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Epigentek/MethylFlash Urine N6methyladenosine (m6A) Quantification Kit (Colorimetric)/P901548/48 188bio精品生物—专注于实验室精品爆款的电商平台 - 蚂蚁淘旗下精选188款生物医学科研用品
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Epigentek/MethylFlash Urine N6methyladenosine (m6A) Quantification Kit (Colorimetric)/P901548/48

InputType:Urine
ResearchArea:RNAMethylation
TargetApplication:AmountQuantitation
VesselFormat:96-WellPlate
100%Guarantee:6months
ProductOverview

The MethylFlash™UrineN6-methyladenosine(m6A)QuantificationKit(Colorimetric) isacompletesetofoptimizedbuffersandreagentstocolorimetricallyquantifym6A inurineusinganinhibitorycompetitiveimmunoassaymethod.Itissuitablefordetectingtotalurinarym6A levels,resultingfromwholebodyturnoverordegradationofDNA/RNAcontainingm6A,usingurinefromhumansandanimals. Theurinesamplescanbeinfreshorfrozenform.Thekithasthefollowingadvantagesandfeatures:

  • Innovativecolorimetricassaywitheasy-to-followstepsforconvenienceandspeed.Theentireprocedurecanbefinishedwithin4hours.
  • 96strip-wellmicroplateformatmakestheassayflexIBLe:manualorhighthroughputanalysis.
  • Innovativekitcompositionenablesbackgroundsignalstobeextremelylow,whicheliminatestheneedforplateblockingandallowstheassaytobesimple,accurate,reliable,andconsistent.
  • Thelevelofm6AmeasuredinhumanurinesamplesusingthiskitiscomparabletothatdetectedbyHPLCmethod. 
  • Anovelassayprincipleallowshighsensitivitytobeachieved.Thedetectionlimitcanbeaslowas0.01ng/assaywell.
  • Lowinputrangeofurineforeachassaywithavolumeof1to20µlandanoptimalvolumeof5µl.
  • Optimizedantibodyandenhancersolutionsallowforhighspecificitytom6A,withoutcross-reactivitytounmethylatedadenosine. 
  • Negativecontrolandpositivestandardareincluded,whicharesuitableforquantificationofm6Ainfreeformandm6AcontainedinDNA/RNAfragmentsfromdifferenturinesamples.

BackgroundInformation 
Nucleobasem6A,amodifiedformofadenosineconvertedbyadenosinemethyltransferasesiswidespreadindifferentcellularRNAsandalsofoundinDNA.TheBIOLOGicalimportanceofDNA/RNAm6A-methylationasamajorepigeneticmodificationinphenotypeandgeneexpressionhasbeenrecognizedwidely.m6AplayscrucialrolesinregulatingDNAreplication,DNAdamage,RNAsplicing,transposition,transcription,andcellulardefense.Inhumans,them6AmodificationisprobablycatalyzedbyamethyltransferasecomplexMETTL3/METTL14andremovedbytheα-ketoglutarate(α-KG)-andFe2+-dependentdioxygenasessuchasFTO,ALKBH5andTET-likeenzymes.ItwasshownthatMETTL3andα-KG/Fe2+-dependentdioxygenasesplayimportantrolesinmanybiologicalprocesses,rangingfromdevelopmentandmetabolismtofertility. Urinaryexcretionofm6AisanindicationofthewholebodyturnoverorthedegradationofDNA/RNA,especiallytRNA.Theurinarym6Alevelcanbechangedwithachangeofthebodies’turnoverofm6ADNA/RNAoralterationofcellularDNA/RNAm6Astatus.Anumberofstudieshaveindicatedthatm6AexcretedinurinehasthepotentialtoactasacancerbioMarker.Forexample,anelevatedlevelofurinarym6Awasobservedincolorectalcancerpatientswithactivediseasestates. 

Principle&Procedure
InthisELISA-likeinhibitorycompetitiveimmunoassay,urinesamplesandthem6Astandardarefirstincubatedwitham6Aantibodysolutionandthentransferredtostripwellscoatedwithm6Apolynucleotide.ThewelliswashedtoremoveanyunboundreagentsafterincubationandthenadetectionantibodyisaddedtogenerateasignalthatcanbemeasuredcolorimetricallybyreADIngtheabsorbanceinamicroplatespectrophotometer.Becausem6Aintheurinesampleinhibitsthebindingofm6Aantibodytom6Acoatedonthewell,higherconcentrationsofm6Aintheurinesampleleadtoareducedbindingoftheantibodytothem6Aonthewell.ThereforethesignalorODintensitymeasuredfromthewellwillbeinverselyproportionaltotheamountofm6Aintheurinesampleandtheamountofm6Aintheurinesamplecanbequantifiedbyacomparisonwithapredeterminedm6Astandard.

StartingMaterials
Thevolumeofurineforeachassaycanbebetween1and20µl.Foroptimalquantification,theinputurinevolumeshouldbe5µl.

ProductComponents

WB(10XWashBuffer)
BS(BindingSolution)
NC(NegativeControl,100µg/ml)*
PC(PositiveControl, m6A2µg/ml)*
CA(CaptureAntibody,1000X)*
DA(DetectionAntibody,1000X)*
ES(EnhancerSolution)*
FD(FluoroDeveloper)*
FE(FluoroEnhancer)*
DB(DilutionBuffer)
8-WellAssayStrips(WithFrame)

*Spinthesolutiondowntothebottompriortouse.

 

 


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