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Hotline:400-820-3792Inhibitors?ScreeningLibraries?Proteinswww.MedChemETofacitinibcitrateCat.No.:HY-40354ACASNo.:540737-29-9Synonyms:Tasocitinibcitrate;CP-690550citrate分?式:C??H??N?O?分?量:504.49作?靶點(diǎn):JAK;Apoptosis;Bacterial;Fungal;InfluenzaVirus作?通路:Epigenetics;JAK/STATSignaling;ProteinTyrosineKinase/RTK;StemCell/Wnt;Apoptosis;Anti-infection儲(chǔ)存?式:4°C,sealedstorage,awayfrommoistureandlight*Insolvent:-80°C,6months;-20°C,1month(sealed
storage,awayfrommoistureandlight)溶解性數(shù)據(jù)體外實(shí)驗(yàn)DMSO:28.57mg/mL(56.63mM;Needultrasonic)H2O:3.33mg/mL(6.60mM;Needultrasonic)MassSolvent1mg5mg10mgConcentration制備儲(chǔ)備液1mM1.9822mL9.9110mL19.8220mL5mM0.3964mL1.9822mL3.9644mL10mM0.1982mL0.9911mL1.9822mL請(qǐng)根據(jù)產(chǎn)品在不同溶劑中的溶解度選擇合適的溶劑配制儲(chǔ)備液;?旦配成溶液,請(qǐng)分裝保存,避免反復(fù)凍融造成的產(chǎn)品失效。儲(chǔ)備液的保存?式和期限:-80°C,6months;-20°C,1month(sealedstorage,awayfrommoistureandlight)。-80°C儲(chǔ)存時(shí),請(qǐng)?jiān)?個(gè)?內(nèi)使?,-20°C儲(chǔ)存時(shí),請(qǐng)?jiān)?個(gè)?內(nèi)使?。體內(nèi)實(shí)驗(yàn)請(qǐng)根據(jù)您的實(shí)驗(yàn)動(dòng)物和給藥?式選擇適當(dāng)?shù)娜芙?案。以下溶解?案都請(qǐng)先按照InVitro?式配制澄的儲(chǔ)備液,再依次添加助溶劑:(為保證實(shí)驗(yàn)結(jié)果的可靠性,澄的儲(chǔ)備液可以根據(jù)儲(chǔ)存條件,適當(dāng)保存;體內(nèi)實(shí)驗(yàn)的?作液,建議您現(xiàn)?現(xiàn)配,當(dāng)天使?;以下溶劑前顯?的百分?指該溶劑在您配制終溶液中的體積占?;如在配制過(guò)程中出現(xiàn)沉淀、析出現(xiàn)象,可以通過(guò)加熱和/或超聲的?式助溶)1/4MasterofBioactiveMolecules—您?邊的抑制劑?師www.MedChemE1.請(qǐng)依序添加每種溶劑:10%DMSO>>40%PEG300>>5%Tween-80>>45%salineSolubility:≥2.5mg/mL(4.96mM);Clearsolution2.請(qǐng)依序添加每種溶劑:10%DMSO>>90%(20%SBE-β-CDinsaline)Solubility:≥2.5mg/mL(4.96mM);Clearsolution3.請(qǐng)依序添加每種溶劑:10%DMSO>>90%cornoilSolubility:≥2.5mg/mL(4.96mM);Clearsolution4.請(qǐng)依序添加每種溶劑:5%DMSO>>95%(20%SBE-β-CDinsaline)Solubility:≥1.43mg/mL(2.83mM);Clearsolution5.請(qǐng)依序添加每種溶劑:50%PEG300>>50%salineSolubility:2.5mg/mL(4.96mM);Clearsolution;NeedultrasonicBIOLOGICALACTIVITY?物活性TofacitinibcitrateJAK3/2/1抑制劑,IC50分別為1,20和112nM。Tofacitinibcitrate具有抗,抗真菌和抗病毒活性。IC50&TargetJAK3JAK2JAK1Rock-II1nM(IC50)20nM(IC50)112nM(IC50)3400nM(IC50)Lck3870nM(IC50)體外研究Tofacitinib(CP-690550)citratebindspotentiallyatJAK3andJAK2as2.2nMand5nM(Kd).ThereportincludesadditionalbindingforTofacitinibatCamk1(Kdof5,000nM),DCamkL3(Kdof4.5nM),Mst2(Kdof4,300nM),Pkn1(Kdof200nM),Rps6ka2(Kin.Dom.2-C-terminal)(Kdof1,400nM),Rps6ka6(Kin.Dom.2-C-terminal)(Kdof1,200nM),Snark(Kdof420nM),Tnk1(Kdof640nM)andTyk2(Kdof620nM)[1].K562,KCL22,andTHP-1cellsareexposedtodifferentdosesofSTI571orJAKinhibitorsfor72htoquantifytheeffectsoftyrosinekinaseinhibitor(TKI)activity.CellgrowthinhibitionisthenevaluatedusingtheMTTassay.TheproliferationofK562andKCL22cells,butnotTHP-1cells,isinhibitedbyIMAinaconcentration-dependentmanner.TheIC50valueofIMAis0.28μMforK562and0.17μMforKCL22.AlthoughtreatmentwithTofacitinib(TOF)orINCB018424alonedoesnotsuppresscellproliferation,bothTofacitinibandINCB018424maketheK562andKCL22moresensitivetoIMA[4].體內(nèi)研究AnimalsthataretreatedwithTofacitinibshowasignificantlylowerproductionofanti-drugantibodies(ADAs)comparewithPEG-treatedcontrolmice(forfiveweeksafterinitialimmunization,p[2].Basedonpreviousdose-responsestudies,adailydoseofTofacitinibof6.2mg/kgisselectedtoprovide80%inhibitionofhindpawvolumeandplasmaexposurecapableofsuppressingtheJAK1andJAK3signalingpathwaysfor>4hours[3].PROTOCOLCellAssay[4]CellsurvivalassayisperformedusingMTT.Briefly,K562,KCL22,andTHP-1cells(1×105cells/well)are2/4MasterofBioactiveMolecules—您?邊的抑制劑?師www.MedChemEplatedonto96-wellmicroplatesandtreatedwithorwithoutIMA(0.06-1.0μM)and/orTofacitinib(10-1,000nM)orRUX(10-1,000nM)for72hat37°Cinahumidified5%(v/v)CO2atmosphere.Themedium(200μL)isthenincubatedwith10μLof5mg/mlMTTsolutionfor4hat37°C.Afterbeingcentrifugedat352gfor5min,theculturemediumisremoved,and100μLofDMSOareaddedtoeachwelltodissolvetheformazan.Absorbanceismeasuredat570nmusingamicroplatereader.Theresultsareexpressedaspercentages[4].MCEhasnotindependentlyconfirmedtheaccuracyofthesemethods.Theyareforreferenceonly.AnimalMice[2]Administration[2][3]FemaleBALB/cmice(6-8weeksold)areused.MicereceiveTofacitinibinPEG300(100mg/mL)orvehiclealone(PEG300)byosmoticpumpinfusion(0.25μL/hour,28days).Fourdayspriortoimmunization,miceareanesthetizedandtheirdorsalsurfaceisshaved.Aonecmincisionismadeonthebacktocreateasubcutaneouspocketandinsertthepump.Theincisionsiteisclosedwithwoundclips.Miceareinjectedweekly(i.p.)withSS1Precombinantimmunotoxin(RIT;5μg/mouse)beginningonday0;controlmicereceivedinjectionsofsalinealone.EveryweekbeforeSS1Porvehicleimmunization,50μLofbloodisdrawntoobtainserumsamples.Seraarestoredat-80°Cuntilanalyzed.Rats[3]Adjuvant-inducedarthritis(AIA)isinducedinfemaleLewisrats.RatsarerandomizedaccordingtohindpawvolumeandassignedtoTofacitiniborvehicletreatmentregimens.Groupsof7-8ratspertreatmentgroup,andnormalnaiverats(n=4pergroup),areeuthanizedeither4hours,4days,or7daysafterbeginningtreatment(days16,20,and23afterimmunization,respectively).Once-dailyoraladministrationofvehicleorTofacitinib(6.2mg/kg)isinitiatedonday16followingimmunizationandcontinuedthroughday23.Pawvolumesarereassessed4and7daysafterthebeginningoftreatment(days20and23afterimmunization,respectively).Formicro-computedtomography(micro-CT)imaging,aswellastartrate-resistantacidphosphatase(TRAP)staininginpawtissue,AIAisinducedinaseparatecohortofLewisrats.
MCEhasnotindependentlyconfirmedtheaccuracyofthesemethods.Theyareforreferenceonly.戶使?本產(chǎn)品發(fā)表的科研?獻(xiàn)?AnnRheumDis.2021Sep;80(9):1201-1208.?SciTranslMed.2018Jul18;10(450).pii:eaaq1093.?BMCMed.2021Oct15;19(1):247.?CellSyst.2018Apr25;6(4):424-443.e7.?CellRep.2020Sep15;32(11):108158.Seemorecustomervalidationsonwww.MedChemEREFERENCES[1].JiangJK,etal.Examiningthechirality,conformationandselectivekinaseinhibitionof3-((3R,4R)-4-methyl-3-(methyl(7H-pyrrolo[2,3-d]pyrimidin-4-yl)amino)piperidin-1-yl)-3-oxopropanenitrile(CP-690,550).JMedChem.2008Dec25;51(24):8012-8.[2].OndaM,etal.Tofacitinibsuppressesantibodyr
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