Deprecated: Required parameter $cat_id follows optional parameter $type in /www/wwwroot/ebimall.com/systems/hong.php on line 2088

Deprecated: Required parameter $where follows optional parameter $tree_id in /www/wwwroot/ebimall.com/systems/hlb.php on line 3505
AntibodiesOnline/UCHL1 ELISA Kit (Ubiquitin Carboxylterminal Esterase L1 (Ubiquitin Thiolesterase)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
您好,欢迎您进入188进口试剂采购网网站! 服务热线:4000-520-616
蚂蚁淘商城 | 现货促销 | 科研狗 | 生物在线

AntibodiesOnline/UCHL1 ELISA Kit (Ubiquitin Carboxylterminal Esterase L1 (Ubiquitin Thiolesterase)

Antigen
UbiquitinCarboxyl-terminalEsteraseL1(UbiquitinThiolesterase)(UCHL1)
  • cb358
  • wu:fc55h08
  • UCHL1
  • UCH-L1
  • park5
  • pgp9.5
  • uch-l1
  • MGC132191
  • uchl1
  • AW822034
  • C88048
  • PGP9.5
  • PGP9.5
  • R75593
  • UCHL-1
  • gad
  • PARK5
  • PGP95
  • Uch-L1
  • ubiquitincarboxyl-terminalesteraseL1(ubiquitinthiolesterase)
  • Ubiquitincarboxyl-terminalhydrolaseisozymeL1
  • ubiquitincarboxyl-terminalesteraseL1
  • ubiquitincarboxy-terminalhydrolaseL1
  • uchl1
  • UCHL1
  • LOC100304750
  • LOC100348287
  • LOC100357806
  • Uchl1
Alternatives
Rat(Rattus)UCHL1ELISAKit
Kitswithalternativereactivityto:
11Human
11Rat(Rattus)
9Mouse(Murine)
2Pig(Porcine)
1Cow(Bovine)
MethodType
SandwichELISA
DetectionRange
20.6-15.000pg/mL
MinimumDetectionLimit
20.6pg/mL
Application
ELISA
Options
Bulkdiscount
Supplier
SupplierProductNo.
PurposeTheChemiluminescentImmunoassaykitisdesignedfortheinvitrosensitivequantitativemeasurementofUCHL1inrattissuehomogenatesandotherbiologicalfluids.
SampleTypeSerum,Plasma,TissueHomogenate,CellLysate,BiologicalFluids
AnalyticalMethodQuantitative
DetectionMethodChemiluminescent
Specificity

ThisassayhashighsensitivityandexcellentspecificityfordetectionofUbiquitinCarboxylTerminalHydrolaseL1(UCHL1).
Nosignificantcross-reactivityorinterferencebetweenUbiquitinCarboxylTerminalHydrolaseL1(UCHL1)andanalogueswasobserved.

Cross-Reactivity(Details)Nosignificantcross-reactivityorinterferencebetweenUbiquitinCarboxylTerminalHydrolaseL1(UCHL1)andanalogueswasobserved.
Sensitivity7.3pg/mL
Components
  • Pre-coated,readytouse96-wellstripplate
  • Platesealerfor96wells
  • StandardDiluent
  • AssayDiluentA
  • AssayDiluentB
  • StopSolution
  • Standard
  • DetectionReagentA
  • DetectionReagentB
  • TMBSubstrate
  • WashBuffer(30×concentrate)
  • Instructionmanual
Materialnotincluded
  • Luminometercapableofreading96-wellmicroplateswiththefollowingparameters:lagtime30.0secs,readtime1.0sec/well.
  • Precisionsingleormulti-channelpipettesandpipettetipswithdisposabletips.
  • EppendorfTubesfordilutingsamples.
  • Deionizedordistilledwater.
  • Absorbentpaperforblottingthemicrotiterplate.
  • ContainerforWashSolution
AlternativeNameUCHL1(UCHL1ELISAKitAbstract)
UniProtQ00981
PathwaysFeedingBehaviour
ApplicationNotes
  • Limitedbythecurrentconditionandscientifictechnology,wecannotcompletelyconductthecomprehensiveidentificationandanalysisontherawmaterialprovidedbysuppliers.Sotheremightbesomequalitativeandtechnicalriskstousethekit.
  • Thefinalexperimentalresultswillbecloselyrelatedtovalidityoftheproducts,operationskillsoftheendusersandtheexperimentalenvironments.Pleasemakesurethatsufficientsamplesareavailable.
  • Kitsfromdifferentbatchesmaybealittledifferentindetectionrange,sensitivityandcolordevelopingtime.
  • Donotmixorsubstitutereagentsfromonekitlottoanother.Useonlythereagentssuppliedbymanufacturer.
  • Protectallreagentsfromstronglightduringstorageandincubation.Allthebottlecapsofreagentsshouldbecoveredtightlytopreventtheevaporationandcontaminationofmicroorganism.
  • Theremaybesomefoggysubstanceinthewellswhentheplateisopenedatthefirsttime.Itwillnothaveanyeffectonthefinalassayresults.Donotremovemicrotiterplatefromthestoragebaguntilneeded.
  • Wrongoperationsduringthereagentspreparationandloading,aswellasincorrectparametersettingfortheplatereadermayleadtoincorrectresults.Amicroplateplatereaderwithabandwidthof10nmorlessandanopticaldensityrangeof0-3O.D.orgreaterat450±10nmwavelengthisacceptableforuseinabsorbancemeasurement.Pleasereadtheinstructioncarefullyandadjusttheinstrumentpriortotheexperiment.
  • Eventhesameoperatormightgetdifferentresultsintwoseparateexperiments.Inordertogetbetterreproducibleresults,theoperationofeverystepintheassayshouldbecontrolled.Furthermore,apreliminaryexperimentbeforeassayforeachbatchisrecommended.
  • EachkithasbeenstrictlypassedQ.Ctest.However,resultsfromendusersmightbeinconsistentwithourin-housedataduetosomeunexpectedtransportationconditionsordifferentlabequipments.Intra-assayvarianceamongkitsfromdifferentbatchesmightarisefromabovefactors,too.
  • Kitsfromdifferentmanufacturersforthesameitemmightproducedifferentresults,sincewehavenotcomparedourproductswithothermanufacturers.
Comment

Informationonstandardmaterial:
Thestandardmightberecombinantproteinornaturalprotein,thatwilldependonthespecifickit.Moreover,theexpressionsystemisE.colioryeastormammalcell.Thereis0.05%proclin300inthestandardaspreservative.

Informationonreagents:
Thestopsolutionusedinthekitissulfuricacidwithconcentrationof1mol/L.AndthewashsolutionisTBS.Thestandarddiluentcontains0.02%sodiumazide,assaydiluentAandassaydiluentBcontain0.01%sodiumazide.SomekitscancontainisBSAinthem.

Informationonantibodies:
Theprovidedantibodiesandtheirhostvaryindifferentkits.

SampleVolume100μL
AssayTime3h
PlatePre-coated
ProtocolThemicroplateprovidedinthiskithasbeenpre-coatedwithanantibodyspecifictoUbiquitinCarboxylTerminalHydrolaseL1(UCHL1).Standardsorsamplesarethenaddedtotheappropriatemicroplatewellswithabiotin-conjugatedantibodyspecifictoUbiquitinCarboxylTerminalHydrolaseL1(UCHL1).Next,AvidinconjugatedtoHorseradishPeroxidase(HRP)isaddedtoeachmicroplatewellandincubated.ThenthemixtureofsubstrateAandBisaddedtogenerateglowlightemissionkinetics.Uponplatedevelopment,theintensityoftheemittedlightisproportionaltotheUbiquitinCarboxylTerminalHydrolaseL1(UCHL1)levelinthesampleorstandard.,
ReagentPreparation
  • Bringallkitcomponentsandsamplestoroomtemperature(18-25°C)beforeuse.
  • Standard-ReconstitutetheStandardwith1.0mLofStandardDiluent,keptfor10minutesatroomtemperature,shakegently(nottofoam).Theconcentrationofthestandardinthestocksolutionis5,000pg/mL.Pleaseprepare7tubescontaining0.5mLStandardDiluentandproduceadoubledilutionseries.Mixeachtubethoroughlybeforethenexttransfer.Setup7pointsofdilutedstandardsuchas5,000pg/mL,2,500pg/mL,1,250pg/mL,625pg/mL,312pg/mL,156pg/mL,78pg/mL,andthelastEPtubeswithStandardDiluentistheblankas0pg/mL.
  • AssayDiluentAandAssayDiluentB-Dilute6mLofAssayDiluentAorBConcentrate(2×)with6mLofdeionizedordistilledwatertoprepare12mLofAssayDiluentAorB.(Infact,morethan6mLAssayDiluentAandAssayDiluentBarecontainedinthebottles.Therefore,ineverytest,pleasepreciselypipetterequiredamountofDiluentandmakedoubledilutioninanewcontainer.Thepreparedworkingdilutioncannotbefrozen.)
  • DetectionReagentAandDetectionReagentB-BrieflyspinorcentrifugethestockDetectionAandDetectionBbeforeuse.DilutetotheworkingconcentrationwithworkingAssayDiluentAorB,respectively(1:100).
  • WashSolution-Dilute20mLofWashSolutionconcentrate(30×)with580mLofdeionizedordistilledwatertoprepare600mLofWashSolution(1×).
  • SubstrateworkingSolution-MixthesubstrateAandBbytheratioof99:1tomakethesubstrateworkingsolution.Mixthoroughly.Forexample,prepare1,000µLSubstrateworkingSolutionwith990µLSubstrateA+10µLSubstrateB.
Note:
  • Makingserialdilutioninthewellsdirectlyisnotpermitted.
  • Preparestandardwithin15minutesbeforeassay.Pleasedonotdissolvethereagentsat37°Cdirectly.
  • PleasecarefullyreconstituteStandardsorworkingDetectionReagentAandBaccordingtotheinstruction,andavoidfoamingandmixgentlyuntilthecrystalsarecompletelydissolved.Tominimizeimprecisioncausedbypipetting,usesmallvolumesandensurethatpipettorsarecalibrated.Itisrecommendedtosuckmorethan10µLforoncepipetting.
  • ThereconstitutedStandards,DetectionReagentAandDetectionReagentBcanbeusedonlyonce.
  • PrepareSubstrateworkingSolutionwithin15minutesbeforeassay.
  • IfcrystalshaveformedintheWashSolutionconcentrate(30×),warmtoroomtemperatureandmixgentlyuntilthecrystalsarecompletelydissolved.
  • Contaminatedwaterorcontainerforreagentpreparationwillinfluencethedetectionresult.
SampleCollectionTissueHomogenates:Thepreparationoftissuehomogenateswillvarydependingupontissuetype.Forthisassay,rinsetissuesinice-coldPBS(0.02mol/L,pH7.0-7.2)toremoveexcessbloodthoroughlyandweighbeforehomogenization.Mincethetissuestosmallpiecesandhomogenizethemin5-10mLofPBSwithaglasshomogenizeronice(MicroTissueGrinderswork,too).Sonicatetheresultingsuspensionwithanultrasoniccelldisrupterorsubjectittotwofreeze-thawcyclestofurtherbreakthecellmembranes.Centrifugatethehomogenatesfor5minutesat5000×g.Removethesupernateandassayimmediatelyoraliquotandstoreat-20°C

BiologicalFluids:Centrifugesamplesfor20minutesat1000×g.Removeparticulatesandassayimmediatelyorstoresamplesinaliquotat-20°Cor-80°Cforlateruse.Avoidrepeatedfreeze/thawcycles.
SamplePreparation
  • Weareonlyresponsibleforthekititself,butnotforthesamplesconsumedduringtheassay.Theusershouldcalculatethepossibleamountofthesamplesusedinthewholetest.Pleasereservesufficientsamplesinadvance.
  • Pleasepredicttheconcentrationbeforeassaying.Ifvaluesforthesearenotwithintherangeofthestandardcurve,usersmustdeterminetheoptimalsampledilutionsfortheirparticularexperiments.Sampleshouldbedilutedby0.01mol/LPBS(PH=7.0-7.2).
  • Ifthesamplesarenotindicatedinthemanual,apreliminaryexperimenttodeterminethevalidityofthekitisnecessary.
  • TissueorcellextractionsamplespreparedbychemicallysisbuffermaycauseunexpectedELISAresultsduetotheimpactsfromcertainchemicals.
  • Duetothepossibilityofmismatchingbetweenantigenfromotheroriginandantibodyusedinourkits(e.g.antibodytargetsconformationalepitoperatherthanlinearepitope),somenativeorrecombinantproteinsfromothermanufacturersmaynotberecognizedbyourproducts.
  • Influencedbythefactorsincludingcellviability,cellnumberorsamplingtime,samplesfromcellculturesupernatantmaynotbedetectedbythekit.
  • Freshsampleswithoutlongtimestorageisrecommendedforthetest.Otherwise,proteindegradationanddenaturalizationmayoccurinthosesamplesandfinallyleadtowrongresults.
AssayProcedure
  1. Prepareallreagents,samplesandstandards,
  2. Add100μLstandardorsampletoeachwell.Incubate2hoursat37 °C,
  3. Aspirateandadd100μLpreparedDetectionReagentA.Incubate1hourat37 °C,
  4. Aspirateandwash3times,
  5. Add100μLpreparedDetectionReagentB.Incubate30 minutesat37 °C,
  6. Aspirateandwash5times,
  7. Add100μLSubstrateSolution.Incubate10 minutesat37 °C,
  8. ReadRLUvalueimmediately.
CalculationofResults

Averagetheduplicatereadingsforeachstandard,control,andsamplesandsubtracttheaveragezerostandardrelativelightunit(RLU).Createastandardcurveonlog-loggraphpaper,withUCHL1concentrationonthey-axisandtheRLUvalueonthex-axis.Drawthebestfitstraightlinethroughthestandardpointsanditcanbedeterminedbyregressionanalysis.Usingsomeplotsoftware,suchascurveexpert1.30,isalsorecommended.Ifsampleshavebeendiluted,theconcentrationreadfromthestandardcurvemustbemultipliedbythedilutionfactor.
Inordertomakethecalculationeasier,weplottheRLUvalueofthestandard(X-axis)againsttheknownconcentrationofthestandard(Y-axis),althoughconcentrationisindeedtheindependentvariablewhileRLUvalueisthedependentvariable.Further,inthispart,inordertohelpthecustomerperformtheassaymorevisual,weprovidethecustomerwiththerawdata(notthelogofdata).However,plottinglogofthedatatoconstructthecurvewillberecommended.TheRLUvaluesofthestandardcurvemayvaryaccordingtotheconditionsofassayperformance(e.g.operator,pipettingtechnique,washingtechniqueortemperatureeffects).Thiscurveisprovidedfordemonstrationonly.Thecustomersshouldestablishtheirownstandardcurveforeachtestconducted.

AssayPrecision

Intra-assayPrecision(Precisionwithinanassay):3sampleswithlow,middleandhighlevelUbiquitinCarboxylTerminalHydrolaseL1(UCHL1)weretested20timesononeplate,respectively.
Inter-assayPrecision(Precisionbetweenassays):3sampleswithlow,middleandhighlevelUbiquitinCarboxylTerminalHydrolaseL1(UCHL1)weretestedon3differentplates,8replicatesineachplate.
CV(%)=SD/meanX100
Intra-Assay:CV<10%
Inter-Assay:CV<12%

RestrictionsForResearchUseonly
PrecautionofUseTheStopSolutionsuggestedforusewiththiskitisanacidsolution.Weareye,hand,face,andclothingprotectionwhenusingthismaterial.
HandlingAdvice

Thestabilityofkitisdeterminedbythelossrateofactivity.Thelossrateofthiskitislessthan5 %withintheexpirationdateunderappropriatestoragecondition.
Tominimizeextrainfluenceontheperformance,operationproceduresandlabconditions,especiallyroomtemperature,airhumidity,incubatortemperatureshouldbestrictlycontrolled.Itisalsostronglysuggestedthatthewholeassayisperformedbythesameoperatorfromthebeginningtotheend.

Storage4°C
StorageComment
  • Forunopenedkit:Allthereagentsshouldbekeptaccordingtothelabelsonvials.TheStandard,DetectionReagentA,DetectionReagentBandthe96-wellstripplateshouldbestoredat-20°Cuponreceiptwhiletheothersshouldbeat4°C.
  • Foropenedkit:Whenthekitisopened,theremainingreagentsstillneedtobestoredaccordingtotheabovestoragecondition.Besides,pleasereturntheunusedwellstothefoilpouchcontainingthedesiccantpack,andresealalongentireedgeofzip-seal.
    Note:Itishighlyrecommendedtousetheremainingreagentswithin1monthprovidedthisiswithintheexpirationdateofthekit.
  • ForELISAkit,1daystorageat37°Ccanbeconsideredas2monthsat4°C,whichmeans3daysat37°Cequaling6monthsat4°C.
ExpiryDate6months