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THE COMMISSION OF THE EUROPEAN COMMUNITIES,
Having regard to the Treaty establishing the European Economic Community,
Having regard to Council Directive 76/118/EEC of 18 December 1975 on the approximation of the laws of the Member States relating to certain partly or wholly dehydrated preserved milk for human consumption(1), and in particular Article 11 thereof,
Whereas under Article 11 of Directive 76/118/EEC, the composition of certain partly or wholly dehydrated preserved milk is required to be verified by Community methods of analysis;
Whereas it is desirable to adopt an initial series of methods in respect of which studies have been completed;
Whereas the measures provided for in this Directive are in accordance with the opinion of the Standing Committee of Foodstuffs,
HAS ADOPTED THIS DIRECTIVE:
Member States shall take all measures necessary to ensure that the analyses necessary for verification of the criteria set out in Annex I are carried out in accordance with the methods described in Annex II.
Where alternative methods for a single determination are specified, the sample may be analysed by either method. The test report referred to in Annex II must state the method which has been employed.
Member States shall bring into force the laws, regulations and administrative provisions necessary to comply with this Directive within 18 months of its notification. They shall forthwith inform the Commission thereof.
This Directive is addressed to the Member States.
Done at Brussels, 13 November 1979.
For the Commission
Étienne Davignon
Member of the Commission
unsweetened condensed high fat milk (using method 1, Annex II),
unsweetened condensed milk (using method 1, Annex II),
unsweetened condensed partly skimmed milk (using method 1, Annex II),
unsweetened condensed skimmed milk (using method 1, Annex II),
sweetened condensed milk (using method 1, Annex II),
sweetened condensed partly skimmed milk (using method 1, Annex II),
sweetened condensed skimmed milk (using method 1, Annex II).
dried high fat milk or high fat milk powder (using method 2, Annex II), — dried whole milk or whole milk powder (using method 2, Annex II),
dried partly skimmed milk or partly skimmed-milk powder (using method 2, Annex II),
dried skimmed milk or skimmed-milk powder (using method 2, Annex II).
unsweetened condensed high fat milk (using method 3, Annex II),
unsweetened condensed milk (using method 3, Annex II),
unsweetened condensed partly skimmed milk (using method 3, Annex II),
unsweetened condensed skimmed milk (using method 3, Annex II),
sweetened condensed milk (using method 3, Annex II),
sweetened condensed partly skimmed milk (using method 3, Annex II),
sweetened condensed skimmed milk (using method 3, Annex II),
dried high fat milk or high fat milk powder (using method 4, Annex II),
dried whole milk or whole milk powder (using method 4, Annex II),
dried partly skimmed milk or partly skimmed-milk powder (using method 4, Annex II),
dried skimmed milk or skimmed-milk powder (using method 4, Annex II).
sweetened condensed milk (using method 5, Annex II),
sweetened condensed partly skimmed milk (using method 5, Annex II),
sweetened condensed skimmed milk (using method 5, Annex II).
dried high fat milk or high fat milk powder (using method 6, Annex II),
dried whole milk or whole milk powder (using method 6, Annex II),
dried partly skimmed milk or partly skimmed-milk powder (using method 6, Annex II),
dried skimmed milk or skimmed-milk powder (using method 6, Annex II).
dried high fat milk or high fat milk powder (using method 7 or 8, Annex II),
dried whole milk or whole milk powder (using method 7 or 8, Annex II),
dried partly skimmed milk or partly skimmed-milk powder (using method 7 or 8, Annex II),
dried skimmed milk or skimmed-milk powder (using method 7 or 8, Annex II).
Unsweetened condensed milk
Unsweetened condensed partly skimmed milk
Unsweetened condensed skimmed milk
Shake and invert the closed can. Open the can and slowly pour the milk into a second container which can be closed hermetically, mixing by repeated transfer. Ensure that all remaining fat and milk adhering to the wall and the ends of the can are mixed in with the sample. Close the container. If the contents are not homogeneous warm the container in a waterbath at 40 oC. Shake vigorously every 15 minutes. After two hours, remove the container from the water-bath and let it cool to room temperature. Remove the lid and thoroughly mix the contents of the container with a spoon or spatula (if the fat has separated the sample should not be tested). Store in a cool place.
Sweetened condensed partly skimmed milk
Sweetened condensed skimmed milk
Cans: Warm the closed can in a waterbath at 30 to 40 oC for about 30 minutes. Open the can and thoroughly mix the contents with a spatula or a spoon by making upward, downward, and circular movements in order to obtain an intimate mixture of the top and bottom layers with all the contents. Ensure that the remaining milk adhering to the wall and end of the can is incorporated in the sample. As far as possible, pour the contents into a second container provided with an air-tight lid. Close the container and store in a cool place.
Tubes: Cut the end and pour the contents into a container provided with an air-tight lid. Next, cut the tube lengthwise. Scrape out all material adhering to the interior and mix it carefully with the rest of the contents. Store the container in a cool place.
Dried whole milk or whole milk powder
Dried partly skimmed milk or partly skimmed-milk powder
Dried skimmed milk or skimmed-milk powder
Transfer the milk powder to a clean, dry container (with air-tight lid) of a capacity of twice the volume of the powder. Close the container immediately and thoroughly mix the milk powder by repeatedly shaking and inverting the container. During the preparation of the sample exposure of the milk powder to the atmosphere should be avoided as far as possible to minimize absorption of moisture.
All chemicals used shall be of recognized analytical reagent quality except where otherwise specified.
The lists of equipment contain only those items with a specialized use and items with a particular specification.
Analytical balance means a balance capable of weighing to at least 0,1 mg.
Except where otherwise specified, the results shall be calculated as a percentage by mass of the sample as received by the laboratory.
The result shall not contain more significant figures than are justified by the precision of the method of analysis used.
The test report shall identify the method of analysis used as well as the results obtained. In addition, it shall mention all details of procedure not specified in the method of analysis, or which are optional, as well as any circumstances that may have influenced the results obtained.
The test report shall give all the information necessary for the complete identification of the sample.
This method determines the dry matter content of:
unsweetened condensed high fat milk,
unsweetened condensed milk,
unsweetened condensed partly skimmed milk,
unsweetened condensed skimmed milk,
sweetened condensed milk,
sweetened condensed partly skimmed milk,
sweetened condensed skimmed milk.
The dry matter content of condensed milks: dry matter content as determined by the method specified.
A known amount of the sample is diluted with water, mixed with sand and dried at a temperature of 99 oC ± 1 oC. The mass after drying is the mass of dry matter and is calculated as a percentage by mass of the sample.
Quartz sand or sea sand, treated with hydrochloric acid (size of the grains: 0,18 to 0,5 mm, that is passing through a 500 micron sieve and retained by a 180 micron sieve). It should meet the following control test:
Heat about 25 g of sand for two hours in the drying oven (5.3) as described in 6.1. to 6.3. Add 5 ml of water, heat again in the oven for two hours, cool and reweigh. The difference between the two masses should not exceed 0,5 mg.
If necessary treat the sand with a 25 % hydrochloric acid solution for three days, mixing occasionally. Wash with water until the acid reaction disappears or the wash water is chloride free. Dry at 160 oC and re-test as above.
The content of dry matter, calculated as a percentage by mass of the sample, is given by:
where:
=
mass, in g of the dish, lid and sand after process 6.3;
=
mass, in g of the dish, lid, sand and sample after process 6.4;
=
mass, in g of the dish, lid, sand and dried sample after process 6.11.
The difference between the results of two determinations carried out simultaneously or in rapid succession on the same sample, by the same analyst, under the same conditions, shall not exceed 0,2 g of dry matter per 100 g of the product.
Total dry matter (obtained by method 1, Annex II) — sucrose (obtained by method 5, Annex II).
Total dry matter (obtained by method 1, Annex II) — (sucrose content obtained by method 5, Annex II) and fat content (obtained by method 3, Annex II).
Total dry matter (obtained by method 1, Annex II) — fat content (obtained by method 3, Annex II).
This method determines the loss of mass on drying of:
dried high fat milk or high fat milk powder,
dried whole milk or whole milk powder,
dried partly skimmed milk or partly skimmed-milk powder,
dried skimmed milk or skimmed-milk powder.
Moisture content: the loss of mass on drying as determined by the method specified.
The residual mass of a test portion is determined after drying at atmospheric pressure in an oven at 102 oC ± 1 oC to constant mass. The loss of mass is calculated as a percentage by mass of the sample.
Calculate the loss of mass on drying of the sample, expressed as a percentage by mass, by the formula:
where:
=
mass, in g of the dish and its lid after process 5.2;
=
mass, in g of the dish, its lid and sample after process 5.3;
=
mass, in g of the dish, its lid and final sample after process 5.5.
The difference in results between two determinations carried out simultaneously or in rapid succession on the same sample, by the same analyst, under the same conditions, shall not exceed 0,1 g of moisture per 100 g of product.
This method determines the fat content of:
unsweetened condensed high fat milk,
unsweetened condensed milk,
unsweetened condensed partly skimmed milk,
unsweetened condensed skimmed milk,
sweetened condensed milk,
sweetened condensed partly skimmed milk,
sweetened condensed skimmed milk.
The fat content of condensed milks: fat content as determined by the method specified.
The fat content is determined by extraction of the fat from an ammoniacal alcoholic solution of the sample with diethyl ether and light petroleum followed by evaporation of the solvents and weighing of the residue and calculation as a percentage by mass of the sample, according to the principle of Rose-Gottlieb.
All reagents should conform to the requirements specified in the blank test (6.1). If necessary, reagents may be redistilled in the presence of about 1 g of butterfat for 100 ml of solvent.
Note 1:
To test for peroxides, add to 10 ml of the ether in a small glass stoppered cylinder, previously rinsed with the ether, 1 ml freshly prepared 10 % potassium iodide solution. Shake and let stand for one minute. No yellow colour should be observed in either layer.
Note 2:
Diethyl ether may be maintained free from peroxides by adding wet zinc foil that has been completely immersed in dilute acidified copper sulphate solution for one minute and subsequently washed with water. Use per litre approximately 8 000 mm2 zinc foil; cut in strips long enough to reach at least halfway up the container.
At the same time as the determination of the fat content of the sample, carry out a blank determination on 10 ml of water using the same type of extraction apparatus, the same reagents in the same amounts and the same procedure as described hereafter, excluding clause 6.2.2. If the blank exceeds 0.5 mg, the reagents should be checked and the impure reagent or reagents should be purified or replaced.
Note:
When a centrifuge which is not driven by a three-phase motor, is used, sparks may occur and care must therefore be taken to avoid an explosion or fire from any ether vapours, coming, for example, from a broken tube.
Note:
If the transfer is not made using a siphon, it may be necessary to add a little water in order to raise the interface between the two layers thus aiding decantation.
Note:
It is not mandatory to carry out this third extraction when analysing skimmed unsweetened condensed milk and skimmed sweetened condensed milk samples.
The mass, in g of fat extracted is:
(M1 — M2) — (B1 — B2)
and the fat content of the sample, expressed as a percentage is:
where:
=
mass, in g of flask M with fat after stage 6.2.15;
=
mass, in g of flask M after stage 6.2.1 or, in the case of undissolved material or doubt, stage 6.2.16.2;
=
mass, in g of flask B of the blank after stage 6.2.15;
=
mass, in g of flask B after stage 6.2.1 or, in the case of undissolved material or doubt, stage 6.2.16.2;
=
mass, in g of sample used.
The difference between results of two determinations carried out obtained simultaneously or in rapid succession on the same sample, by the same analyst, under the same conditions, shall not exceed 0,05 g fat per 100 g of the product.
This method determines the fat content of:
dried high fat milk or high fat milk powder,
dried whole milk or whole milk powder,
dried partly skimmed milk or partly skimmed-milk powder,
dried skimmed milk or skimmed-milk powder.
The fat content of dried milks: fat content as determined by the method specified.
The fat content is determined by extraction of the fat from an ammoniacal alcoholic solution of sample with diethyl ether and light petroleum, followed by evaporation of the solvents and weighing of the residue and calculation as a percentage by mass of the sample, according to the principle of Rose-Gottlieb.
All reagents should conform to the requirements specified in the blank test (6.1). If necessary, reagents may be redistilled in the presence of about 1 g of butterfat per 100 ml of solvent.
Note 1:
To test for peroxide, add to 10 ml of the ether in a small glass stoppered cylinder, previously rinsed with the ether, 1 ml freshly prepared 10 % potassium iodide solution. Shake and let stand for one minute. No yellow colour should be observed in either layer.
Note 2:
Diethyl ether may be maintained free from peroxides by adding wet zinc foil that has been completely immersed in dilute acidified copper sulphate solution for one minute and subsequently washed with water. Use per litre approximately 8 000 mm2 zinc foil cut in strips long enough to reach at least halfway up the container.
At the same time as the determination of the fat content of the sample, carry out a blank determination on 10 ml of water using the same type of extraction apparatus, the same reagents in the same amounts and the same procedure as described hereafter, excluding clause 6.2.2. If blank exceeds 0.5 mg, the reagents should be checked and the impure reagent or reagents should be purified or replaced.
Note:
When a centrifuge which is not driven by a three-phase motor is used, sparks may occur and care must therefore be taken to avoid an explosion or fire from any ether vapours coming, for example, from a broken tube.
Note:
If the transfer is not made using a siphon, it may be necessary to add a little water in order to raise the interface between the two layers thus aiding decantation.
Note:
It is not mandatory to carry out this third extraction when analysing dried skimmed milk samples.
Heat the flask, placed on its side, for one hour in the oven, allow to cool to the temperature of the balance room, as before (6.2.1) and weigh to the nearest 0,1 mg. The mass of fat is the difference between the mass under 6.2.15 and this final mass.
The mass, in g of fat extracted is:
(M1 — M2) — (B1 — B2)
and the fat content of the sample, expressed as a percentage, is:
where:
=
mass, in g of flask M with fat after stage 6.2.15;
=
mass, in g of flask M after stage 6.2.1 or, in the case of undissolved material or doubt, stage 6.2.16.2;
=
mass, in g of flask B of the blank after stage 6.2.15;
=
mass, in g of flask B after stage 6.2.1 or, in the case of undissolved material or doubt, stage 6.2.16.2;
=
mass, in g of sample used.
The difference between results of two determinations carried out simultaneously or in rapid succession on the same sample, the same analyst, under the same conditions, shall not exceed 0,2 g fat per 100 g of product with the exception of skimmed-milk powder for which the difference must not exceed 0,1 g fat per 100 g of product.
This method determines the sucrose content of:
sweetened condensed milk,
sweetened condensed partly skimmed milk,
sweetened condensed skimmed milk.
Samples must not contain invert sugar.
The sucrose content of sweetened condensed milks: the sucrose content as determined by the method specified.
The method is based on the principle of the Clerget inversion, a mild treatment of the sample with acid which produces complete hydrolysis of sucrose but almost none of lactose or other sugars. The sucrose content is obtained from the change in rotating power of the solution.
A clear filtrate of the sample, without mutarotation by lactose, is prepared by treatment of the solution with ammonia followed by neutralization and clearing by the successive addition of zinc acetate and potassium hexacyanoferrate II solutions.
In a portion of the filtrate the sucrose is hydrolyzed in a specified manner.
From the rotation of the filtrate before and after inversion, the sucrose content is calculated using the appropriate formulae.
Polarimeter with sodium light or mercury green light (mercury vapour lamp with prism or the special Wratten Screen No 77 A), to be read with an accuracy of at least 0.05 angular degrees,
Saccarimeter with international sugar scale, using white light passing through a filter of 15 mm of a 6 % solution of potassium bichromate, or sodium light, to be read with an accuracy of at least 0,1o on the international sugar scale.
In order to standardize the procedure, reagents and apparatus, carry out a control determination in duplicate as described below using a mixture of 100 g of milk and 18 g pure sucrose or a mixture of 110 g of skimmed milk and 18 g pure sucrose, each corresponding to 40 g of condensed milk containing 45 % sucrose. Calculate the sugar content using the formulae under 7, substituting for M, F and P respectively in formula 1 the quantity of milk taken and the fat and protein content of this milk, and in formula 2 for M, the value of 40,0. The mean of the values found shall not differ by more than 0,2 % from 45,0 %.
Note:
During any of the stages so far described all additions of water or reagents should have been made in such manner as to avoid the formation of air bubbles, and with the same object in view, all mixing should have been carried out by rotation of the flask rather than by shaking. If air bubbles are found to be present before making up to 200 ml volume, their removal can be assisted by temporarily connecting the flask to a vacuum pump, and rotating the flask.
Place the flask in a waterbath of 60 oC for 15 minutes, ensuring that the entire bulb of the flask has been immersed. Mix by a rotatory movement during the first five minutes, in which time the contents of the flask should have attained the temperature of the bath. Cool to 20 oC, and make up to volume with water at 20 oC. Mix and allow to stand for one hour at this temperature.
Determine the rotation of the inverted solution at 20 oC ± 0.2 oC. (However, if temperature T of the liquid in the polarization tube differs by more than 0.2 oC during the measurement, the temperature correction referred to under 7.2 must be applied.)
Calculate the sucrose content by means of the following formulae:
where:
=
sucrose content;
=
mass of the weighed sample in grams;
=
percentage of fat in the sample;
=
percentage Of protein (N x 6.38) in the sample;
=
volume in ml to which the sample is diluted before filtration;
=
correction in ml for the volume of the precipitate formed during clarification;
=
direct polarimeter reading (polarization before inversion);
=
polarimeter reading after inversion;
=
length in dm of the polarimeter tube;
=
inversion factor, the values of which are given below.
Remarks:
When exactly 40,0 g of condensed milk are weighed and a polarimeter with sodium light, angular degrees and a 2dm polarimeter tube at 20,0 oC ± 0,1 oC is used the sucrose content of normal condensed milk (C = 9) can be calculated from the following formula:
S = (D — 1,25 I) x (2,833 — 0,00612 F — 0,00878 P)
If the invert polarization is measured at a temperature other than 20 oC, the figures should be multiplied by:
(1 + 0,0037 (T — 20).
The following formulae give accurate values for Q, for various sources of light with corrections for concentration and temperature:
Sodium light and polarimeter with angular degrees:
=
0,8825 + 0,0006 (C — 9) — 0,0033 (T — 20).
Mercury green light and polarimeter with angular degrees:
=
1,0392 + 0,0007 (C — 9) — 0,0039 (T — 20).
White light with dichromate filter and saccharimeter with international sugar scale degrees:
=
2,549 + 0,0017 (C — 9) — 0,0095 (T — 20).
In the above formulae:
=
Percentage of total sugars in the inverted solution as polarized,
=
Temperature of the inverted solution in the polarimetric reading.
Note 1:
The percentage of total sugars C in the inverted solution may be calculated from the direct reading and the change on inversion in the usual manner, using the usual values for the specific rotations of sucrose, lactose and invert sugar.
The correction 0,0006 (C — 9) etc., is only accurate when C is approximately 9; for normal condensed milk, this correction can be neglected, C being close to 9.
Note 2:
Variation in temperature from 20 oC of 1 oC makes little difference in the direct reading, but variation of over 0,2 oC in the invert reading necessitates a correction. The correction - 0,0033 (T — 20) etc., is only accurate between 18 oC and 22 oC.
The difference between results of two determinations carried out simultaneously or in rapid succession on the same sample, by the same analyst, under the same conditions, shall not exceed 0,3 g of sucrose per 100 g of condensed milk.
This method determines the lactic acid and lactates, expressed as lactic acid, contents of:
dried high fat milk or high fat milk powder,
dried whole milk or whole milk powder,
dried partly skimmed milk or partly skimmed-milk powder,
dried skimmed milk or skimmed-milk powder.
Lactic acid and lactates content of dried milks: the lactic acid and lactates, expressed as lactic acid, contents as determined by the method specified.
Fat, protein and lactose are simultaneously removed from a solution of the sample by addition of copper sulphate and calcium hydroxide followed by filtration.
The lactic acid and lactates in the filtrate are converted into acetaldehyde by concentrated sulphuric acid in the presence of copper II sulphate.
The lactic acid content is determined colorimetrically using p-hydroxydiphenyl.
The lactic acid and lactates content is expressed as mg of lactic acid per 100 g of solids-non-fat.
Note:
All glassware must be perfectly clean and designated for use solely in this determination. Rinse glassware containing precipitate residues with concentrated hydrochloric acid before washing.
Carry out a blank test by placing 30 ml of water into a 50 ml graduated tube and treating this tube as described under 6.2.4 to 6.2.11 inclusive. If the blank measured against water exceeds an equivalent of 20 mg of lactic acid per 100 g solids-non-fat, the reagents should be checked and the impure reagents or reagent should be replaced. Carry out the blank test at the same time as the analysis of the sample.
Note: Avoid contamination with impurities especially with saliva and sweat.
Convert the optical density measured under 6.2.12 or 6.2.13 into mg of lactic acid per 100 g of solids-non-fat in the sample by reference to the standard curve. Multiply this result by the dilution factor where the filtrate has been diluted according to 6.2.13.
The difference between the results of two determinations carried out simultaneously or in rapid succession on the same sample, by the same analyst, under the same conditions, shall not exceed 8 mg of lactic acid per 100 g of solids-non-fat for contents up to 80 mg. For higher values, this difference may not exceed 10 % of the lowest value.
This method describes the determination of phosphatase activity in:
dried high fat milk or high fat milk powder,
dried whole milk or whole milk powder,
dried partly skimmed milk or partly skimmed-milk powder,
dried skimmed milk or skimmed-milk powder.
The phosphatase activity of dried milks is a measure of the quantity of active alkaline phosphatase present. It is expressed as the quantity of phenol in μg liberated by 1 ml of reconstituted milk, as determined by the procedure described below.
The phosphatase activity of dried milks is determined by the ability of the phosphatase to liberate the phenol from disodiumphenylphosphate. The quantity of phenol liberated under prescribed conditions is determined by a spectrophotometric measurement of the colour developed with Gibb's reagent.
Barium borate hydroxide buffer: pH 10,6 ± 0,1 at 20 o C.
Dissolve: 25,0 g of barium hydroxide (Ba(OH)2.8H2O) in water and dilute to 500 ml.
Dissolve: 11,0 g of boric acid (H3BO3) in water and dilute to 500 ml.
Warm the two solutions to 50 o C and mix.
Shake and cool the mixture to room temperature.
Adjust the pH to 10,6 ± 0,1 with the barium hydroxide solution and filter.
Store the solution in a tightly stoppered container.
Before use, dilute the buffer with an equal quantity of water.
Colour development buffer.
Dissolve: 6,0 g of sodium metaborate (NaBO2) (or 12,6 g of NaBO2.4H2O) and 20,0 g of sodium chloride (NaCl) in water and dilute to 1 000 ml with water.
Buffer substrate solution.
Precipitant.
Dissolve 3,0 g of zinc sulphate (ZnSO4.7H2O) and 0,6 g of copper (II) sulphate (CUSO4.5H2O) in water and make up to 100 ml with water.
Gibb's reagent.
Dissolve 0,040 g of 2,6-dibromoquinone 1,4 — chloroimide (O.C6H2Br2.NCl) in 10 ml of 96 % ethanol. Store the solution in a dark glass bottle kept in a refrigerator. Discard this reagent when it has become discoloured.
Dilute 10 ml of Solution B (4.2), colour development buffer, to 100 ml with water.
Dissolve 0,05 g of copper (II) sulphate (CUSO4.5H2O) in water and make to 100 ml with water.
Dissolve 0,2 ± 0,001 g of pure phenol in water and make up to 100 ml in a volumetric flask with water. This solution can be stored for several months in a refrigerator. Dilute 10 ml of this solution to 100 ml with water. This diluted solution contains 200 μg of phenol in 1 ml and can be used for preparing more dilute solutions.
Precautions:
Avoid direct exposure to sunlight.
All the glassware, stoppers and removal material should be perfectly clean. It is recommended that they be rinsed and boiled with water or that they be treated with steam.
Avoid using plastic materials (stoppers for example) as they may contain phenols.
Saliva contains phosphatase; contamination by traces of saliva must therefore be carefully avoided.
If this limit is exceeded, dilute a suitable volume of reconstituted milk according to 6.1.1 with a suitable volume of this milk carefully boiled as indicated in 6.2.2 to inactivate the phosphatase present.
Phosphatase activity = 2,4 x P
where P = the quantity of phenol in μg according to 8.1.1.
The difference between the results of two determinations carried out simultaneously or in rapid succession on the same sample, by the same analyst, under the same conditions, shall not exceed 2 μg of phenol liberated by 1 ml of reconstituted milk.
This method describes the determination of phosphatase activity in:
dried high fat milk or high fat milk powder,
dried whole milk or whole milk powder,
dried partly skimmed milk or partly skimmed-milk powder,
dried skimmed milk or skimmed-milk powder.
The phosphatase activity of dried milks is a measure of the quantity of active alkaline phosphatase present in the product. It is expressed as the quantity of p-nitrophenol in micrograms liberated by 1 ml of the reconstituted sample, under the conditions described.
The reconstituted sample is diluted with a buffer substrate at pH 10,2 and incubated at a temperature of 37 oC for two hours. Any alkaline phosphatase present in the sample will, under these circumstances, liberate p-nitrophenol from added disodium p-nitrophenyl phosphate. The p-nitrophenol liberated is determined by direct comparison with standard colour glasses in a simple comparator using reflected light.
Dissolve 3,5 g of anhydrous sodium carbonate and 1,5 g of sodium bicarbonate in water and dilute to 1 000 ml in a volumetric flask with water.
Dissolve 1,5 g of disodium p-nitrophenylphosphate in sodium carbonate-bicarbonate buffer (4.1) and dilute to 1 000 ml in a volumetric flask with buffer (4.1).
This solution is stable if stored in a refrigerator (≤ 4 oC) for one month but a colour control test should be carried out on such stored solutions — see 6, precaution number 3.
Dissolve 30,0 g of zinc sulphate (ZnSO4) in water and dilute to 100 ml in a volumetric flask with water.
Dissolve 17,2 g of potassium hexacyanoferrate (II) trihydrate (K4Fe(CN)6.3H20) and dilute to 100 ml in a volumetric flask with water.
Precautions:
After use, test tubes must be emptied, rinsed in water, washed in hot water containing an al kaline detergent, followed by thorough rinsing in clean hot tap water. Finally, they must be rinsed in water and dried before use.
Pipettes must be thoroughly rinsed in clean cold tap water immediately after use, followed by rinsing in water and dried before use.
The test tube stoppers must be thoroughly rinsed in hot tap water immediately after use, followed by boiling for two minutes in water.
The buffer substrate solution (4.2) should remain stable for at least one month if stored in a refrigerator at 4 oC or less. Any instability is denoted by the formation of a yellow colour. Whilst the test is always read against a boiled product control containing the same buffer substrate solution, it is recommended that the solution should not be used if it gives a colour reading in excess of 10 μg when read in a 25 mm cell in the comparator using distilled water in the other 25 mm cell.
Use a separate pipette for each sample and avoid contaminating the pipette with saliva.
The test must not be exposed to direct sunlight at any time.
Dissolve 10 g of the powder in 90 ml of water. The temperature for dissolving the powder must not exceed 35 oC.
The direct reading obtained under 6.2.4 is recorded as μg p-nitrophenol per ml sample or per ml of reconstituted sample.
The difference between the results of two determinations carried out simultaneously or in rapid succession on the same sample, by the same analyst, under the same conditions, shall not exceed 2 μg of p-nitrophenol liberated by 1 ml of reconstituted milk.
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