人肝再生增強(qiáng)因子基因的克隆、真核表達(dá)載體構(gòu)建及原核表達(dá).pdf

1、東北農(nóng)業(yè)大學(xué)碩士學(xué)位論文人肝再生增強(qiáng)因子基因的克隆、真核表達(dá)載體構(gòu)建及原核表達(dá)姓名：趙春麗申請(qǐng)學(xué)位級(jí)別：碩士專(zhuān)業(yè)：基礎(chǔ)獸醫(yī)學(xué)指導(dǎo)教師：郝艷紅李慶章2003.6.1東北農(nóng)業(yè)大學(xué)農(nóng)學(xué)碩士學(xué)位論文CloningConstructionofEucaryoteExpressionVectorandProcaryoticExpressionofHumanAugmenterofLiveRegenerationGeneAbstractHLLrflana

2、ugmenterofliverregeneration(hALRlisanovelcytokinewhichstimulatesspecificallyhepaticcellproliferationandisableto“：scueacutelivel“failurecausedbyhepatotoxinforexamplecarbonteWaehlorideand刪actosanamineeta1Theobjectofthisstu

3、dyishAL凡focusonitsmolecularcloningconstructionofeucaryoteexpressionvectorandprocaryotieexpressionTheexperimentextractedtotalRNAfi10m6monthoIdfetalliverandamplifiedhALRgenefragmentbytwinstepsRTPCRtechniqueTargetgonewllscl

4、onedintotheprocaryoficfusionexpressionvectorPET28a()thensubclonedintotheeucaryoteexpressionvectorpcDNA31()aftersequenceanalysisProcaryoticexpressionvectorrecombinantwas恤tnsfolTnedintocompetentBL21inducedandexpressedbyIPT

5、GrevulsantexploredthebestinducingtimeandthebesteoneenlrationofrevulsantExpressedproteinw∞analyzedtodeterminequalityandquamiIybyWesternblotandScionImage402Betasof‰treThiSexperimentclonedsoecess削ly431bphALRgermfragmentAfte

6、rsequencingandcomparingwithGenebankitw豳theclonedgenehad3basedifference(36th、177th、312th)mhomologyofnueleotideacidsequencebetweenclonedhALRgeneandpublishedonew∞994％n”constructionofeucmyoteexpressionvectorwasaccomplishedan

7、dtheprophasepreparationforeucacyoteexpressionofhALRgenewasmadeWesternblotanalysisprovedthatfusionproteinofmolecularweight187KDw勰薩in酣afterprocmyoficinducemantandexpressionIt吣discoveredfirstlythathALRalsod—essedalittlewhen

8、／twasnotinducedWhellulfimaconcentrationofE町Gwas10mmol／Landinducedfor3hourstheproteinexpressionquantitywasthemostCandidate：ZlmoChunliMajor：BasicvetennaryScienceSupervisor：ProfHaoYanhongProfLiQmghangKeywordshumanaugmentero