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当前位置: 首页 > 产品中心 > Fluorescent_dyes > AAT Bioquest/Cell Navigator™ Lysosome Staining Kit *NIR Fluorescence*/22652/500 Tests
商品详细AAT Bioquest/Cell Navigator™ Lysosome Staining Kit *NIR Fluorescence*/22652/500 Tests
AAT Bioquest/Cell Navigator™ Lysosome Staining Kit *NIR Fluorescence*/22652/500 Tests
AAT Bioquest/Cell Navigator™ Lysosome Staining Kit *NIR Fluorescence*/22652/500 Tests
商品编号: 22652
品牌: aatbio
市场价: ¥56560.00
美元价: 33936.00
产地: 美国(厂家直采)
公司:
产品分类: 荧光染料
公司分类: Fluorescent_dyes
联系Q Q: 3392242852
电话号码: 4000-520-616
电子邮箱: info@ebiomall.com
商品介绍
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Ex/Em(nm)636/650
MWN/A
CAS#N/A
SolventN/A
StorageF/D/L
CategoryCellBIOLOGy
LabelingCells
RelatedFluorescenceImaging
BiochemicalAssays
Lysosomesarecellularorganelleswhichcontainacidhydrolaseenzymestobreakupwastematerialsandcellulardebris.Lysosomesdigestexcessorworn-outorganelles,foodparticles,andengulfedvirusesorbacteria.ThemembranearoundalysosomeallowsthedigestiveenzymestoworkatpH4.5.Theinteriorofthelysosomesisacidic(pH4.5-4.8)comparedtotheslightlyalkalinecytosol(pH7.2).ThelysosomemaintainsthispHdifferentialbypumpingprotonsfromthecytosolacrossthemembraneviaprotonpumpsandchlorideionchannels.OurCellNavigator™fluorescenceimagingkitsareasetoffluorescenceimagingtoolsforlabelingsub-cellularorganellessuchasmembranes,lysosomes,mitochondria,nuclei,etc.Theselectivelabelingoflivecellcompartmentsprovidesapowerfulmethodforstudyingcellulareventsinaspatialandtemporalcontext.ThisparticularkitisdesignedtolabellysosomesoflivecellsinNIRfluorescenceatEx/Em=636/650nm.LysoBrite™NIR,theproprietarylysotropicdyeusedinthekit,selectivelyaccumulatesinlysosomesprobablyviathelysosomepHgrADIent.Thelysotropicindicatorisahydrophobiccompoundthateasilypermeatesintactlivecells,andtrappedinlysosomesafteritgetsintocells.Itsfluorescenceissignificantlyenhanceduponenteringlysosomes.Thiskeyfeaturesignificantlyreducesitsstainingbackgroundandmakesitusefulforavarietyofstudies,includingcelladhesion,chemotaxis,multidrugresistance,cellviABIlity,apoptosisandcytotoxicity.Itissuitableforproliferatingandnon-proliferatingcells,andcanbeusedforbothsUSPensionandadherentcells.LysoBrite™dyessignificantlyoutperformtheequivalentLysoTracker™dyes(fromInvitrogen).LysoBrite™dyescanstayinlivecellsformorethanaweekwithveryminimalcelltoxicitywhiletheLysoTrackerdyescanonlybeusedforafewhours.LysoBrite™dyescansurviveafewgenerationsofcelldivision.Inaddition,LysoBrite™dyesaremuchmorephotostablethantheLysoTrackerdyes.
SpectrumAdvancedSpectrumViewer

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Thisprotocolonlyprovidesaguideline,andshouldbemodifiedaccordingtoyourspecificneeds.

1.PrepareLysosome-stainingsolution:

1.1   WarmLysoBrite™NIR(ComponentA)toroomtemperature.

1.2   Preparedyeworkingsolutionbydiluting20µLofLysoBrite™NIR(ComponentA)to10mLofLiveCellStainingBuffer(ComponentB).

Note1:20µLofLysoBrite™NIR(ComponentA)isenoughforone96-wellplate.AliquotandstoreunusedLysoBrite™NIR(ComponentA)at<-20oC.Protectitfromlightandavoidrepeatedfreeze-thawcycles.

Note2:Theoptimalconcentrationofthefluorescentlysosomeindicatorvariesdependingonthespecificapplication.Thestainingconditionsmaybemodifiedaccordingtotheparticularcelltypeandthepermeabilityofthecellsortissuestotheprobe.

2.Prepareandstaincells:

2.1   Foradherentcells:Growcellseitherina96-wellblackwall/clearbottomplate(100µL/well/96-wellplate)oroncover-slipsinsideapetridishfilledwiththeappropriateculturemedium.Whencellsreachthedesiredconfluence,addequalvolumeofthedye-workingsolution(fromStep1.2).Incubatethecellsina37°C,5%CO2incubatorfor30minutes.Washthecellstwicewithpre-warmed(37°C)Hanksand20mMHepesbuffer(HBSS)orbufferofyourchoice,fillthecellwellswithHBSSorgrowthmedium.ObservethecellsusingafluorescencemicroscopefittedwithaCy5filterset.

Note:Itisrecommendedtoincreaseeitherthelabelingconcentrationortheincubationtimetoallowthedyetoaccumulateifthecellsdonotappeartobesufficientlystained.

 

2.2   Forsuspensioncells:Addequalvolumeofdye-workingsolution(fromStep1.2)intothecells.Incubatethecellsina37°C,5%CO2incubatorfor30minutes.Washthecellstwicewithpre-warmed(37°C)Hanksand20mMHepesbuffer(HBSS)orbufferofyourchoice,fillthecellwellswithHBSSorgrowthmedium.ObservethecellsusingafluorescencemicroscopeequippedwithaCy5filterset.

Note1:Itisrecommendedtoincreaseeitherthelabelingconcentrationortheincubationtimetoallowthedyetoaccumulateifthecellsdonotappeartobesufficientlystained.

Note2:Suspensioncellsmaybeattachedtocover-slipsthathavebeentreatedwithBDCell-Tak®(BDBiosciences)andstainedasadherentcells(seeStep2.1).

References&Citations
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ATriple-FluorophoreLabeledNucleicAcidpHNanosensortoInvestigateNon-ViralGeneDelivery
Authors:DavidRWilson,DenisRoutkevitch,YuanRui,ArmanMosenia,KarlJWahlin,AlfredoQuinones-Hinojosa,DonaldJZack,JordanJGreen
Journal:MolecularTherapy(2017)

Silica-basednanoparticlesasbi-functionalandbi-modalimagingcontrastagents
Authors:SéverineLechevallier,RobertMauricot,HélèneGros-Dagnac,SylvianeChevreux,GillesLemercier,ErickPhonesouk,MurielGolzio,MarcVerelst
Journal:ChemPlusChem(2017)

Decidua-derivedmesenchymalstemcellsascarriersofmesoporoussilicananoparticles.Invitroandinvivoevaluationonmammarytumors
Authors:JuanLParis,PazdelaTorre,MiguelManzano,MVictoriaCabanas,AnaIFlores,MaríaVallet-Regí
Journal:ActaBiomaterialia(2016):275--282

Rhodamineboundmaghemiteasalong-termdualimagingnanoprobeofadiposetissue-derivedmesenchymalstromalcells
Authors:VratislavCmiel,JosefSkopalik,KaterinaPolakova,JanSolar,MarketaHavrdova,DavidMilde,IvanJustan,{cmiel2016rhodamineMagro
Journal:EuropeanBiophysicsJournal(2016):1--12

Endocytosedβ2-microglobulinamyloidfibrilsinducenecrosisandapoptosisofrabbitsynovialfibroblastsbydisruptingendosomal/lysosomalmembranes:anovelmechanismonthecytotoxicityofamyloidfibrils
Authors:TadakazuOkoshi,ItaruYamaguchi,DaisakuOzawa,KazuhiroHasegawa,HironobuNaiki
Journal:PloSone(2015):e0139330

FluorescenceImagingofsiRNADeliverybyPeptideNucleicAcid-basedProbe
Authors:TakayaSato,YusukeSato,KentaIwai,ShusukeKuge,NorioTeramae,SeiichiNishizawa
Journal:AnalyticalSciences(2015):315--320

Theconsiderationofindolicidinmodificationtobalanceitshemocompatibilityanddeliveryefficiency
Authors:Ching-WeiTsai,Wei-WenHu,Chih-ILiu,Ruoh-ChyuRuaan,Bing-ChangTsai,Shiow-LianCatherineJin,YungChang,Wen-YihChen
Journal:Internationaljournalofpharmaceutics(2015):498--505

AmonitoringmethodforAtg4activationinlivingcellsusingpeptide-conjugatedpolymericnanoparticles
Authors:Kyung-miChoi,HaeYunNam,JinHeeNa,SeongWhoKim,SangYoonKim,KwangmeyungKim,IckChanKwon,HyungJunAhn
Journal:Autophagy(2011):1052--1062


品牌介绍
美国AAT Bioquest Inc.(前身是ABD Bioquest,Inc.)是一家为从事生命科学研究、诊断研发及药物开发的科学家研发、生产和销售生物分析研究试剂和试剂盒的公司。公司致力于光谱学检测领域,包括吸收(颜色)、荧光和发光技术。AAT Bioquest的产品帮助全世界的科学家和生物医药研究者更好的了解生物化学、免疫学、细胞生物学和分子生物学等领域。AAT Bioquest会不断研发新产品,快速地丰富各个领域的产品。 1)提供反应探针和发光探针,生物素和端粒酶能够应用于标记药物小分子和生物聚合物,如蛋白、核酸以及其他碳水化合物; 2)研究并生产荧光和发光探针用于检测蛋白,核酸和活细胞; 3)不断推出新型的荧光和发光探针用于检测多种酶,特别是检测水解酶和氧化还原酶类; 4)致力于开发用于信号转导研究的试剂; 5)提供生理和神经探针,特别是钙离子指示剂和膜电位探针。
品牌分类
淋巴细胞信号传导 GPCR抗体 羰基活性生物素 细胞代谢 胺反应生物素 链霉亲和素结合物 生物素化抗IgGs 乙酰基特异性抗体 细胞骨架抗体
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