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    BS EN 14131-2003 Foodstuffs - Determination of folate by microbiological assay《食品 微生物检定法测定叶酸盐含量》.pdf

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    BS EN 14131-2003 Foodstuffs - Determination of folate by microbiological assay《食品 微生物检定法测定叶酸盐含量》.pdf

    1、BRITISH STANDARD BS EN 14131:2003 Foodstuffs Determination of folate by microbiological assay The European Standard EN 14131:2003 has the status of a British Standard ICS 07.100.30 BS EN 14131:2003 This British Standard, was published under the authority of the Standards Policy and Strategy Committe

    2、e on 12 June 2003 BSI 12 June 2003 ISBN 0 580 42040 X National foreword This British Standard is the official English language version of EN 14131:2003. The UK participation in its preparation was entrusted to Technical Committee AW/-/3, Horizontal analysis, which has the responsibility to: A list o

    3、f organizations represented on this committee can be obtained on request to its secretary. Cross-references The British Standards which implement international or European publications referred to in this document may be found in the BSI Standards Catalogue under the section entitled “International

    4、Standards Correspondence Index”, or by using the “Find” facility of the BSI Standards Electronic Catalogue. A British Standard does not purport to include all the necessary provisions of a contract. Users of British Standards are responsible for their correct application. Compliance with a British S

    5、tandard does not of itself confer immunity from legal obligations. aid enquirers to understand the text; present to the responsible European committee any enquiries on the interpretation, or proposals for change, and keep the UK interests informed; monitor related international and European developm

    6、ents and promulgate them in the UK. Summary of pages This document comprises a front cover, an inside front cover, the EN title page, pages 2 to 19 and a back cover. The BSI copyright date displayed in this document indicates when the document was last issued. Amendments issued since publication Amd

    7、. No. Date CommentsEUROPEANSTANDARD NORMEEUROPENNE EUROPISCHENORM EN14131 June2003 ICS07.100.30 Englishversion FoodstuffsDeterminationoffolatebymicrobiologicalassay ProduitsalimentairesDterminationdesfolatesparessai microbiologique LebensmittelMikrobiologischeBestimmungvonFolat ThisEuropeanStandardw

    8、asapprovedbyCENon21April2003. CENmembersareboundtocomplywiththeCEN/CENELECInternalRegulationswhichstipulatetheconditionsforgivingthisEurope an Standardthestatusofanationalstandardwithoutanyalteration.Uptodatelistsandbibliographicalreferencesconcernings uchnational standardsmaybeobtainedonapplication

    9、totheManagementCentreortoanyCENmember. ThisEuropeanStandardexistsinthreeofficialversions(English,French,German).Aversioninanyotherlanguagemadebytra nslation undertheresponsibilityofaCENmemberintoitsownlanguageandnotifiedtotheManagementCentrehasthesamestatusasthe official versions. CENmembersarethena

    10、tionalstandardsbodiesofAustria,Belgium,CzechRepublic,Denmark,Finland,France,Germany,Greece, Hungary,Iceland,Ireland,Italy,Luxembourg,Malta,Netherlands,Norway,Portugal,Slovakia,Spain,Sweden,SwitzerlandandUn ited Kingdom. EUROPEANCOMMITTEEFORSTANDARDIZATION COMITEUROPENDENORMALISATION EUROPISCHESKOMIT

    11、EEFRNORMUNG ManagementCentre:ruedeStassart,36B1050Brussels 2003CEN Allrightsofexploitationinanyformandbyanymeansreserved worldwideforCENnationalMembers. Ref.No.EN14131:2003EEN14131:2003(E) 2 Contents page Foreword. 3 1 Scope . 3 2 Normativereferences . 3 3 Principle. 3 4 Reagents 4 5 Apparatus 8 6 P

    12、rocedure 9 7 Calculation. 13 8 Precision 14 9 Testreport . 14 AnnexA (informative) Optionalenzymetreatment. 16 AnnexB (informative) Resultsofinterlaboratorytests 19 Bibliography . 20EN14131:2003(E) 3 Foreword Thisdocument(EN14131:2003)hasbeenpreparedbyTechnicalCommitteeCEN/TC275“Foodanalysis Horizon

    13、talmethods”,thesecretariatofwhichisheldbyDIN. ThisEuropeanStandardshallbegiventhestatusofanationalstandard,eitherbypublicationofanidentical textorbyendorsement,atthelatestbyDecember2003,andconflictingnationalstandardsshallbewithdrawn atthelatestbyDecember2003. AnnexesAandBareinformative. Accordingto

    14、theCEN/CENELECInternalRegulations,thenationalstandardsorganizationsofthefollowing countriesareboundtoimplementthisEuropeanStandard:Austria,Belgium,CzechRepublic,Denmark, Finland,France,Germany,Greece,Hungary,Iceland,Ireland,Italy,Luxembourg,Malta,Netherlands, Norway,Portugal,Slovakia,Spain,Sweden,Sw

    15、itzerlandandtheUnitedKingdom. 1Scope ThisEuropeanStandardspecifiesamicrobiologicalmethodforthedeterminationofthetotalfolatecontentof foodstuffsbyturbidimetricdetectionofthegrowthofthemicroorganism Lactobacilluscasei, subsp. rhamnosus(ATCC7469). Themethodallowsforthedeterminationoffolatesinfoodstuffs

    16、,includingnaturallyoccurringfolatesand addedfolicacid(pteroylglutamicacid). 2 Normativereferences ThisEuropeanStandardincorporatesbydatedorundatedreference,provisionsfromotherpublications. Thesenormativereferencesarecitedattheappropriateplacesinthetextandthepublicationsarelisted hereafter.Fordatedre

    17、ferences,subsequentamendmentstoorrevisionsofanyofthesepublicationsapplyto thisEuropeanStandardonlywhenincorporatedinitbyamendmentorrevision.Forundatedreferencesthe latesteditionofthepublicationreferredtoapplies(includingamendments). ENISO3696, WaterforanalyticallaboratoryuseSpecificationsandtestmeth

    18、ods(ISO3696:1987). 3Principle treatmentmaybeusedtofurtherdigestthefoodmatrix.Naturallyoccurringfolylpolyglutamatesare 1tofolylmonoorfolyldiglutamates. Extractedfolatesaredilutedwithbasalmediumcontainingallrequiredgrowthnutrientsexceptfolate.The growthresponseof Lactobacilluscasei ,subsp. rhamnosus(A

    19、TCC7469)toextractedfolatesisfollowed turbidimetricallyandiscomparedtothegrowthresponsetocalibrantsolutionswithknownconcentration. Themethodallowsfortheoptionaluseofasemiautomatedliquidhandlingsystemandofamicroplateortest tubesforincubationofthemicroorganism.EN14131:2003(E) 4 4Reagents 4.1General Dur

    20、inganalysis,unlessotherwisestated,useonlyreagentsofrecognisedanalyticalgradeandwaterofat leastgrade1asdefinedinENISO3696.Thewaterusedforreagentpreparationshallbeglassdistilled. 4.2Solventsandchemicals 4.2.1Glycerol, w(C 3 H 8 O 3 )=80% Mix120mlofglycerolwith30mlofglassdistilledwater. 4.2.21Octanol,C

    21、 8 H 18 O 4.2.3Toluene, C 7 H 8 4.2.42Mercaptoethanol,c(C 2 H 6 OS)=0,1mol/l Add70lof2mercaptoethanolto10mlofwater. 4.2.5 Sodiumascorbate, C 6 H 7 O 6 Na Sodiumascorbateisusedasareagentinseveralsolutionsspecifiedinthisdraftstandard.Ascorbicacidmay equallywellbeused,butproceduresforpHadjustmentmaynee

    22、dtobemodified. 4.2.6 Hydrochloricacid, c(HCl)=1mol/l 4.2.7 Sodiumhydroxide, w(NaOH)=40% Dissolve400gofsodiumhydroxideinwateranddiluteto1l. 4.2.8 Ammoniumsulfate, H 8 N 2 O 4 S 4.2.9Sodium phosphate, monobasic,anhydrous,NaH 2 PO 4 Theamountsofmonobasicsodiumphosphateusedforbufferpreparation(4.3)haveb

    23、eencalculatedforthe anhydroussubstance.Themonoordihydratedsubstancemayalsobeused,withtheproceduresadjusted accordingly. 4.2.10 2(NCyclohexylamino)ethanesulfonicacid(CHES), C 8 H 17 NO 3 S 4.2.11 N(2Hydroxyethyl)piperazineN(2ethanesulfonicacid )(HEPES), C 8 H 18 N 2 O 4 S 4.2.12Carbonpowder, acidwash

    24、ed 4.2.13Saline, sterile Dissolve9gofsodiumchloridein1000mlofwater.Dispense10mlportionsinto20mmx150mmtesttubes. Captubesandheatat+121Cfor15min.Coolandstorerefrigerated.EN14131:2003(E) 5 4.2.14 Folicacidfreebasalmediumsolution, doublestrength Foreach100mlneeded,suspendtherecommendedamountofbasalmediu

    25、m(BactoFolicAcidCasei Mediumorequivalent 1) )in100mlofglassdistilledwater.Add0,050gofsodiumascorbate(4.2.5)andheatto boilingfor1minto2min.AllowcoolingtoroomtemperatureandadjustpHto6,10,1. 4.2.15 Folicacidstandardsubstance Folicacidcanbeobtainedfromvarioussuppliersandmaycontainupto8%water.Thepurityof

    26、thefolicacid standardmayvaryanditisthereforenecessarytodeterminetheconcentrationofthecalibrationsolutionby UVabsorptionmeasurement(seeprocedureforstandardisationin6.4.2). 4.3Buffers 4.3.1 Phosphatebuffer, pH5,0( c=0,002mol/l) Dissolve0,24gofsodiumphosphate,monobasic(4.2.9)in900mlofwater.AdjustpHto5,

    27、00,1with sodiumhydroxide(4.2.7)anddiluteto1000mlwithwater. 4.3.2 Phosphatebuffer, pH7,0( c=0,1mol/l) Dissolve12,0gofsodiumphosphate,monobasic(4.2.9)in900mlofwater.AdjustpHto7,00,1with sodiumhydroxide(4.2.7)anddiluteto1000mlwithwater. 4.3.3 Phosphatebuffer, pH5,0( c=0,1mol/l)with2mercaptoethanol( c=1

    28、0mmol/l) Dissolve12,0gofsodiumphosphate,monobasic(4.2.9)in900mlofwater.AdjustpHto5,00,1,add 0,70mlof2mercaptoethanol(4.2.4)anddiluteto1000mlwithwater. 4.3.4 Phosphatebuffer, pH4,5( c=0,1mol/l)withascorbate(1%) Dissolve12,0gofsodiumphosphate,monobasic(4.2.9)and10gofsodiumascorbate(4.2.5)in900mlof wat

    29、er.AdjustpHto4,50,1withsodiumhydroxide(4.2.7)anddiluteto1000mlwithwater.Preparefreshon dayofuse. 4.3.5 Phosphatebuffer, pH6,1( c=0,1mol/l)withascorbate(1%) Dissolve12,0gofsodiumphosphate,monobasic(4.2.9)and10gofsodiumascorbate(4.2.5)in900mlof water.AdjustpHto6,10,1withsodiumhydroxide(4.2.7)anddilute

    30、to1000mlwithwater.Preparefreshon dayofuse. 4.3.6 Phosphatebuffer, pH7,8( c=0,1mol/l)withascorbate(1%) Dissolve12,0gofsodiumphosphate,monobasic(4.2.9)and10gofsodiumascorbate(4.2.5)in900mlof water.AdjustpHto7,80,1withsodiumhydroxide(4.2.7)anddiluteto1000mlwithwater.Preparefreshon dayofuse. 1) BactoFol

    31、icAcidCaseiMediumisthetradenameofaproductsuppliedbyDifco.Thisinformationisgivenforthe convenienceofusersofthisEuropeanStandardanddoesnotconstituteanendorsementbyCENoftheproductnamed. Equivalentproductsmaybeusediftheycanbeshowntoleadtothesameresults.EN14131:2003(E) 6 4.3.7CHES/HEPES buffer, pH7,85( c

    32、=0,05mol/l)withascorbateand2mercaptoethanol(4.2.4)forthe dialysisofratbloodplasma. Dissolve23,8gofHEPES(4.2.11),20,7gofCHES(4.2.10),40gofsodiumascorbate(4.2.5)and1,4mlof 2mercaptoethanol(4.2.4)in1900mlofwater.AdjustpHto7,850,1withsodiumhydroxide(4.2.7)and diluteto2000mlwithwater.Add4gofacidwashedcar

    33、bonpowder(4.2.12).Preparefreshondayofuse. 4.4Enzymes 4.4.1 Additionalenzymetreatment(optional) ProceduresforadditionalenzymetreatmentarefurtherdiscussedinAnnexA. 4.4.2 4.4.2.1General 0fromoneofseveralsources.An 4.4.2.2). A. The appropriatenessofthechosenenzymepreparationshallbecheckedwithasuitablete

    34、chnique. NOTE Ayeastpowder,lyophilisedpigsliver(e.g.BCRCRM4872),ortoalimitedextentpteroyltriglutamicacidcan beappropriatesamplestouseforthecheckingoftheenzymepreparation. 4.4.2.2 3 Homogenise250goffreshhogkidneyat+2Cin750mlofphosphatebufferwith2mercaptoethanol(4.3.3). Centrifugeat+2C(18000 g,20min).

    35、Incubatesupernatantat+50Cfor2hwithgentleagitationand repeatcentrifugation.Fractionatethesupernatantbyprecipitationwithsaturatedammoniumsulfate(4.2.8). Collectthefractionprecipitatedbetween50%and75%saturationwithammoniumsulfate.Suspend precipitateinaminimalvolumeofphosphatebuffer(4.3.1).Dialyseagains

    36、tthesamebuffer2x24hand centrifuge(18000 g,20min).Transfer1mlaliquotstovialsandlyophilise. 4.5Inoculum 4.5.1 Testorganism Lyophilisedcultureof Lactobacilluscasei subsp. rhamnosus(ATCC7469) 2) . 4.5.2 Culturemedium Dilute50mlofdoublestrengthfolicacidfreebasalmediumsolution(4.2.14)to100mlwithglassdisti

    37、lled water.Add0,5mlofdilutedfolicacidstocksolution(6.4.4),mixandsterilefilterorheatat+121Cfor15min andrapidlycooltoroomtemperature. 4.5.3 Cryoprotectedinoculum Aseptically,add1mlofthepreparedculturemedium(4.5.2)tothelyophilisedculture(4.5.1)andtransfer 0,15mloftheresultingsuspensiontotheculturemediu

    38、maccordingto4.5.2.Incubateat+37Cfor18h. 2) DistributorsincludeNationalCollectionofIndustrialandMarineBacteriaLtd(Aberdeen,UK)andCultureCollection, UniversityofGteborg(Gothenburg,Sweden).ThisinformationisgivenfortheconvenienceofusersofthisEuropean StandardanddoesnotconstituteanendorsementbyCENofthedi

    39、stributorsnamed.EN14131:2003(E) 7 Heat150mlofglycerol(4.2.1)at+121Cfor15minandcoolinicebath.Coolincubatedbacterialculturein icebathandadd100mlsterilisedandcooledglycerol.Mixgently.Dispense2mlaliquotsintosterilevials. Storeat20Cforuptothreemonthsorat70Cforuptosixmonths. NOTE Itisessentialtomaintainas

    40、epticconditionsthroughoutthewholeprocess. 4.5.4 Workinginoculum 4.5.4.1 Workinginoculumfortubecultures Dilute2mlcryoprotectedinoculum(4.5.3)to50mlwithsterilesaline(4.2.13).Vortexmix. 4.5.4.2 Workinginoculumformicroplatecultures(optional) Add5mlofsterilesaline (4.2.13)to2mlcryoprotectedinoculum(4.5.3

    41、).Vortexmix. 4.5.5 Inoculatedfolicacidfreebasalmediumsolution, formicroplateassay(optional). Add1lworkinginoculum(4.5.4.2)per1mlfolicacidfreebasalmediumsolution(4.2.14).Mixthoroughly. 5Apparatus Usuallaboratoryapparatus,glasswareand,inparticular,thefollowing: 5.1Centrifuge,cooled, forpreparationofhogkidneyconjugase(4.4.2.2),suitabl


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