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《【2016年】無血清體外培養(yǎng)樹突狀細胞的研究【醫(yī)學(xué)論文】》由會員上傳分享���,免費在線閱讀��,更多相關(guān)內(nèi)容在學(xué)術(shù)論文-天天文庫。
1���、醫(yī)學(xué)論文-無血清體外培養(yǎng)樹突狀細胞的研究??????????????作者:張懷東���,宋振嵐,李偉平【摘要】?本研究的目的是建立對外周血來源的樹突狀細胞(dendriticcell,DC)的無血清培養(yǎng)方案。以含胎牛血清(FCS)����、人AB血清的培養(yǎng)液作為對照。分離健康志愿者外周血單個核細胞(PBMNC)�,在不同培養(yǎng)液中分別加入GM-CSF(100ng/ml)、IL-4(500U/ml)培養(yǎng)6天���,再分別加入鈣離子載體A23187(100ng/ml)繼續(xù)培養(yǎng)24小時����,于倒置顯微鏡下觀察細胞形態(tài)���,流式細胞術(shù)分析細胞表型,MTT比色法檢測各組DC刺激同種異體外周血
2���、T細胞增殖的能力和DC刺激的T細胞對K562細胞的殺傷作用����。結(jié)果表明:無血清培養(yǎng)組培養(yǎng)出典型形態(tài)的DC����,其表面CD14分子的表達明顯減少,CD83���、HLA-DR����、CDw123分子的表達明顯增高,具有明顯的刺激同種異體T細胞增殖的能力和DC刺激的T細胞對K562細胞的殺傷作用�����。無血清組與兩個含血清的對照組比較��,組間無顯著性差異(P>0.05)�����。結(jié)論:無血清培養(yǎng)液培養(yǎng)的DC與含血清的培養(yǎng)液培養(yǎng)的DC相比��,無顯著性差異��。DC無血清培養(yǎng)具有臨床應(yīng)用前景�����?���!娟P(guān)鍵詞】?樹突狀細胞;無血清培養(yǎng)液��;鈣離子載體�����;外周血 InVitro?CultivationofDe
3、ndriticCellswithSerum-freeMedium AbstractThisstudywasaimed?toinvestigatetheprotocol?invitro??toincubatethe?dendriticcell(DC)derivedfromperipheralbloodmonocytesusingserum-freemediumX-VIVO20.?Peripheralbloodmonocytesfromhealthydonorsweretreatedwith100ng/mlGM-CSFand500U/mlIL-4,r
4��、espectively.Aftercultivationfor6days,theyweretreatedwith100ng/mlcalciumionophoreA23187.Aftercultivationfor24hoursthecellularmorphologywasobservedunderinvertmicroscope,thesurfacemarkerswereanalyzedbyflowcytometry,??theproliferationofallogeneticTcells?wasdetectedbyMTTcolorimetry,
5���、?thespecificcytotoxicityofTcellsprimedwithDCwasexaminedbyMTTassay.Theresultsshowedthatinallthreegroupswithserum-free,fetalcalfserum(FCS)andhumanABserummediums,cellsdisplayedcharacteristicmorphologicalfeaturesofDC.Simultaneously??CD14expression?wasdecreased,?and?CD83,HLA-DRandCD
6、w123expressionwereincreased?onthesecells.Inaddition,DCsculturedwiththesemethodscouldevidentlystimulatetheproliferationofallogeneticTcell.Ascomparedwiththetwocontrolsofserumcontaininggroups,theculturedcellsintheserum-freegroupsshowedalmostthesameallo-stimulatorycapabilityandcell
7�、ularmorphologyandsurfacemarkers,andTlymphocytesprimedwiththeculture-derivedDCexhibitedthesimilarkillingactivitytoK562(P>0.05).ItisconcludedthatthereisnosignificanceinDCnumbers,morphology,?epitopeandabilitytostimulatetheproliferationofallogeneticTcellsbetweenDCinducedbyserum-fre
8、eX-VIVO20mediumandDCinducedbyserum-containedmedium.DC?
