AAT Bioquest/Amplite™ Colorimetric Glucose Quantitation Kit/40004/500 Tests,AAT Bioquest,,AAT Bioquest,aatbio,AAT Bioquest公司代理生物计划 AAT Bioquest药物分子,,Array.Array.Array蚂蚁淘厂家直采.

产品名称：AAT Bioquest/Amplite™ Colorimetric Glucose Quantitation Kit/40004/500 Tests

产品编号：40004

市场价：¥56560.00

场地：美国(厂家直采)

产品分类：试剂盒>其它试剂盒>定量试剂盒>

联系QQ：1570468124

电话号码：4000-520-616

邮箱： info@ebiomall.com

美元价：$2828.00

品牌： AAT Bioquest

公司：AAT Bioquest

公司分类：

商品介绍

Overview

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Ex/Em(nm)	575/None
MW	N/A
CAS#	N/A
Solvent	N/A
Storage	F/D/L
Category	SmallMoleculeDetection DiagnosticMolecules
Related	GlucoseTransporters BiochemicalAssays

Glucose,amonosaccharide,isthemostimportantcarbohydrateinBIOLOGy.Itisasourceofenergyandmetabolicintermediateforcellgrowth.Asoneofthemainproductsofphotosynthesis,glucosestartscellularrespirationinbothprokaryotesandeukaryotes.Glucoselevelisakeydiagnosticparameterformanymetabolicdisorders,e.g.,diabetes.ThisAmplite™ColorimetricGlucoseQuantitationKitprovidesaquickandsensitivemethodforthemeasurementofglucose.Itusesglucoseoxidase-basedenzymecoupledreactionstodetectglucosethroughtheproductionofhydrogenperoxide,whichismonitoredbyourAmplite™Redperoxidasesubstrate.Amplite™Redperoxidasesubstratecanbereadbyanabsorbancemicroplatereaderat~570nm.Theassayisrobust,andcanbereADIlyadaptedforawidevarietyofapplicationsthatrequirethemeasurementofglucose.TheassayhasverylowbackgroundsinceitisrunintheredvisIBLerangethatsignificantlyreducestheinterferencefrombiologicalsamples.WiththeAmplite™ColorimetricGlucoseQuantitationKit,wecandetectaslittleas3?MD-glucose.

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Thisprotocolonlyprovidesaguideline,andshouldbemodifiedaccordingtoyourspecificneeds.

1.Preparestocksolutions:

1.1 250XAmplite™Redstocksolution:Add100µLofDMSO(ComponentE)intothevialofAmplite™Redsubstrate(ComponentA).Thestocksolutionshouldbeusedpromptly.Anyremainingsolutionshouldbealiquotedandrefrozenat-20^oC.

Note1:Avoidrepeatedfreeze-thawcycles.

Note2:TheAmplite™Redsubstrateisunstableinthepresenceofthiolssuchasdithiothreitol(DTT)and2-mercaptoethanol.ThefinalconcentrationofDTTor2-mercaptoethanolinthereactionshouldbenohigherthan10μM.TheAmplite™RedsubstrateisalsounstableathighpH(>8.5).Therefore,thereactionshouldbeperformedatpH7–8.Theprovidedassaybuffer(pH7.4)isrecommended.

1.2 10U/mLHRPstocksolution:Add1mLofassaybuffer(ComponentB)intothevialofhorseradishperoxidase(ComponentC).

Note:TheunusedHRPsolutionshouldbedividedintosingleusealiquotsandstoredat-20^oC.

1.3 100U/mLglucoseoxidasesolution:Add1mLofassaybuffer(ComponentB)intothevialofglucoseoxidase(ComponentD).

Note:Theunusedglucoseoxidasesolutionshouldbedividedintosingleusealiquotsandstoredat-20^oC.

1.4 800mMglucosestocksolution:Add1mLofassaybuffer(ComponentB)intothevialofglucose(ComponentF).

Note:Theunusedglucosesolutionshouldbestoredat-20^oC.

2.Prepareassayreactionmixture:

PrepareAssayreactionmixtureaccordingtothefollowingtables,protectedfromlight.

Table1Assayreactionmixtureforoneclearbottom96-wellmicroplate(2X)

Components	Volume
250XAmplite™RedStockSolution(fromStep1.1)	20μL
10U/mLHRPStockSolution(fromStep1.2)	100μL
100U/mLGlucoseOxidaseSolution(fromStep1.3)	100μL
AssayBuffer(ComponentB)	4.78mL
Totalvolume	5mL

Table2Layoutofglucosestandardsandtestsamplesinaclearbottom96-wellmicroplate

BL	BL	TS	TS	….	….
GS1	GS1	….	….	….	….
GS2	GS2
GS3	GS3
GS4	GS4
GS5	GS5
GS6	GS6
GS7	GS7

Note:GS=Glucosestandards,BL=Blankcontrol,TS=testsamples.

Table3.Reagentcompositionforeachwell

GlucoseStandard	BlankControl	TestSample
SerialDilutions*:50μL	AssayBuffer(ComponentB):50μL	50μL

*Note:Addtheseriallydilutedglucosestandardsfromapproximately1.6µMto100µMintoeachwellfromGS1toGS7induplicate.

3.RunGlucoseassay:

3.1 Prepareaglucosestandardbydilutingtheappropriateamountofthe800mMglucosestocksolution(fromStep1.4)intoassaybuffer(ComponentB)toproduceglucoseconcentrationsof100μM.Thenperform1:2serialdilutionsinassaybuffer(ComponentB)togetapproximately50,25,12.5,6.3,3.1and1.6μMseriallydilutedglucosestandards.Anon-glucosebuffercontrolisincludedasblankcontrol.

3.2 Add50μLofassayreactionmixture(fromStep2)intoeachwellofglucosestandard,blankcontrol,andtestsamples(seeStep2,Table3)tomakethetotalglucoseassayvolumeof100µL/well

Note:Fora384-wellplate,add25μLofsampleand25μLofassayreactionmixtureintoeachwell.

3.3 Incubatethereactionfor10to30minutesat37^oC,protectedfromlight.

3.4 MonitortheabsorbanceincreasewithanabsorbanceplatereaderatOD=570nm.

References&Citations

CitationExplorer

MicroRNAsregulategeneplasticityduringcoldshockinzebrafishlarvae
Authors:I-ChenHung,Yu-ChuanHsiao,HSunnySun,Tsung-MingChen,Shyh-JyeLee
Journal:BMCgenomics(2016):922

Glucosemetabolismandgeneexpressioninjuvenilezebrafish(Daniorerio)challengedwithahighcarbohydratediet:effectsofanacuteglucosestimulusduringlateembryoniclife
Authors:FilipaRocha,JorgeDias,SofiaEngrola,PauloGavaia,IngeGeurden,MariaTeresaDinis,StephanePanserat
Journal:BritishJournalofNutrition(2015):403--413

Glucoseoverloadinyolkhaslittleeffectonthelong-termmodulationofcarbohydratemetabolicgenesinzebrafish(Daniorerio)
Authors:FilipaRocha,JorgeDias,SofiaEngrola,PauloGavaia,IngeGeurden,MariaTeresaDinis,StephanePanserat
Journal:JournalofExperimentalBiology(2014):1139--1149

ImpactofL-FABPandglucoseonpolyunsaturatedfattyacidinductionofPPARα-regulatedβ-oxidativeenzymes
Authors:AncaDPetrescu,HuanHuang,GregoryGMartin,AveryLMcIntosh,StephenMStorey,DaniloLandrock,AnnBKier,FriedhelmSchroeder
Journal:AmericanJournalofPhysiology-GastrointestinalandLiverPhysiology(2013):G241--G256

InhibitorsoffattyacidsynthesisinducePPARα-regulatedfattyacidβ-oxidativegenes:synergisticrolesofL-FABPandglucose
Authors:HuanHuang,AveryLMcIntosh,GregoryGMartin,AncaDPetrescu,KerstinKLandrock,DaniloLandrock,AnnBKier,FriedhelmSchroeder
Journal:PPARresearch(2013)

Aquaporin-9proteinistheprimaryrouteofhepatocyteglyceroluptakeforglycerolgluconeogenesisinmice
Authors:SABInaJelen,SörenWacker,CamiloAponte-Santamaría,MartinSkott,AleksandraRojek,UrbanJohanson,PerKjellbom,SørenNielsen,BertLdeGroot,MichaelRützler
Journal:JournalofBiologicalChemistry(2011):44319--44325

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