DIN EN 15652-2009 Foodstuffs - Determination of niacin by HPLC English version of DIN EN 15652 2009-09《食品 高效液相色谱法(HPLC)测定烟酸 英文版本DIN EN 15652-2009-09》.pdf

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1、September 2009DEUTSCHE NORM English price group 12No part of this standard may be reproduced without prior permission ofDIN Deutsches Institut fr Normung e. V., Berlin. Beuth Verlag GmbH, 10772 Berlin, Germany,has the exclusive right of sale for German Standards (DIN-Normen).ICS 67.050!$YN“1544394ww

2、w.din.deDDIN EN 15652Foodstuffs Determination of niacin by HPLCEnglish version of DIN EN 15652:2009-09Lebensmittel Bestimmung von Niacin mit HPLCEnglische Fassung DIN EN 15652:2009-09www.beuth.deDocument comprises 23 pagesDIN EN 15652:2009-09 National foreword This standard has been prepared by Tech

3、nical Committee CEN/TC 275 “Food analysis Horizontal methods” (Secretariat: DIN, Germany). Preliminary work was done by Working Group WG 9 “Vitamins and Carotenoids”. The responsible German body involved in its preparation was the Normenausschuss Lebensmittel und landwirtschaftliche Produkte (Food a

4、nd Agricultural Products Standards Committee), Technical Committee NA 057-01-13 AA Vitamine und Carotinoide. The DIN Standards corresponding to the International Standards referred to in this document are as follows: EN ISO 3696 DIN ISO 3696 ISO 5725-2 DIN ISO 5725-2 National Annex NA (informative)

5、Bibliography DIN ISO 3696, Water for analytical laboratory use Specification and test methods ISO 5725-2, Accuracy (trueness and precision) of measurement methods and results Part 2: Basic method for the determination of repeatability and reproducibility of a standard measurement method 2 EUROPEAN S

6、TANDARD NORME EUROPENNE EUROPISCHE NORM EN 15652 May 2009 ICS 67.050 English Version Foodstuffs Determination of niacin by HPLC Produits alimentaires Dosage de la niacine par CLHP Lebensmittel Bestimmung von Niacin mit HPLC This European Standard was approved by CEN on 23 April 2009. CEN members are

7、 bound to comply with the CEN/CENELEC Internal Regulations which stipulate the conditions for giving this EuropeanStandard the status of a national standard without any alteration. Up-to-date lists and bibliographical references concerning such national standards may be obtained on application to th

8、e CEN Management Centre or to any CEN member. This European Standard exists in three official versions (English, French, German). A version in any other language made by translation under the responsibility of a CEN member into its own language and notified to the CEN Management Centre has the same

9、status as theofficial versions. CEN members are the national standards bodies of Austria, Belgium, Bulgaria, Cyprus, Czech Republic, Denmark, Estonia, Finland,France, Germany, Greece, Hungary, Iceland, Ireland, Italy, Latvia, Lithuania, Luxembourg, Malta, Netherlands, Norway, Poland, Portugal,Romani

10、a, Slovakia, Slovenia, Spain, Sweden, Switzerland and United Kingdom. EUROPEAN COMMITTEE FOR STANDARDIZATION COMIT EUROPEN DE NORMALISATION EUROPISCHES KOMITEE FR NORMUNG Management Centre: Avenue Marnix 17, B-1000 Brussels 2009 CEN All rights of exploitation in any form and by any means reserved wo

11、rldwide for CEN national Members. Ref. No. EN 15652:2009: EEN 15652:2009 (E) 2 Contents Page Foreword 31 Scope 42 Normative references 43 Principle 44 Reagents .45 Apparatus .76 Procedure 107 Calculation . 118 Precision 129 Test report . 14Annex A (informative) Typical chromatogram 15Annex B (inform

12、ative) Precision data for acid-, enzymatic- and acid/alkaline hydrolysis . 16Annex C (informative) Comparison between three different ways of hydrolysis 19Bibliography . 21DIN EN 15652:2009-09 EN 15652:2009 (E) 3 Foreword This document (EN 15652:2009) has been prepared by Technical Committee CEN/TC

13、275 “Food analysis - Horizontal methods”, the secretariat of which is held by DIN. This European Standard shall be given the status of a national standard, either by publication of an identical text or by endorsement, at the latest by November 2009, and conflicting national standards shall be withdr

14、awn at the latest by November 2009. Attention is drawn to the possibility that some of the elements of this document may be the subject of patent rights. CEN and/or CENELEC shall not be held responsible for identifying any or all such patent rights. WARNING The use of this standard may involve hazar

15、dous materials, operations and equipment. This standard does not purport to address all the safety problems associated with its use. It is the responsibility of the user of this standard to establish appropriate safety and health practices and determine the applicability of regulatory limitations pr

16、ior to use. According to the CEN/CENELEC Internal Regulations, the national standards organizations of the following countries are bound to implement this European Standard: Austria, Belgium, Bulgaria, Cyprus, Czech Republic, Denmark, Estonia, Finland, France, Germany, Greece, Hungary, Iceland, Irel

17、and, Italy, Latvia, Lithuania, Luxembourg, Malta, Netherlands, Norway, Poland, Portugal, Romania, Slovakia, Slovenia, Spain, Sweden, Switzerland and the United Kingdom. DIN EN 15652:2009-09 EN 15652:2009 (E) 4 1 Scope This European Standard specifies a method for the determination of the mass fracti

18、on of niacin in foodstuffs by high performance liquid chromatography (HPLC) by three different ways of hydrolysis, acid hydrolysis (A), enzymatic hydrolysis (B) or acid/alkaline hydrolysis (C). The method has been validated in interlaboratory tests on fortified and non-fortified samples such as brea

19、kfast cereal powder, chocolate cereals, cooked ham, green peas, lyophilized green peas with ham, lyophilized soup, nutritive orange juice, milk powder and wheat flour, at levels from 0,5 mg/100 g to 24 mg/100 g. For further information on the validation data, see Annex B. A and B give similar result

20、s for niacin. In options A and B niacin is calculated as the sum of nicotinamide and nicotinic acid, and expressed as nicotinic acid 1. Option C gives higher results than A and B for niacin with non-supplemented cereals, but similar results for other products. In option C, niacin is calculated and e

21、xpressed as nicotinic acid after transformation of nicotinamide into nicotinic acid 2. Option A is faster and cheaper than B and C. Option B is used if an exact quantification of nicotinamide and nicotinic acid is needed. This cannot be done with option A, because there is a slight transformation of

22、 nicotinamide into nicotinic acid during the acid hydrolysis. Option C quantifies total niacin. The alkaline hydrolysis is able to liberate other forms giving higher results for niacin, which in some foods such as maize and cereals are not normally biologically available, see 3, 4 and 5. Information

23、 on a comparison between the three different ways of hydrolysis is given in Annex C. 2 Normative references The following referenced documents are indispensable for the application of this document. For dated references, only the edition cited applies. For undated references, the latest edition of t

24、he referenced document (including any amendments) applies. EN ISO 3696:1995, Water for analytical laboratory use Specification and test methods (ISO 3696:1987) 3 Principle Niacin vitamers are extracted from food by an acid (option A), an enzymatic (option B) or an acid/alkaline (option C) treatment

25、and quantified by HPLC with a fluorimetric detection after a post-column derivatization with UV irradiation, see 1 and 2. For option A and option B, niacin is determined as the sum of nicotinamide and nicotinic acid. Niacin is expressed as nicotinic acid after correction of the molecular weights. Fo

26、r option C, niacin is determined and expressed as nicotinic acid. The alkaline treatment transforms all nicotinamide into nicotinic acid. 4 Reagents 4.1 General During the analysis, unless otherwise stated, use only reagents of recognized analytical grade and water of at least grade 1 according to E

27、N ISO 3696:1995. DIN EN 15652:2009-09 EN 15652:2009 (E) 5 4.2 Chemicals and solutions 4.2.1 Sodium acetate, mass fraction w(C2H3NaO2) 99 % 4.2.2 Potassium monohydrogen phosphate, w(K2HPO4) 99,5 % 4.2.3 Potassium dihydrogen phosphate, w(KH2PO4) 99,5 % 4.2.4 Non stabilized hydrogen peroxyde solution,

28、w(H2O2) = 30 % 4.2.5 Copper sulfate, w(Cu(II)SO45H2O) 99 % 4.2.6 Acetic acid, w(CH3COOH) 99,8 % 4.2.7 Concentrated hydrochloric acid solution (option A and C), w(HCl) = 37,0 % 4.2.8 NADase from Neurospora crassa (option B), enzyme activity 0,55 U/mg of protein. Store below 0 oC. NOTE For the interla

29、boratory study, NADase from Neurospora crassa from Sigma Chemicals with reference N 9629, lyophilised powder, 0,5 U/mg to 3,0 U/mg protein (biuret) has been used1. 4.2.9 Acetic acid solution, substance concentration c(CH3COOH) = 5 mol/l 4.2.10 Sodium acetate solution, c(C2H3NaO2)= 2,5 mol/l 4.2.11 C

30、opper sulfate solution, c(Cu(II)SO4.5H2O) = 0,005 mol/l 4.2.12 Sodium acetate solution (option B), c(C2H3NaO2)= 0,05 mol/l, pH = 4,5 Dissolve 4,10 g of sodium acetate (4.2.1) in 900 ml of water. Adjust the solution to pH = 4,5 with acid acetic (4.2.6), and then dilute to 1000 ml with water. 4.2.13 P

31、hosphate buffer solution (option B), c(K2HPO4) = 0,05 mol/l and c(KH2PO4) = 0,05 mol/l, pH = 6,8 Mix 1 part per volume of K2HPO4solution (0,05 mol/l) and 1 part per volume of KH2PO4solution (0,05 mol/l). Adjust pH to 6,8 with sodium acetate solution (4.2.10) if necessary. 4.2.14 NADase solution (opt

32、ion B) Dissolve 2,9 mg of NADase (4.2.8) in 5 ml of phosphate buffer (4.2.13). This solution is stable for 1 week at -18 C. 4.2.15 Hydrochloric acid solution (options A and C), c(HCl) = 0,1 mol/l 1 This information is given for the convenience of users of this European Standard and does not constitu

33、te an endorsement by CEN of the product named. Equivalent products may be used if they can be shown to lead to the same results. DIN EN 15652:2009-09 EN 15652:2009 (E) 6 4.2.16 HPLC mobile phase Dissolve 4,77 g of potassium dihydrogen phosphate (4.2.3) in 400 ml of water. Add 3,8 ml of hydrogen pero

34、xide solution (4.2.4) and 0,5 ml of copper sulfate solution (4.2.11). Dilute to 500 ml. The pH is about 4,5. Filter through a membrane filter (5.7). This solution is stable for one day. 4.2.17 Sodium hydroxide (option C), w(NaOH) 99 % 4.2.18 Sodium hydroxide solution (option C), c(NaOH) = 5 mol/l Di

35、ssolve 20 g of sodium hydroxide (4.2.17) in 80 ml of water. After cooling dilute to 100 ml. 4.2.19 Hydrochloric acid solution (option C), w(HCl) = 3,7 % Dilute 5 ml of the concentrated hydrochloric acid solution (4.2.7) to 50 ml with water. 4.3 Standard substances 4.3.1 General Nicotinic acid and ni

36、cotinamide can be obtained from various suppliers. The purity may vary and it is therefore necessary to determine the concentration of the calibration solution by a spectrometric determination (see 4.4.3). 4.3.2 Nicotinic acid, w(C6H5NO2) 99,5 % 4.3.3 Nicotinamide (options A and B), w(C6H6N2O) 99,5

37、% 4.4 Stock solutions 4.4.1 Nicotinic acid stock solution, mass concentration (C6H5NO2) = 1 mg/ml Dissolve an amount of the nicotinic acid standard substance (4.3.2), e.g. approximately 100 mg to the nearest 1 mg in 100 ml of water. This solution is stable for 1 week at -18 C. 4.4.2 Nicotinamide sto

38、ck solution, (options A and B), (C6H6N2O) = 1 mg/ml Dissolve an amount of the nicotinamide standard substance (4.3.3), e.g. approximately 100 mg to the nearest 1 mg in 100 ml of water. This solution is stable for 1 week at -18 C. 4.4.3 Concentration tests 4.4.3.1 Nicotinic acid solution, (C6H5NO2) =

39、 1 mg/ml Dilute 1 ml of the nicotinic acid stock solution (4.4.1) in 100 ml of hydrochloric acid solution (4.2.15) and measure the absorbance at 260 nm in a 1 cm cell using a UV spectrometer (5.2) against hydrochloric acid solution (4.2.15) as reference. Calculate the mass concentration, , in millig

40、ram per millilitre of the stock solution, using Equation (1): 4201000260=A (1) where DIN EN 15652:2009-09 EN 15652:2009 (E) 7 A260 is the absorbance value of the solution at 260 nm; 420 is the % 1cm 1E value for nicotinic acid in 0,1 mol/l HCl, see 6. 4.4.3.2 Nicotinamide solution, (C6H6N2O) = 1 mg/

41、ml Dilute 1 ml of the nicotinamide stock solution (4.4.2) in 100 ml of hydrochloric acid solution (4.2.15) and measure the absorbance at 260 nm in a 1 cm cell using a UV spectrometer (5.2) against hydrochloric acid solution (4.2.15) as reference. Calculate the mass concentration, , in milligram per

42、millilitre of the stock solution, using Equation (2): 4101000260=A (2) where A260is the absorbance value of the solution at 260 nm; 410 is the % 1cm 1E value for nicotinamide in 0,1 mol/l HCl, see 6. 4.5 Nicotinic acid and nicotinamide standard solutions, (C6H5N02) = (C6H6N2O) = 0,05 g/ml to 5 g/ml

43、Prepare e.g. a first solution with 1 ml of each stock solution (4.4.1) or (4.4.2) in 100 ml of water. From this solution prepare four standard solutions (0,5 ml, 2,5 ml, 10 ml and 50 ml) in 100 ml of water. These solutions are stable for one day at room temperature. 5 Apparatus 5.1 General Usual lab

44、oratory apparatus and glassware, and the following. 5.2 UV spectrometer Capable of measurement of absorbance at defined wavelenghts 5.3 Oven, capable of maintaining a temperature of 37C 5.4 Autoclave, capable of maintaining a temperature of 120C 5.5 HPLC system Consisting of a pump, sample injecting

45、 device, fluorescence detector with excitation and emission wavelengths set at 322 nm and 380 nm, and an evaluation system such as an integrator. DIN EN 15652:2009-09 EN 15652:2009 (E) 8 5.6 Analytical reverse phase separating column, e.g. LiChrospher60 RP-18 Select B endcapped2The column, with the

46、following characteristics, shall ensure a baseline resolution of the analytes concerned: a) a length of 25 cm; b) an inner diameter of 4,0 mm; c) a particle size of 5 m. Other particle sizes or column dimensions than specified in this European Standard may be used. Separation parameters shall be ada

47、pted to such other materials to guarantee equivalent results. 5.7 Filter device Membrane filter with a pore size of for example 0,45 m. 5.8 Post-column derivatization tube and UV lamp A polytetrafluoroethylene (PTFE) tube (length of 5 m, inner diameter of 0,5 mm, external diameter of 1,6 mm) surroun

48、ding a UV black-light-blue (BLB) lamp with low-pressure tube (VL-120 BLB, 20 W, 365 nm, intensity is 55 W/cm2from Vilber Lourmat)2), see Figure 1 and Figure 2 and also 7. WARNING 1 Harmful UV light could come out of the metal box containing the lamp. WARNING 2 If bubble formation occurs in the tube

49、due to overheating, the tube should be efficiently cooled by air circulation, for example by lifting the box. 2 LiChrospher60 RP-18 Select B endcapped and VL-120 BLB are examples of suitable products available commercially. This information is given for the convenience of users of ths European Standard and does not constitute an endorsement by CEN of the product named. Equivalent products may be used if they can be shown to lead to the same results. DIN EN 15652:2

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