and agar surface facing down).
- Take a wire hoop from the positive middle indicator and inoculate it into 5 ml of SPW, in a 16x160 mm sterile glass tube in order to dilute the culture.
- proceed as such with each positive tube.
- identify the dish and write down on the lid the number of the analysis and the letter of the tube being confirmed.
- homogenise the culture and take a wire hoop.
- isolate the Hektoën agar on the surface to enable the development of isolated colonies.
- incubate 24 hours at 37°C 1°C.
- Select at least 2 isolated colonies considered to be typical.
- Confirmation
- Biochemical tests
- Confirmation
- identify the different colonies by using specific miniaturised galleries (API 20E gallery) by referring to the recommendations of the manufacturer.
- incubate 24 hours at 37°C 1°C.
- At the same time inoculate: an agar to confirm the purity of the strain.
- 1 agar TSAYE inclined for serological typing.
- incubate 24 hours at 37°C 1°C.
- Read the API20E gallery following the manufacturer’s indications.
- compare the profile obtained to the standard profiles given by the manufacturer.
- Store TSAYE agar in the refrigerator until utilisation.
- Serological tests:
Tests are conducted if the strain profile corresponds to Salmonella following the recommendations defined by the manufacturer from cultures obtained on agar and after eliminating self-agglutinating strains.
Elimination of self-agglutinating strains:
- Place a drop of 8.5 g/l saline solution on a perfectly clean glass slide.
- Disperse a little bit of the culture removed from the nutritive agar to obtain a homogeneous and cloudy solution using a Pasteur pipette.
- Oscillate the slide for 30 to 60 seconds.
- On a black background using a magnifying glass: if any observation reveals more or less distinct clusters, the strain is considered as being self-agglutinating and should not be subjected to serological typing.
9.5. Results
According to the results based on the interpretation of biochemical and serological testing, the results are expressed as follows:
- Presence of Salmonella in m number of grams or ml of product.
- Absence of Salmonella in m number of grams or ml of product.
Diagram of biochemical and serological interpretations |
- Count of Escherichia coli by the counting of colonies obtained at 44°C
10.1. Principle
Inoculating rapid E. coli agar in depth is carried out in a Petri dish for each of the dilutions chosen. Following a 24 hour incubation at 44°C, all characteristic colonies which appear are counted.
10.2. Apparatus and analytical conditions
- Cultures are carried out in a sterility zone ensured by the usage of a Bunsen burner.
- Plastic sterile Petri dishes with a diameter of 90 millimetres
- Sterile 16x60 cottoned glass test tubes
- Tube holder
- 2 ml plastic sterile pipettes with 0.1 ml graduations
- Water bath at 100°C 2°C
- Water bath at 47°C 2°C
- Tube shaker
- Oven at 44°C 1°C
- Bunsen burner
- Colony counter
10.3. Reagents
- Sterile diluent for decimal dilutions: tryptone salt (TS)
- 16x160 pre-filled sterile tubes with 9ml of sterile TS
- Rapid’E.coli cooling agar (R.E.C)
10.4. Procédure
10.4.1. Bacteriological agar medium
- Melt R.EC agar in a boiling water bath. Avoid overheating.
- Never use a culture medium above 50°C.
- For immediate usage, keep agar in the water bath at 47°C 2°C.
- Do not cool over 8 hours.
- For a deferred usage maintain the cooling agar in an oven at 55°C 1°C.
- The melted culture medium not used within 8 hours will not re-solidify for another usage.
- Culture
- Homogenise each dilution before inoculation in Petri dishes and before carrying out decimal dilutions.
- Transfer 1 ml from the reference solution and/or the retained decimal dilutions in the respective Petri dishes. Change the pipette after each dilution.
- Introduce at least 20 minutes after inoculum, 15 to 20 ml of R.EC maintained in the water bath at 47°C 2°C.
- Slowly homogenise by shaking.
- Let solidify on the bench (lid up).
- Pour 4 to 5 ml of R.EC maintained at 47°C 2°C.
- Let solidify on a bench (lid up).
- Return the dishes and incubate in an oven 24 hours ± 2 hours at 44°C 1°C.
- Count
Dishes containing between 15 and 150 characteristic colonies of two successive solutions are retained for counting.
If the dish inoculated with 1 ml of first dilution contains characteristic colonies and fewer than 15, it will be retained for counting.
Characteristic colonies are counted using a counter or are counted manually after 24 hours 2 hours of incubation.
10.5. Results
10.5.1. General case
The dishes contain between 15 and 150 characteristic colonies for two successive dilutions.
10.5.1.1. Method of calculation
The two dishes retained have between 15 and 150 characteristic colonies. The number N of counted micro-organisms at 44.5°C per millilitre (ml) or by gram (g) of product is obtained by calculating the weighted mean on 2 dishes retained.
- c : sum of characteristics counted on 2 dishes retained
- d : rate of dilution corresponding to first dilution
- Expression of results
- Round off the number N to 2 significant digits
- Express to the tenth power
ex.: 1.6 103 / g or ml |
10.5.2. Estimation of small numbers
If the dish inoculated with 1 ml of the 1st retained solution for analysis contains at least 15 characteristic colonies, express the result as follows:
- c : sum of characteristic colonies counted
- d : rate of dilution
If the dish inoculated with 1 ml of the 1st retained solution for analysis does not contain any colonies, express the result as follows:
- d : rate of dilution
- Count of Staphylococci with a positive coagulase by the counting and confirmation of colonies obtained at 37°C
11.1. Principle
Decimal dilutions and inoculation on the surface of 1 Baird Parker agar drawn previously in a Petri dish with each of the dilutions retained, are carried out simultaneously from the sample (liquid product) or from the reference solution (other products).
After an incubation of 48 hours at 37°C the characteristic and/or non characteristic colonies are counted and then confirmed by the coagulase test.
11.2. Apparatus and analytical conditions
Cultures are carried out in a sterility zone ensured by the usage of a Bunsen burner.
- Sterile glass 16x160 cottoned test tubes
- Sterile plastic precipiting tubes with plastic stoppers
- 2 ml plastic sterile pipettes with 0.1 ml graduations
- Sterile plastic spreader
- Sterile Pasteur pipettes
- Tube shaker
- Incubate at 37°C 1°C
- Bunsen burner
- Colony counter
- Reagents
- Sterile diluent for tryptone salt (TS) decimal dilutions.
- 16x160 sterile tubes pre-filled with 9ml of sterile TS.
- Baird Parker agar pre-poured in a Petri dish.
- Tubes pre-filled with 5ml brain heart bouillon (sterile).
- Plasma of lyophilised rabbit rehydrated at the time of use.
- Procedure
- Culture
- Procedure
- Dry the agar plates in an incubator at 46°C 1°C until the droplets on the surface of the environment have completely disappeared (cover is removed and the agar surface is turned downwards).
- homogenise each dilution prior to inoculation of the surface of agar plate surface before carrying out decimal dilutions.
- Place 0.1 ml of reference solution and/or the retained decimal dilutions on the agar surface while changing the pipette after each dilution.
- Carefully spread the inoculum as quickly as possible using a spreader without touching the edges of the plate.
- Leave the plates with the lids closed for 15 minutes at room temperature.
- Incubate 48 hours 2 hours at 37°C ± 1°C
- Counting
Dishes containing less than 150 characteristic and/or non-characteristic colonies on two successive dilutions are retained, but one of them must include at least 15 colonies. The characteristic and/or non-characteristic colonies are counted either manually or by using a counter.
Characteristic colonies
after 48 hours 2 hours of incubation:
- Black or grey, shiny or convex with at least a 1 mm in diameter and a maximum of 2.5 mm in diameter outlined with lightening and precipitation halos.
Non-characteristic colonies
after 48 hours 2 hours of incubation:
- Black and shiny with or without a white edge with lightening or precipitation halos absent or barely visible.
- Grey without light zones.
11.2.2.3. Confirmation
Remove 3 characteristic colonies or 3 colonies of each type (characteristic or non-characteristic) and submit them to the coagulase test.
Coagulase test:
a ) Bouillon culture:
- Take part of the selected colony using a Pasteur pipette sterilised with the Bunsen burner flame and inoculate into a brain heart bouillon.
- Repeat this manipulation for other selected colonies.
- Identify the tubes by sample number and its dilution with a blue marker for characteristic colonies and a green marker for non-characteristic colonies
- Incubate at 37°C 1°C for 20 to 24 hours 2H.
b ) Testing for free coagulase:
- Add 0.5 ml of culture obtained in brain heart bouillon to 0.5 ml of rehydrated rabbit plasma in a sterile precipiting tube and identify as follows.
- Repeat this procedure for each bouillon culture.
- Incubate 4 to 6 hours at 37°C 1°C.
- Check for the presence of coagulum or examine the tube after 24 hours 2 hours of incubation.
11.2.3. Results
Coagulase is considered positive when it occupies ¾ of the initial volume of the liquid.
11.2.3.1. General case
The plates contain a maximum of 150 characteristic and/or non-characteristic colonies.
Calculation procedure:
Number of Staphylococci with positive coagulase for each plate:
- is the number of spotted characteristic colonies
- is the number of spotted non-characteristic colonies
- is the number of characteristic colonies of positive Staphylococci coagulase
- is the total number of non-characteristic colonies of positive coagulase Staphylococci
- is the total number of characteristic colonies of positive coagulase Staphylococci for the plate retained.
- is the total number of non-characteristic colonies of positive coagulase Staphylococci positive for the plate retained
Round off the number to the nearest whole number.
Number of positive coagulase Staphylococci in trials: N
The weighted average, calculated as follows from two successive retained solutions:
- a : sum of positive coagulase Staphylococci colonies identified on 2 retained plates
- F: rate of dilution corresponding to the 1st retained dilution.
expression of results:
- round off the number N to the two largest whole digits
- express to the tenth power
ex.: |
Amount obtained |
Amount rounded off |
Result |
36364 |
36000 |
3.6 104 |
11.2.3.2. Estimation of small numbers:
If the plate inoculated with 0.1 ml of the first dilution retained for analysis contains less than 15 colonies, the result will be expressed as follows:
- a : number of positive coagulase Staphylococci identified.
- d : rate of dilution for the first dilution retained for analyse.
If the dish inoculated with 0.1 ml of the first dilution retained for analysis contains no positive coagulase Staphylococci the result shall be expressed as follows:
- d : Rate of dilution from the first retained dilution for analysis.
- Coliform count by counting colonies obtained at 30°C
- Principle
Inoculation in deeply in crystal violet to neutral red (VRBL) lactose bile agar was carried out in Petri dishes for each of the dilutions retained. After incubation for 24 hours at 30°C, the characteristic colonies were counted.
12.2. Apparatus and analytical conditions
Cultures are carried out in a sterile environment as ensured by a Bunsen burner.
- Plastic sterile Petri dishes with a diameter of 90 millimetres
- Sterile glass 16 x 160 cottoned tubes
- Tube holder
- 2 ml plastic sterile pipettes graduated at 0.1 ml
- Water bath at 47°C 2°C.
- Tube shaker
- Incubate at 30°C 1°C
- Incubate at 55°C 1°C
- Bunsen burner
- Colony counter
12.3. Reagents
- Sterile diluent for decimal dilutions: tryptone salt (TS)
- 16 160 sterile tubes pre filled with 9ml of sterile TS
- Cooled crystal violet and neutral red lactose bile agar (VRBL).
12.4. Procedure
12.4.1. Agar medium
- Once prepared, keep the VRBL agar cooled in the water bath at 47°C 2°C (for immediate usage).
- Never use a culture medium at a temperature higher than 50°C.
- Do not cool over 8 hours.
- For a deferred usage, keep agar cooled in an incubator at 55°C ± 1°C.
- Melted culture mediums unused within 8 hours, shall never re-solidify for later usage.
12.4.2. Culture
Homogenise each dilution before inoculating in Petri dishes prior to carrying out decimal dilutions.
Transfer 1 ml of reference solution and/or decimal dilutions retained in respective Petri dishes with pipettes changed after each dilution
- Introduce up to 20 minutes after the inoculum 15 to 20 ml of VRBL maintained in the water bath at 47°C 2°C.
- Slowly homogenise by shaking.
- Let solidify on laboratory bench (lid upwards).
- Pour approximately 5 ml of VRBL maintained in the water bath at 47 °C 2°C.
- Let solidify on laboratory bench (lid upwards).
- Turn over dishes and incubate immediately 24 hours 2 hours at 30°C 1°C.
-
- Count
Dishes containing less than 150 characteristic or non-characteristic colonies based on two successive dilution are retained, but one of them must contain at least 15 characteristic colonies.
If only the dish inoculated with 1 ml of the 1st dilution contains under 15 characteristic colonies, then the dish will be retained for counting.
Characteristic colonies are counted manually or by using a counter.
Characteristic colonies after 24 hours 2 hours of incubation
- violet colonies surrounded sometimes by a red area (bile precipitation)
- diameter 0.5 mm
12.5. Results
12.5.1. General case
Dishes containing less than 150 characteristic or non-characteristic colonies, based on two successive dilutions with one containing at least 15 characteristic colonies.
Method of calculation:
Number N of micro-organisms counted at 30°C per millilitre (ml) or by gram (g) of product is obtained by calculating the weighted average of 2 retained dishes.
- c : sum of characteristic colonies counted of 2 retained dishes
- D : dilution rate corresponding to the 1st dilution
Expression of results:
- round off the number N to the 2 largest digits
- express to the tenth power
ex: 1.6 103 / g or ml
12.5.2. Estimation of small numbers
If the dish inoculated with 1 ml of the 1st dilution retained for analysis contains less than 15 characteristic colonies, the result will be expressed as follows:
- c : sum of characteristic colonies counted
- d : rate of dilution
If the dish inoculated with 1ml of the 1st dilution retained for analysis contains no colonies then the result will be expressed as follows:
- d : rate of dilution.
Annex 1: Review of methods of coliform research- Escherichia coli and Staphylococcus
- Selective- Differential medium for coliforms. Desoxycolate agar
Ingredients/l |
|
Peptone |
10.0 g |
Lactose |
10.0 g |
Sodium desoxycolate |
1.0 g (Inhibition of the flora accompanying coliforms) |
Sodium chloride |
5.0 g |
Dipotassium phosphate |
2.0 g |
Ferric ammonium citrate |
1.0 g |
Sodium citrate |
1.0 g |
Bacteriological agar |
15.0 g |
Neutral red |
0.03 g |
- Selective- differential medium for Escherichia coli. MET
Sodium laurisulphate and sodium desoxycolate are used as selective factors, in accordance with their properties to inhibit the development of Gram-positive cocci and sporulated bacteria. The differential nature of the method is provided by the chromogen 5-bromo, 6-chloro-indolyl-β-D-glucuronide.
- Selective- Differential medias for Staphylococcus
Giolitti and Cantoni medium |
|
Composition (g) for 1 litre of medium: |
|
Tryptone |
10,0 |
Meat extract |
5,0 |
Autolytic yeast extract |
5,0 |
Glycine |
1,2 |
Mannitol |
20,0 |
Sodium piruvate |
3,0 |
Sodium chloride |
5,0 |
Lithium chloride |
5,0 |
Tween 80 |
1,0 |
pH medium |
6,9 0,2 |
Baird Parker solid medium Composition (g/l) |
|
Tryptone |
10,0 |
Meat extract |
5,0 |
Autolytic yeast extract |
1,0 |
Sodium pyruvate |
10,0 |
Glycine |
12,0 |
Lithium chloride |
5,0 |
Bacteriological agar |
20 |
Egg yolk emulsion |
47 ml |
Potassium tellurite at 3,5 % |
3 ml |
Sulfamehazine |
0,05 g/l (if necessary inhibit Proteus) |
pH medium |
7,2 0,2 |
[1] Tomato juice is used to improve lactic bacterial growth. Preparation: take commercial (without additives) or homemade tomato juice, centrifuge at 4000g for 20 min, filter if necessary and use the clear juice.
Copper- Determination by AAS
COEI-2-CUIVRE Determination of copper by atomic absorption spectrometry
- Principle
The copper is determined by atomic absorption spectrometry by flame by using the method of measured additions.
- Apparatus
Instrumental parameters: (given as an example)
- Atomic absorption spectrophotometer
- flame: oxidant air-acetylene
- wave length: 324.7 nm
- hollow-cathode lamp (copper)
- width of slit: 0.5 nm
- intensity of the lamp: 3.5 mA
- no correction of non specific absorption.
- Reagents
3.1. pure demineralised water for analysis
3.2. pure nitric acid for analysis at 65%
3.3. reference solution copper at 1 g/l, commercial or prepared as follows: dissolve 3.8023 g of Cu(NO3)2.3H2O in a solution of HNO3 0.5M, adjust at 1 l with HNO3 0.5M.
3.4. copper solution at 10 mg/l: place 2 ml of the reference copper solution in a 200 ml graduated flask, add 2 ml of nitric acid at 65% and complete to volume with demineralised water.
Adjust apparatus using a calibration solution at 0.4 mg/l (2 ml of the copper solution at 10 mg/l in a 50 ml graduated flask, complete to volume with pure demineralised water for analysis).
- Preparation of samples (Method of measured additions)
Addition of 02 mg/l of copper:
- place 5 ml of liquid oenological product or mineralisate of oenological product obtained by dry process in a flask and add 100 µl of the copper solution at 10 mg/l
Addition of 0.4 mg/l of copper:
- place 5 ml of liquid oenological product or mineralisate in a flask and add 200 µl of the copper solution at 10 mg/l
Dilution of the sample
Dilution of the sample: the dilution is only necessary if the copper content is more than 0.5 mg/l of copper.
- Procedure
For each sample, pass in order:
- blank solution (demineralised water)
- sample with 0.2 mg/l of copper
- sample with 0.4 mg/l of copper
- sample without addition
- the results are obtained automatically or by manual graph.
Iron- Determination by AAS
COEI-2-FER Determination of iron by atomic absorption spectrometry
- Principle
The iron is determined by atomic absorption spectrophotometry by flame.
- Apparatus
2.1. Instrumental parameters: (given as an example)
- atomic absorption spectrophotometry
- flame: oxidant air-acetylene
- hollow-cathode lamp (iron)
- wave length: 248.3 nm
- width of slit: 0.2 nm
- intensity of the lamp: 5 mA
- no correction of non specific absorption.
- Reagents
3.1. Pure demineralised water for analysis
3.2. iron solution at 1 g/l, commercial or prepared as follows: dissolve 7.2336 g of Fe(NO3)2,9H2O in a solution HNO3 0.5 M adjust at 1 l avec HNO3 0.5 M.
3.3. iron solution at 100 mg/l
Place 10 ml of the reference iron solution in a 100 ml graduated flask, complete with demineralised water pure for analysis
3.4. set of calibration solution: 2, 4, 6, 8 mg/l of iron
place successively 1.0, 2.0, 3.0 and 4.0 ml of the solution at 100 mg/l of iron in 4, 50 ml graduated flasks; complete to volume with pure demineralised water for analysis
Perform a blank without iron in the same conditions.
- Preparation of samples
4.1. Case of liquid or solution oenological products
Each sample is diluted with demineralised water in order to have a concentration of iron between 0 and 8 mg/l.
4.2. Case of solid oenological products
Proceed with mineralisation by dry process.
Put in each solution of the set of calibration the same quantity of acid used for putting of cinders in solution; each sample is diluted with demineralised water in order to have a concentration of iron between 0 and 8 mg/l.
- Procedure
Pass successively the calibration solutions and the blank which will be demineralised water or a water-acid solution with concentrations used for samples of solid oenological products mineralised by dry process and perhaps diluted.
Mercury- Determination
COEI-2-MERCUR Determination of mercury by the generation of vapour and atomic fluorescence spectrometry
- Field of application
This method is applied to the analysis of mercury in oenological products in the concentration range of 0 to 10 μg/l.
- Description of the technique
2.1. Principle of the method
2.1.1. Mineralisation by the wet process of the oenological product to be analysed.
2.1.2. Reduction of the permanganate not consumed by hydroxylamine hydrochloride.
2.1.3. Reduction of mercury(II) into metal mercury by tin chloride (II).
2.1.4. Entrainment of mercury by a current of argon at room temperature.
Detremining mercury in the state of monoatomic vapour by atomic fluorescence spectrometry, with the wave length at 254 nm: the mercury atoms are excited by a mercury vapour lamp; the atoms thus excited reemit fluorescent radiation that enables to quantify the mercury present using a photonic detector placed at 90° in relation to excitation beam; detection by atomic fluorescence enables to obtain good linearity and eliminates memory effects.
2.2. Principle of the analysis (figure n°1)
The peristaltic pump draws up the tin chloride (II) solution, the blank (demineralised water containing 1% nitric acid) and the mineralised sample or calibration.
The metal mercury is entrained in the gas-liquid separator by a current of argon.
After going through the membrane of a dessicator, the mercury is detected by fluorescence.
Then the gaseous current goes through a potassium permanganate solution in order to trap the mercury.
- Reagents and preparation of reagent solutions
3.1. Ultra-pure demineralised water
3.2. Ultra-pure nitric acid at 65%
3.3. Blank: demineralised water (3.1.) containing 1% nitric acid (3.2.)
3.4. Nitric acid solution 5.6 M: introduce 400 ml of nitric acid (3.2.) into a 1000 ml flask; complete to volume with demineralised water (3.1.).
3.5. Sulphuric acid (d = 1.84)
3.6. Sulphuric acid solution 9 M: introduce 200 ml of demineralised water (3.1.) in a 1000 ml flask, then 500 ml of sulphuric acid (3.5.); after cooling, complete to volume with demineralised water (3.1.).
3.7. Potassium permanganate KMnO4
3.8. Potassium permanganate solution at 5%: dissolve with demineralised water (3.1.), 50 g of potassium permanganate (3.7.) in a 1000 ml flask; complete to volume with demineralised water (3.1.).
3.9. Hydroxylamine hydrochloride NH2OH,HCl
3.10. Reducing solution: weigh 12 g of hydroxylamine hydrochloride (3.9.) and dissolve in 100 ml of demineralised water (3.1.).
3.11. Tin chloride II (SnCl2,2 H2O)
3.12. Concentrated hydrochloric acid
3.13. Tin (II) chloride solution: weigh 40 g of tin chloride (3.11.) and dissolve in 50 ml of hydrochloric acid (3.12.); complete to 200 ml with demineralised water (3.1.).
3.14. Mercury reference solution at 1 g/l prepared by dissolution of 1.708 g of Hg(NO3)2.H2O, in 1 l of HNO3 solution at 12% (m/n).
3.15. Mercury calibration solution at 10 mg/l, containing 5 % of nitric acid and prepared from the reference solution at 1 g/l (3.14).
3.16. Mercury solution at 50 µg/l: place 1 ml of the solution at 10 mg/l (3.14.) in a 200 ml flask; add 2 ml of nitric acid (3.2.); complete to volume with demineralised water (3.1.).
- Apparatus
4.1. Glassware:
4.1.1. graduated flasks 100, 200 and 1000 ml (class A)
4.1.2. graduated pipettes 0.5; 1.0; 2.0; 5; 10 and 20 ml (class A)
4.1.3. precautions: before use, the glassware must be washed with nitric acid at 10%, left in contact for 24 hours, then rinsed with demineralised water.
4.2. Mineralisation apparatus (see Compendium of international methods of analysis of wines and musts)
4.3. Thermostatic heating mantle
4.4. Peristaltic pump
4.5. Cold vapour generator
4.5.1. gas-liquid separator
4.6. Dessicator (hygroscopic membrane) covered by an air current (supplied by a compressor) and placed before the detector
4.7. Spectrofluorimeter:
4.7.1. mercury vapour lamp, adjusted to the wave length of 254 nm
4.7.2. specific atomic fluorescence detector
4.8. PC:
4.8.1. software that adjusts the parameters of the vapour generator and atomic fluorescence detector and allows calibration and the analysis of results.
4.8.2. printer that archives results
4.9. Bottle of neutral gas (argon)
- Preparation of the set of calibration solutions and samples
5.1. Set of calibration solutions: 0; 0.25; 0.5 and 1.0 μg/l
Introduce 0; 0.5; 1.0; 2.0 ml of the mercury solution at 50 μg/l (3.15.) in 4 100 ml flasks; add 1% nitric acid (3.2.); complete to volume with demineralised water (3.1.).
5.2. Samples
Mineralise the samples by wet process The test sample is introduced into the round-bottomed flask in borosilicate glass placed on a disc with a hole. The neck is inclined.
Add 5 ml of concentrated sulphuric acid (R) and 10 ml of concentrated nitric acid (R) and gently heat. When the mixture starts to turn brown, add a small quantity of nitric acid while continuing to heat and so forth until the liquid remains colourless and that the atmosphere of the flask fills with white smoke of SO3. Allow to cool, take 10 ml of distilled water and heat again to allow the nitrous fumes to escape until the release of the white smoke. This operation is repeated; after a third time, boil an instant, cool, stabilise with several drops (about 10) of potassium permanganate (aqueous sol.) at 5% (m/m) and add water to the liquid to reach 40 ml.
Filter on filters without cinders. Introduce 10 ml of filtrate into a 50 ml flask. Add potassium permanganate (3.8.) until persistence of coloration. Solubilise the precipitate (MnO2) with the reducing solution (3.10.). Complete to volume with demineralised water (3.1.).
Do a blank test with demineralised water.
- Procedure
6.1. Analytical determination
Turn on the fluorimeter; the apparatus is stabilised after 15 minutes.
The peristaltic pump draws up the blank solution (3.3.), the tin chloride (II) solution (3.13.) and the calibrations or samples (5.1.) or (5.2.).
Check if there is a bubbling in the gas-liquid separator.
Present successively the calibration solutions (5.1.); start the programming of the vapour generator. The computer software sets up the calibration curve (percentage of fluorescence depending on the concentration of mercury in µg/l).
Then present the samples (5.2.).
6.2. Self-check
Every five determinations, an analytical blank solution and a calibration are analysed in order to correct a possible drift of the spectrofluorimeter.
- Expression of results
The results are given by the computer software and are expressed in p.p.b. (or μg/l).
The concentration of mercury in oenological products is calculated according to the test sample and the dilution of the mineralisate. It is expressed in μg/kg.
- Control of results
The quality control is performed by placing, after the set of calibration solutions and all five samples, a reference material whose mercury content is known with certainty.
A control card is set up for each reference material used. The control limits are set at: +/- 2SR intra (SR intra: standard deviation for reproducibility).
- Bibliography
- CAYROL M., BRUN S., 1975. Dosage du mercure dans les vins. Feuillet Vert de l’O.I.V. n°371.
- REVUELTA D., GOMEZ R., BARDON A., 1976. Dosage du mercure dans le vin par la méthode des vapeurs froides et spectrométrie d’absorption atomic. Feuillet Vert de l’O.I.V. n°494.
- CACHO J., CASTELLS J.E., 1989. Determination of mercury in wine by flameless atomic absorption spectrophotometry. Atomic Spectroscopy, vol. 10, n°3.
- STOCKWELL P.B., CORNS W.T., 1993. The role of atomic fluorescence spectrometry in the automatic environmental monitoring of trace element analysis. Journal of Automatic Chemistry, vol. 15, n°3, p 79-84.
- SANJUAN J., COSSA D., 1993. Dosage automatique du mercure total dans les organismes marins par fluorescence atomique. IFREMER, Rapport d’activité.
- AFNOR, 1997. Dosage du mercure total dans les eaux par spectrométrie de fluorescence atomique. XPT 90-113-2.
- GAYE J., MEDINA B., 1998. Dosage du mercure dans le vin par analyse en flux continu et spectrofluorimétrie. Feuillet Vert de l’O.I.V. n°1070.
Heavy metals- Research
COEI-2-METAUX Search for heavy metals
- Principle of the method
Heavy metals react with the thiol function to form sulphurs. The coloration that results is compared to a standard.
- Reagents
2.1. Ammonium acetate,
2.2. Lead nitrate (II),
2.3. Glycerol,
2.4. Methanol,
2.5. Sodium hydroxide, solution at 1 mole NaOH /l,
2.6. Hydrochloric acid at 37%,
2.7. Thioacetamide reagent (R):
2.8. Standard lead solution:
2.8.1. Lead solution at 1000 μg/ml: dissolve 1.598 g of lead nitrate(II) in water and complete to 1000 ml.
2.8.2. Lead solution at 10 μg/ml. Add 10 ml of the solution 2.8.1 and complete to 1000 ml. To be prepared just before use.
2.9. Buffer solution, pH = 3.5: dissolve 6.25 g of ammonium acetate in 6 ml of water, add 6.4 ml of hydrochloric acid (2.6) and dilute with water until 25 ml.
- Procedure
3.1. Test solution: pour 5 ml of buffer solution (2.9), 25.0 g of sample and about 15 ml of water into a 50 ml graduated flask. Complete with water up to the reference mark.
3.2. Coloured solutions:
3.2.1. Sample solution: mix 12.0 ml of test solution (3.1) and 2.0 ml of buffer solution (2.9) in a test tube.
3.2.2. Comparative solution: mix 2.0 ml of test solution (3.1), 2.0 ml of buffer solution (2.9), 0.5 ml of standard lead solution (2.8.2), 4.5 ml of water and 5.0 ml of methanol in a test tube.
3.2.3. Control solution: mix 12.0 ml of test solution (3.1), 2.0 ml of buffer solution (2.9) and 0.5 ml of standard lead solution (2.8.2) in a test tube.
3.2.4. Comparison of colorations:
- add 1.2 ml of thioacetamide reagent (2.7) in the 3 test tubes (3.2.1 to 3), mix and wait 2 minutes. Compare the coloration vertically in the light of day.
- the sample solution must not be darker than the comparative solution.
- the control solution must not be lighter than the comparative solution.
- Results:
The conditions described in 3.2.4 are obtained if the heavy metal content is less than 10 mg/l expressed in lead and with a precision of 1 mg/l.
Mineralisation methods before determination by AAS
COEI-2-MINERA Mineralisation methods of samples before determination by atomic absorption spectrometry
- Mineralisation by dry process
Method applicable for determining the following elements: calcium, magnesium, sodium, iron, copper, zinc.
1.1. Obtaining cinders
- Weigh with precision 5 g of oenological product (or 1 g in the case of products rich in mineral matters), in a platinum or silice capsule cleaned and tared beforehand.
- Gently burn the sample with the flame of a Bunsen burner under a hood.
- Put the capsule in a muffle oven at 525°C 25°C for 12 hours.
- Take up the residue with a few ml of demineralised water.
- Evaporate water over a water bath at 100°C.
- Replace the capsule containing the sample in the oven.
- The mineralisation is over when the cinders are white.
- Putting the cinders in a solution
- The cinders are solubilised with 2 ml of concentrated hydrochloric acid (R), bring to volume at 100 ml with demineralised water
- Complementary dilutions:
- Re-dilute the cinders solution in hydrochloric acid in order to be compatible with the sensitivity of the apparatus; see separately the method of each cation.
- For the determination of calcium and magnesium, add lanthanum chloride during this dilution.
- Do a blank test.
- Mineralisation by wet process
Method applicable for determining the following elements: arsenic, cadmium, lead in oenological products containing water.
2.1. Case of aqueous products
- Weigh with precision in a 50 ml polypropylene tube 3 grammes of pulverised oenological product, add 5 ml of nitric acid at 65%; close with a screw cap; leave 12 hours at room temperature then after unscrewing the cap place the tube in a water bath at 90°C for 3 hours under a hood; allow to cool; adjust the volume to 20 ml with demineralised water; shake; filter on an ashless filter paper (if necessary).
- Do a blank test in the same conditions.
- Case of dry products
The mineralisation is similar as for aqueous products but by using a test sample of 0.5 gramme of oenological product.
Nickel- Determination by AAS
COEI-2-NICKEL Determination of nickel by atomic absorption spectrometry
- Principle
The nickel is directly determined by atomic absorption spectrometry without flame (electro-thermal atomisation).
- Apparatus
2.1. Instrumental parameters: (given as an example)
Atomic absorption spectrophotometer equipped with an atomiser with a graphite tube.
- wave length: 232.0 nm
- hollow-cathode lamp (nickel)
- width of the slit: 0.2 nm
- intensity of the lamp: 4 mA
- correction of continuum by the Zeeman effect
- Introduction in hot conditions of the samples in the graphite oven with an automatic distributor
- rinsing water contains 2 drops of Triton per litre.
- measurement of signal: peak height.
- Time of measurement: 1 second.
- pyrolytic graphite tube:
- pyrolytic graphite oven containing a platform of L’Vov tantalised.
- tantalisation of a platform: see above.
- inert gases: argon and argon + hydrogen mixture (95%: 5%).
Parameters for oven:
Parameters for oven for determining nickel |
|||||
step |
temperature |
time |
gas flow rate |
type of gas |
reading of signal |
n° |
(°C) |
(s) |
(l/min) |
||
1 |
85 |
5.0 |
3.0 |
argon |
no |
2 |
95 |
40.0 |
3.0 |
argon |
no |
3 |
120 |
10.0 |
3.0 |
argon |
no |
4 |
800 |
5.0 |
3.0 |
argon |
no |
5 |
800 |
1.0 |
3.0 |
argon |
no |
6 |
800 |
2.0 |
0 |
argon |
no |
7 |
2 400 |
1.1 |
0 |
argon + hydrogen |
yes |
8 |
2 400 |
2.0 |
0 |
argon + hydrogen |
yes |
9 |
2 400 |
2.0 |
3.0 |
argon |
no |
10 |
75 |
11.0 |
3.0 |
argon |
no |
2.2. Adjustment of automatic sampler (given as an example)
- Parameters of automatic sampler |
|||
volume injected in µl |
|||
solution of Ni |
blank |
matrix modifier |
|
at 50 μg/l |
|||
blank |
17 |
3 |
|
calibration 1 |
5 |
12 |
3 |
calibration 2 |
10 |
7 |
3 |
calibration 3 |
15 |
2 |
3 |
sample |
5 |
12 |
3 |
- Reagents
3.1. Pure demineralised water for analysis
3.2. Pure nitric acid for analysis at 65%
3.3. Anhydrous palladium chloride (59% in Pd)
3.4. Pure hexahydrated magnesium nitrate for analysis
3.5. Ammonium dihydrogenophosphate
3.6. Matrix modifier: mixture of palladium chloride and magnesium nitrate (dissolve 0.25 g of PdCl2 and 0.1 g of Mg(NO3)2.6H2O (3.4) in 50 ml of demineralised water) ammonium dihydrogenophosphate at 6% (dissolve 3 g de NH4H2PO4 in 50 ml of demineralised water), (3.1).
3.7. L-ascorbic acid
3.8. Analytical blank solution: L-ascorbic acid solution at 1% (m/v).
3.9. Nickel reference solution at 1 g/l (1000 µg/ml) off the shelf or prepared as follows: dissolve 4.9533 of Ni(NO3)2.6H2O in a solution of HNO3 0.5 M, adjust at 1 l with HNO3 0.5 M.
- Procedure
Nickel solution at 10 mg/l: place 1 ml of the reference solution (3.8) in a 100 ml graduated flask, add 5 ml of nitric acid (3.2); complete to volume with demineralised water.
Nickel solution at 50 μg/l: place 1 ml of the nickel solution at 10 mg/l in a 200 ml graduated flask, 10 ml of nitric acid (3.2) and complete with demineralised water.
Set of calibration solution: 0, 50, 100 and 150 μg/l of nickel.
The automatic distributor cycle enables to perform this calibration on the platform from a nickel solution at 50 μg/l.
- Preparation of samples
5.1. Case of liquid or solution samples
No preparation or sample dilution is necessary; the samples are placed directly in the cups of the automatic injector.
5.2. Case of solid samples
The solid samples are mineralised by dry process.
- Determinations
The calibration graph (absorbance depending on the concentration of nickel) gives the concentration of nickel in the samples.
Lead- Determination by AAS
COEI-2-PLOMB Determination of lead by atomic absorption spectrometry
- Principle
After mineralisation of the sample in an acid medium, the lead is determined by spectrometry without flame (electro-thermal atomisation).
- Apparatus
2.1. Instrumental parameters: (given as an example)
Atomic absorption spectrophotometer equipped with an atomiser with a graphite tube
- wave length: 283.3 nm
- hollow-cathode lamp (lead)
- width of slit: 0.5 nm
- intensity of the lamp: 5 mA
- correction of continuum: by Zeeman effect
- introduction in hot conditions of the samples in the graphite oven by an automatic distributor (rinsing water contains 2 drops of Triton per litre)
- measurement of signal: peak height
- time of measurement: 1 second
- number of measurements per sample: 2
- pyrolytic graphite tube
- pyrolytic graphite oven containing a platform of L’Vov
- tantalised (tantalisation of a platform: see above).
Parameters for oven
temperature (°C) |
time (s) |
gas flow rate (l / min) |
type of gas |
Reading of signal |
150 |
20.0 |
3.0 |
argon |
no |
150 |
35.0 |
3.0 |
argon |
no |
800 |
15.0 |
3.0 |
argon |
no |
800 |
30.0 |
3.0 |
argon |
no |
800 |
2.0 |
0.0 |
argon |
no |
2250 |
0.8 |
0.0 |
argon |
yes |
2250 |
1.0 |
0.0 |
argon |
yes |
2500 |
1.0 |
1.5 |
argon |
no |
1200 |
9.0 |
3.0 |
argon |
no |
75 |
10.0 |
3.0 |
argon |
no |
2.2. Adjustments of the automatic sampler
(given as an example)
volumes injected in μl |
|||
lead solution at 50 μg/l |
blank |
matrix modifier |
|
blank |
0 |
10 |
2 |
calibration N° 1 |
1 |
9 |
2 |
calibration N° 2 |
2 |
8 |
2 |
calibration N° 3 |
3 |
7 |
2 |
calibration N° 4 |
4 |
6 |
2 |
calibration N° 5 |
6 |
4 |
2 |
Sample to be measured |
10 |
0 |
2 |
- Reagents
3.1. Pure demineralised water for analysis
3.2. Pure nitric acid for analysis at 65%
3.3. Ammonium dihydrogenophosphate
3.4. Matrix modify: ammonium dihydrogenophosphate at 6%.
Introduce 3 g of ammonium dihydrogenophosphate in a 50 ml graduated flask, dissolve and complete to volume with demineralised water.
Lead reference solution at 1 g/l commercial or prepared as follows: dissolve 1.5985 g of pure Pb(NO3)2 for analysis in a solution of HNO3 0.5 M, adjust at 1 l avec HNO3 0.5 M.
Lead solution at 10 mg / l: place 1 ml of the reference lead solution at 1 g/l in a 100 ml graduated flask; add 1 ml of nitric acid at 65% complete to volume with pure demineralised water for analysis.
Lead solution at 0.1 mg/l: place 1 ml of the lead solution at 10 mg/l in a 100 ml graduated flask, add 1 ml of nitric acid at 65%; complete to volume with pure demineralised water for analysis.
Set of calibration solutions: 0, 50, 100, 150, 200, 300 µg/l of lead.
The automatic distributor cycle allows to directly inject these quantities of lead on the platform from the lead solution at 0.050 mg/l.
- Preparation of samples
- The liquid or solution samples must have concentrations between 0 and 300 μg/l of lead.
- The solid samples will be mineralised by wet process (attack by nitric acid).
- The blank is made up of pure water for analysis containing 1% of nitric acid at 65%.
- Procedure
The calibration curve represents the variations of absorbencies depending on the concentrations enabling to calculate the lead content of the samples.
Potassium- Determination by AAS
COEI-2-POTASS Determination of potassium by atomic absorption spectrometry
- Principle
The potassium is determined by mineralisation by dry process by atomic absorption spectrometry.
The addition of a spectral buffer (cesium chloride) to avoid the ionisation of the potassium is necessary.
- Apparatus
2.1. Glassware
- 100 and 200 ml graduated flasks (class A)
- 1, 2, 4 and 10 ml graduated pipettes (class A)
- 100 ml cylindrical vase
- Instrumental parameters (given as an example)
- atomic absorption spectrophotometer
- oxidant air-acetylene flame (flow rate-air: 3 l/min, flow rate-acetylene: 1.8 l/min.)
- Hollow-cathode lamp (potassium)
- wave length: 769.9 nm
- width of the slit: 0.5 nm
- intensity of the lamp: 7 mA
- no correction of non specific absorption.
- Reagents
3.1. Pure demineralised water for analysis
3.2. Cesium chloride (CsCl)
3.3. Cesium chloride solution at 5% in cesium: Dissolve 6.330 g of cesium chloride in 100 ml of demineralised water.
3.4. Potassium reference solution at 1 g/l commercial or prepared as follows: dissolve 2.5856 g KNO3 in water, adjust to 1 l.
3.5. Diluted potassium solution at 100 mg/l: Place 10 ml of the potassium reference solution at 1 g/l in a 100 ml graduated flask and 1 ml of pure nitric acid; complete to volume with pure demineralised water for analysis.
3.6. Set of calibration solution at 0, 2, 4, 6 and 8 mg of potassium per litre:
In a series of 100 ml graduated flasks, introduce 0; 2.0; 4.0; 6.0; 8.0 ml of the potassium solution at 100 mg/l ; add 2 ml of the cesium chloride solution to all the graduated flasks; adjust the volume to 100 ml with pure demineralised water for analysis.
The calibration solutions prepared contain 1 g of cesium per litre.
- Preparation of samples
4.1. Liquid or solution oenological products
In a 50 ml graduated flask, place 1 ml of the cesium chloride solution at 5% and a volume of a sample as is after having completed to volume with demineralised water; the concentration of potassium to be measured is below 8 mg/l.
4.2. Solid oenological products
Proceed with mineralisation by dry process (take cinders in 2 ml of hydrochloric acid in a 100 ml flask, add 2 ml of cesium chloride at 5% and complete to volume with demineralised water).
Perform a blank test with demineralised water.
- Determinations
Present successively the calibration solutions.
Perform an absorbance reading for 10 seconds; perform two measurements.
Set up the calibration curve (absorbance depending on the concentration in mg/l of potassium).
Then present the samples, perform an absorbance reading for 10 seconds; perform two measurements.
Calculate the concentration of potassium in the oenological products in mg/kg.
Saccharoce- Grape sugar- Determination
COEI-2-SUCSAC Grape sugar: Determination of saccharose by HPLC
- Principle
The samples diluted or put in solution are analysed by high performance liquid chromatography: Separation on column of grafted silica NH2 and detection using a differential refractometer.
- Apparatus and analytical conditions (for example)
2.1. Chromatograph
- Grafted silica column NH2 (length 20 cm, internal diameter 4 mm granulometry 5 μm)
- A pumping system
- An auto-sampler (maybe)
- Microfiltres with porosity 0.45 µm
- Differential refractometry detector
- Chromatographic conditions (given as an example)
The water used is deionised and microfiltered.
The acetonitrile is of HPLC quality
The composition of the mobile phase is the following:
- If the column is new: acetonitrile/water (75/25)
- When the fructose - glucose resolution starts to deteriorate, the mobile phase is then a acetonitrile/water 80/20 mixture.
The flow is 1 ml/min.
- Reagents and calibration solutions
3.1. Preparation of the reference solution
The chemicals used for the reference solution preparation are of "pure for analysis" quality.
The composition of this solution is about 10 g/l for each sugar (fructose, glucose and saccharose).
The reference solution is prepared every two weeks (maximum) and stored in the refrigerator in the 100 ml graduated flask used for the preparation.
Selenium- Determination by AAS
COEI-2-SELENI Determination of selenium by atomic absorption spectrometry
- Principle
After mineralisation of the sample by wet process, the selenium is determined by atomic absorption spectrometry without flame (electro-thermal atomisation in the graphite oven).
- Apparatus
2.1. Glassware
- Graduated flasks 50, 100 ml (class A)
- Graduated pipettes 1, 5 and 10 ml (class A)
- Polypropylene tubes 50 ml with screw top.
- Instrumental parameters: (given as an example)
- Atomic absorption spectrophotometer equipped with an atomiser
- with a graphite tube.
- wave length: 196.0 nm
- hollow-cathode lamp (selenium)
- width of slit: 1.0 nm.
- intensity of the lamp: 10 mA
- correction of continuum by the Zeeman effect
- introduction in hot conditions of the samples in the graphite oven with anautomatic distributor (rinsing water contains 2 drops of Tritonper litre).
- measurement of signal: peak height
- time of measurement: 1 second
- number of measurements per sample: 2
Pyrolytic graphite tube:
Pyrolytic graphite oven containing a platform of L’Vov tantalised.
tantalisation of a platform: see given procedure beforehand.
inert gas: argon.
parameters for oven: table I
Table I - Parameters for oven for determining selenium |
|||||
step |
temperature |
time |
gas flow rate |
type of gas |
reading of signal |
(°C) |
(s) |
(l/min) |
|||
1 |
85 |
5 |
3.0 |
argon |
no |
2 |
95 |
40 |
3.0 |
argon |
no |
3 |
120 |
10 |
3.0 |
argon |
no |
4 |
1 000 |
5 |
3.0 |
argon |
no |
5 |
1 000 |
1 |
3.0 |
argon |
no |
6 |
1 000 |
2 |
0 |
argon |
no |
7 |
2 600 |
0.8 |
0 |
argon |
yes |
8 |
2 600 |
2 |
0 |
argon |
yes |
9 |
2 600 |
2 |
3.0 |
argon |
no |
2.3. Automatic sampler parameters (table II)
(given as an example)
Table II - Parameters de automatic sampler. |
|||
volumes injected in µl |
|||
solution |
blank |
matrix modifier |
|
blank |
17 |
3 |
|
calibration n°1 50 μg/l |
5 |
12 |
3 |
calibration n°2 100 μg/l |
10 |
7 |
3 |
calibration n°3 150 μg/l |
15 |
2 |
3 |
sample |
15 |
2 |
3 |
- Reagents
3.1. Pure demineralised water for analysis
3.2. Pure nitric acid for analysis at 65%
3.3. Anhydrous palladium chloride (59% in Pd)
3.4. Pure hexahydrated magnesium nitrate for analysis
3.5. Ammonium dihydrogenophosphate
3.6. Matrix modifier: mixture of palladium chloride and magnesium nitrate (dissolve 0.25 g of PdCl2 and 0.1 g of Mg(NO3)2.6H2O in 50 ml of demineralised water) ammonium dihydrogenophosphate at 6% (dissolve 3 g de NH4H2PO4 in 50 ml of demineralised water).
3.7. Selenium reference solution at 1 g/l, off the shelf or prepared as follows: dissolve 1.4052 g SeO2 in a solution of HNO3 0.5 M, adjust at 1 l avec HNO3 0.5 M.
3.8. Selenium solution at 10 mg/l: place 1 ml of the reference solution at 1 g/l in a 100 ml graduated flask; add 5 ml of nitric acid at 65%; complete to volume with pure demineralised water for analysis
3.9. Selenium solution at 50 µg/l: place 0.5 ml of the selenium solution at 10 mg/l, 5 ml of nitric acid at 65% in a 100 ml graduated flask; complete to volume with pure demineralised water for analysis.
3.10. Set of calibration solutions: 0, 50, 100 and 150 μg/l of selenium.
The automatic distributor cycle enables to perform this calibration on the platform from the selenium solution at 50 μg/l.
- Preparation of samples
Weigh with precision a test sample of 1 to 3 g in the graduated tube; add 5 ml of nitric acid at 65%; close with the screw cap; leave 12 hours at room temperature;
place the tube in a water bath at 90°C for 3 hours (the caps are unscrewed during the heating); allow to cool; adjust the volume to 20 ml with pure demineralised water for analysis.
- Determinations
Set up the calibration graph (absorbance depending on the concentration in µg/l of selenium); determine the concentration of selenium in the samples.
Calculate the concentration of selenium in the mineralisate, then in the samplein μg/kg.
Sodium- Determination by AAS
COEI-2-SODIUM Determination of sodium by absorption atomic spectrometry
- Principle
The sodium is determined after mineralisation by dry process by atomic absorption spectrometry.
The addition of a spectral buffer (cesium chloride) to avoid ionisation of sodium is necessary.
- Apparatus
2.1. Glassware
- Graduated flasks 50 and 100 ml (class A)
- Graduated pipettes 2.0; 5.0; 10.0 ml (class A)
- Automatic pipette 1000 μl
- Cylindrical vase 100 ml.
- Instrumental parameters: (given as an example)
- Atomic absorption spectrophotometer
- oxidant air-acetylene flame (rate-air: 3.1 l/mn; rate-acetylene: 1.8 l/mn)
- wave length: 589.0 nm
- hollow-cathode lamp (sodium)
- width of slit: 0.2 nm
- intensity of the lamp: 5 mA
- no correction of non specific absorption
- Reagents
3.1. Pure demineralised water for analysis
3.2. Pure nitric acid for analysis at 65%
3.3. Cesium chloride solution at 5% in cesium: Dissolve 6.330 g of cesium chloride in 100 ml of pure demineralised water for analysis.
3.4. Sodium reference solution at 1 g/l commercial or prepared as follows: dissolve 3.6968 g NaNO3 in water, adjust at 1 l.
3.5. Diluted sodium solution at 10 mg/l:
Place 1 ml of the reference solution at 1 g/l in a 100 ml graduated flask, 1 ml of nitric acid at 65%, complete to volume with pure demineralised water for analysis.
3.6 Set of calibration solutions 0; 0.25; 0.50; 0.75; 1.00 mg of sodium per litre:
In a series of 100 ml graduated flasks, place 0; 2.5; 5.0; 7.5; 10 ml of the diluted sodium solution; in all the graduated flasks add 2 ml of the cesium chloride solution and adjust the volume at 100 ml with pure demineralised water for analysis.
The calibration solutions prepared contain 1 g of cesium per litre; they are stored in polyethylene flasks.
- Preparation of samples
4.1. Liquid or solution oenological products
In a 50 ml graduated flask, place 1 ml of the cesium chloride solution at 5% and a volume of sample after having been completed to volume with demineralised water, the concentration of sodium to be measured is below at 1 mg/l.
4.2. Solid oenological products
Proceed with a mineralisation by dry process (take up the cinders in 2 ml of hydrochloric acid in a 100 ml flask, add 2 ml of cesium chloride at 5% and complete to volume with demineralised water).
Perform a blank test with demineralised water.
- Determinations
Present successively calibration solutions.
Perform an absorbance reading for 10 seconds; perform two measurements.
Set up the calibration curve (absorbance depending on the concentration in mg/l of sodium).
Then present the samples; determine the concentration of sodium of the diluted samples in mg/l.
Calculate the concentration of sodium in the oenological products in mg/kg.
The dosages of air-acetylene flame are performed manually.
Sulphates- Research
COEI-2-SULFAT Search for sulphates
In a 160 16 mm test tube, place the volume prescribed of the solution obtained by the means indicated in each monography; add 1 ml of diluted hydrochloric acid (R); adjust to 20 ml with water and add 2 ml of barium chloride solution at 10% (R).
Compare the opalescence or any cloudiness to the control sample prepared with 1 ml of solution at 0.100 g of sulphuric acid per litre (i.e. 0.10 mg of H2SO4,) with 1 ml of diluted hydrochloric acid (R) and water until volume of 20 ml and 2 ml of barium chloride solution (R). This tube contains 100 μg of H2SO4.
Tantalisation of platforms
COEI-2-TANTAL Tantalisation of platforms of l’Vov in graphite
- Preparation of tantalum solution at 6% (m/v) according to the zatka process
Three grammes of tantalum powder are put in a 100 ml Teflon cylindrical vase.
Add 10 ml of hydrofluoric acid diluted to a half, 3 g of dehydrated oxalic acid and 0.5 ml of hydrogen peroxide at 30 vol.
Heat carefully to dissolve the metal.
Add a few drops of hydrogen peroxide as soon as the reaction slows down; when the dissolution is complete, add 4 g of oxalic acid and 30 ml of water.
The acid is dissolved and the solution is brought to 50 ml with ultra pure demineralised water.
Store this solution in a plastic flask.
- Treatment of graphite platforms
The platform is placed inside the graphite tube or used pyrolytic graphite tube. It is set to the unit of atomisation of the spectrophotometer.
A volume of 10 μl of tantalum solution is injected on the platform using an automatic distributor of samples;
Put the tantalum solution in the blank’s position on the sample holder.
The temperature cycle is set according to the following programme:
- drying at 100°C for 40 seconds
- mineralisation at 900°C for 60 seconds
- atomisation at 2600°C for 2.5 seconds
- argon is used as an inert gas.
- Reference
- Zatka, Anal. Chem., vol 50, n° 3, March 1978.
Determination of the ability of an enzymatic preparation to interrupt pectic chains by measuring viscosity
COEI-2-VISCPE Determination of the ability of an enzymatic preparation to interrupt pectic chains by measuring viscosity
- Principle
Here, it is proposed to measure the quantity of enzyme needed to halve the viscosity of a standard solution with a given pH, temperature and time.
This is a purely technological measurement designed to test the true clarifying efficiency of the enzyme. It essentially measures the pectinase activity, which cannot be directly deduced from the release of galacturonic acid in the medium.
Comment
To measure the enzyme’s activity, there are two possible approaches:
- Either the time it takes a given concentration of the enzyme to halve the viscosity of the pectin solution,
- Or, the concentration of enzyme needed in order for the pectin solution’s viscosity to be halved in a given period of time.
Tests show that, as long as the substrate is not limiting:
- In the first case, the viscosity logarithm (flow time) is inversely proportional to the reaction time and,
- In the second case, the viscosity logarithm is inversely proportional to the quantity of enzyme in the medium.
- In either case, it is easy to find either the time or the quantity of enzyme needed to halve the viscosity on the basis of a judiciously chosen spectrum.
- Reagent conditions
70 mmol/l phosphate buffer medium 70 mmol/l and 30 mmol/l citrate
Substrate: 70-75 % esterified apple pectin (e.g. Sigma P 8471), diluted to 10 g/l in the buffer solution.
- pH = 3.5
- Temperature: 30 °C
- Reaction time: 15 minutes.
- Pectinase: spectrum of concentrations covering approximately 10 mg/l of enzyme dry weight in the sample; i.e., for example, 0.5 mg in 50 ml of substrate, which corresponds to the quantity of enzyme that is liable to halve the substrate’s viscosity in 15 minutes in the conditions described above.
- Apparatus
3.1. Bath or water circulation thermostat (30 °C 1 °C)
3.2. Capillary flow viscometer (A.3.1: Fig. 2) with a water value (the time for water to flow between the two marks) of approximately 18 to 20 seconds (i.e. a capillary tube roughly 0.5 to 0.6 mm in diameter)
3.3. Timer
3.4. Analytical balance (sensitivity 0,001 g)
3.5. pH meter
3.6. Magnetic stirrer, conventional laboratory glassware
3.7. Rapid paper filters
3.8. Micro-pipettes or micro-syringes for dispensing volumes from 5 to 500 μl
- Pure products
4.1. Pure citric acid (99,5 %)
4.2. Pure disodium hydrogenophosphate (Na2 HPO4·2H2O) (99,0 %)
4.3. 70-75 % esterified apple pectin with more than 90 % purity (e.g. Sigma P 8471)
4.4. Distilled or deionized water
4.5. Pure sodium hydroxide (98 %)
4.6. Pure hydrochloric acid (11.5 M) (33,5 %)
4.7. Pectinase the activity of which is to be measured.
- Solutions
Each solution should be homogenised before using
5.1. M sodium hydroxide
Weigh out 80 g pure sodium hydroxide (4.5) in a 100-ml volumetric flask and dissolve in deionized water (4.4). Top up to the filler mark after complete dissolution and cooling.
5.2. 2M hydrochloric acid
In a 100-ml volumetric flask half-filled with deionized water, place enough pure hydrochloric acid (4.6) to obtain a 2 M solution, (after having topped up to the filler mark).
5.3. 47 mmol/l phosphate buffer, 53 mmol/l citrate, pH 3.5
5.3.1. Put 800 ml deionized water (4.4) in a 1,000-ml volumetric flask
5.3.2. Weigh out 11.22 g citric acid (4.1)
5.3.3. Weigh out 8.30 g pure disodium hydrogenophosphate (Na2 HPO4·2H2O) (4.2)
5.3.4. Transfer the quantitatively-weighed chemical products to the 1,000 ml volumetric flask, stirring all the time
5.3.5. Mix until completely dissolved
5.3.6. Adjust the pH to 3.50 ± 0.05, at ambient temperature, with 2 M sodium hydroxide (5.1) or 2M hydrochloric acid (5.2), depending on the initial pH
5.3.7. Top up to the filler mark with deionized water (4.4). Mix
Stability: 8 days at ambient temperature.
5.4. Substrate: Apple pectin (4.3),
5.4.1. Put a 400-ml cylindrical container into a bath of water with a temperature of 40° C 3° on a rotating stirrer
5.4.2. Add 250 ml of buffer with a pH of 3.5 (5.3), measured exactly, to the cylindrical container
5.4.3. Keep stirring gently at 40 °C
5.4.4. Weigh out 2,500 g ± 0,01 g of pectin (4.3)
5.4.5. Slowly add the pectin whilst stirring vigorously
5.4.6. Then stir slowly for 60 minutes, maintaining the temperature at 40° C
5.4.7. Stop stirring and cool to 30 °C 3 °C
5.4.8. Filter with rapid filter paper (3.8) if necessary (if lumpy)
Stability: 24 hours at ambient temperature.
5.5. 100 g/l dry weight pectinase solution (4.7)
5.5.1. Weigh out 2.50 g 0.01 g of powdered or granulated pectinase
5.5.2. Transfer to a 25-ml volumetric flask
5.5.3. Top up to the filler mark with buffer solution at pH 3.5 (5.3)
5.5.4. Dissolve by stirring for 20 minutes using a magnetic stirrer.
Filter through rapid filter paper if the enzyme is immobilised on an insoluble substance using a rapid filter (3.7)
5.5.5. In the case of a liquid enzymatic preparation, use it directly.
Stability: 4 hours at ambient temperature.
- Measurements
6.1. Put the viscometer in the bath of water at 30 °C or use any device that makes it possible to measure the viscosity at 30 °C.
6.2. Measure the viscosity (the flow time between the two marks on the viscometer) of the buffer solution at pH 3.5; that is, to. This time should be approximately 20 seconds for a capillary tube 0.5 to 0.6 mm in diameter.
6.3. Measure the flow time of the 10 g/l pectin solution, that is, Tp. This time should be approximately 200 seconds or more.
6.4. Prepare a series of 4 volumetric flasks containing 50 ml of 10 g/l pectin and put them in the bath of water at 30 °C.
6.5. Add 5 µl of the 100 g/l enzyme solution to the first flask and homogenize.
Then, approximately every 15 minutes, successively add to the other flasks:
15 μl, 35 μl and 100 μl of the 100 g/l enzyme solution and homogenize.
Measure the time taken by the various solutions to flow between the two marks on the viscometer exactly 15 minutes after adding the enzyme.
- Graphic representation of the measured valued
Deduct the value corresponding to the buffer at pH 3.5 alone from the flow time.
Produce a graph to represent the flow time logarithm as a function of enzyme concentration.
There must be at least three points in a line corresponding to the strongest dilutions. If this is not the case, use a more diluted enzyme solution - 50 g/l or even 10 g/l, for example.
- Interpretation of the results
Find the regression line equation passing through the three aligned points:
Deduct from this the necessary concentration of enzyme C to halve the pectin solution’s viscosity ; that is, .
- Examples
9.1. Determination of the necessary enzyme concentration to halve the viscosity of the pectin solution. (Table 1)
Flow time of the buffer alone to = 19.3 s
Table 1 |
||||
Vol (μl) of 100 g/l enzyme /50 ml of pectin |
Concentration (g/l) |
Flow time(s) |
Corrected time(s) |
Corrected time log. |
0 |
0 |
230 (Tp) |
210.7 (Tp - to) |
2.32 |
5 |
0.01 |
190 |
170.7 |
2.23 |
25 |
0.05 |
107 |
87.7 |
1.94 |
100 |
0.2 |
32.8 |
13.5 |
1.13 |
500 |
1 |
23.8 |
4.5 |
0.65* |
Corrected time = flow time – flow time of buffer with a pH of 3.5
* value not taken into consideration regression line equation (Fig.1)
Therefore, 0.044 g/l of enzyme are needed to halve the viscosity of a 10 g/l apple pectin solution at 30 °C during 15 minutes.
It has been shown that 1 g/l of enzyme was sufficient to almost totally reduce the viscosity of the pectin solution in 15 minutes.
Fig.1 Reduction in the viscosity of a pectin solution as a function of enzyme concentration |
9.2. Reduction in the viscosity of a 10 g/l pectin solution as a function of the reaction time at 30 °C of an enzyme with a concentration of 0.1 g/l. (Fig. 2) – For information only
The buffer flow time was 19.6 seconds.
Table 2:
Table 2: |
|||
Reaction time (mn) |
Flow time(s) |
Corrected flow time(s)* |
Flow time log. |
0 |
170 (Tp) |
150.7 (Tp - to) |
2.18 |
11.5 |
101.4 |
82.1 |
1.91 |
15.6 |
86 |
66.7 |
1.82 |
21.08 |
72.8 |
53.5 |
1.73 |
29 |
59.83 |
40.53 |
1.61 |
40.31 |
48.79 |
29.49 |
1.47 |
57 |
40.08 |
20.78 |
1.32 |
90 |
32.25** |
12.95 |
1.11 |
167 |
26.25** |
6.95 |
0.84 |
* Corrected flow time
**Values not taken into consideration since the remaining quantity of pectin limits the reaction.
|
|
Fig. 2. Changes in the viscosity of a 10 g/l pectin solution as a function of the reaction time of a 0.1 g/l enzyme at 30 °C |
Fig.3. Changes in the viscosity of a 10 g/l pectin solution as a function of the reaction time logarithm of a 0.1 g/l enzyme at 30 °C. |
Interpretation of the results
The values in table 4 show that a T/2 reaction time of 13.3 minutes is needed to halve the viscosity of the 10 g/l pectin solution at 30 °C.
For the calculation, on the basis of the regression line in Fig. 3:
- Bibliography
- Bertrand A. determination de la capacité d'une préparation enzymatique de type polygalacturonase a couper les chaines pectiques par la mesure de la viscosité OIV FV 1260
Zinc- Determination by AAS
COEI-2-ZINC Determination of zinc by atomic absorption spectrometry
- Principle
The zinc is determined directly by atomic absorption spectrometry by flame.
- Apparatus
Instrumental parameters: (given as an example)
- atomic absorption spectrometer
- oxidant air-acetylene flame
- wave length: 213.9 nm
- hollow-cathode lamp (zinc)
- width of slit: 0.5 nm
- intensity of the lamp: 3.5 mA
- correction of the non specific absorption with a deuterium lamp.
- Reagents
3.1. Pure demineralised water for analysis
3.2. Pure nitric acid for analysis at 65%
3.3. Zinc reference solution at 1 g/l commercial or prepared as follows: dissolve 4.5497 g of Zn(NO3)2. 6H2O in a solution of HNO3 0.5 M, adjust at 1 l with HNO3 0.5 M.
3.4. Zinc solution at 10 mg/l:
- place 1 ml of the zinc reference solution in a 100 ml graduated flask, 1 ml of nitric acid (3.2) and complete to volume with pure demineralised water for analysis.
- Set of calibration solution: 0.2; 0.4; 0.6; 0.8; 1.0 mg/l: place successively 1, 2, 3, 4, 5 ml of the zinc solution at 10 mg/l in 5, 50 ml graduated flasks, complete to volume with pure demineralised water for analysis.
- Preparation of samples
The liquid or solution samples must have concentrations between 0 and 1 mg/l of zinc.
The solid samples are mineralised by dry process.
The blank solution is made up of pure water for analysis containing 1% of nitric acid at 65%.
- Procedure
Pass successively the blank, the calibration solutions and the samples of oenological products.
The absorbency readings are performed for 10 seconds and the measurements are duplicated.
The concentrations of zinc in the samples are obtained from absorbency values.