简介：MicroRNAs(miRNAs)aresmall,non-codingsingle-strandedRNAsthatcanmodulatetargetgeneexpressionatposttranscriptionallevelandparticipateincellproliferation,differentiation,andapoptosis.Tcellshaveimportantfunctionsinacquiredimmuneresponse;miRNAsregulatethisimmuneresponsebytargetingthemRNAsofgenesinvolvedinTcelldevelopment,proliferation,differentiation,andfunction.Forinstance,miR-181familymembersfunctioninprogressionbytargetingBcl2andCD69,amongothers.MiR-17tomiR-92clustersfunctionbybindingtoCREB1,PTEN,andBim.ConsideringthatthesuppressionofTcell-mediatedimmuneresponsesagainsttumorcellsisinvolvedincancerprogression,weshouldinvestigatethemechanismbywhichmiRNAregulatesTcellstodevelopnewapproachesforcancertreatment.

简介：Objective:Toexploretheantitumormechanismsofbifidobacteriaadolescenceinvivo.Methods:Thecontentofextracellularsignalregulatedproteins(ERK)1/2,C-JunN-terminalkinase(JNK),p38,c-fosandc-juninnudemousetransplantedlargebowelcarcinomawasdetectedbyusinglaserconfocalmicroscopy.TheexpressionofNF-kBwasdeterminedbyimmunohistochemistry.Results:Afterthenudemousetransplantedtumorwastreatedwithbifidobacteria,theaveragefluorescentstrengthofERK1/2,JNK,c-fosandc-junwassignificantlylowerthanthatintumorcontrolgroup(P<0.01).Theaveragefluorescentstrengthofp38wasnotobviousdifferenceinthetwogroups(P>0.05).ThepositivecelldensityofNF-kBinlargebowelcarcinomatransplantationtumorsinBifidobacteriuminjectiongroupwasmarkedlylowerthanthatintumorgroup(P<0.01).Conclusion:bifidobacteriaadolescencecouldmarkedlydecreasetheactivityofERK1/2andJNK,theexpressionc-fosandc-jun,andtheactivityofNF-kB.

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简介：Objective:Tounderstandwhetherverapamil(VER)resistancedevelopmentinthemultidrug-resistantcelllineanditsmechanism.Methods:K562/ADM/VERcellsublineresistanttoverapamilwasestablishedthroughagradualincreaseofVERconcentrationinthemedia.MTTmethodwasusedtoassayresistancetoVER,crossresistancetodipyriamole(DPM),cyclosporinA(CsA)inthecells,andHPLCandspectrofluorometertodetectintracellularaccumulationofVERorADMrespectively,aswellasS-Pimmunocytochemicaltechniquefordetectionofgenesexpression.Results:Itwereobservedthat7.9-foldincreaseinVERresistance,significantlyreducedintracellularaccumulationofVERorADMandalsodevelopacrossresistancetoDPMandCsAinK562/ADM/VERcells,comparedwithitsparentcell,K562/ADM.High-levelofp-glycoprotein(pgp),middle-levelofp53,p16,waspresentintwocelllineswithoutexpressionofGSTPI,C-myc,C-myc,C-fosandC-erbB-2.Bc1-2proteinexpressionwasfoundonlyinK562/ADMcells.Conclusion:K562/ADMcellswerecapableofbeinginducedtodevelopresistancetoVER.

简介：客观：为了调查抵抗和颠倒的机制，在导致cisplatin的multidrug抵抗ligustrazine和cyclosporinA完成卵巢的癌症房间线3Ao/cDDP。方法：用每周期在30mgcisplatin从临床的化疗计算的相应剂量，我们建立了3Ao/cDDP，3Ao每次在10渭g/ml在常规间隔并且反复暴露了到cisplatin的高级集中24个小时。LRP，MRP，P-gp，GST蟺和TopoII的表情是与FCM检测的份量上。为药抵抗颠倒，没有cytotoxicity，cyclosporinA和ligustrazine在最大的剂量单身地或在联合被管理。抑制率被MTT试金决定。结果：3Ao/cDDP在4.5个月以后被建立，与抵抗因素1.6它类似于临床的抵抗度。MRP和P-gp的低表示层次在3Ao和3Ao/cDDP被发现(P>0.05)，并且在3Ao/cDDP的LRP和GST蟺表示层次比在3Ao的那些显著地高(P<0.005andP<0.05，分别地)，并且在3Ao/cDDP的TopoII显著地更低对3Ao(P<0.05)。cDDP的抑制率是20.807卤0.015%，加ligustrazine的cDDP27.421卤0.07%(P>0.05对cDDP)，加cyclosporinA的cDDP49.635卤0.021%(P<0.01对cDDP)，并且加ligustrazine和cyclosporinA的cDDP58.861卤0.014%(P<0.01对cDDP)。结论：3Ao/cDDP，由cisplatin导致了并且由为上皮的卵巢的癌症模仿临床的化疗的特征建立了，是为cisplatinresistanceinvitro的调查的一个理想的模型。在3Ao/cDDP的Cisplatin抵抗能被说明为由更高的LRP，GST蟺和更低的TopoII表示并且没与MRP或P-gp被联系。Ligustrazine没在A能颠倒的cisplatin抵抗，而是cyclosporin上有重要颠倒效果抵抗有效地。