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《抗Ⅰ型鴨肝炎病毒RdRp蛋白噬菌體單鏈抗體庫(kù)構(gòu)建及單鏈抗體的淘選.pdf》由會(huì)員上傳分享�,免費(fèi)在線閱讀,更多相關(guān)內(nèi)容在行業(yè)資料-天天文庫(kù)�����。
1、第37卷第5期中國(guó)預(yù)防獸醫(yī)學(xué)報(bào)VO1.37.No.52015年5月ChineseJournalofPreventiveVeterinaryMedicineMay.2015doi:10.3969~.issn.1008-0589.2015.05.03抗I型鴨肝炎病毒RdRp蛋白噬茵體單鏈抗體庫(kù)構(gòu)建及單鏈抗體的淘選王永娟�,一,李碧春����,沈明君,洪偉鳴���,左偉勇’(1.揚(yáng)州大學(xué)動(dòng)物科學(xué)與技術(shù)學(xué)院���,江蘇揚(yáng)州225009;2.江蘇農(nóng)牧科技職業(yè)學(xué)院江蘇省獸用生物制藥高技術(shù)研究重點(diǎn)實(shí)驗(yàn)室���,江蘇泰州225300)摘要:為構(gòu)建抗1型鴨肝炎病毒(DH
2�����、V.1)RdRp蛋白的單鏈抗體(scFv)庫(kù)���,并淘選特異性scFv,本研究采用RT.PCR方法從DHV.1基因組中擴(kuò)增RdRp基因,將其克隆于pET.32a載體中進(jìn)行重組RdRp蛋白原核表達(dá)�。將純化的重組蛋白免疫小鼠,以提取的免疫鼠脾臟總RNA為模板���,利用抗體輕鏈可變區(qū)(VL)和重鏈可變區(qū)(VH)簡(jiǎn)并引物���,經(jīng)RT.PCR擴(kuò)增抗體的VL和VH編碼序列,由Linker序列連接�,通過(guò)重疊延伸PCR(SOE.PCR1擴(kuò)增完整的scFv基因(VI_-Linker-V.)。將擴(kuò)增的seFv基因克隆于pCANTAB5E載體中構(gòu)建噬菌體sc
3�、Fv文庫(kù),利用純化的重組RdRp蛋白開(kāi)展4輪吸附.洗脫.富集以淘選抗RdRp的ScFv���;最后對(duì)淘選到的陽(yáng)性ScFv進(jìn)行可溶性表達(dá)����,以ELISA方法檢測(cè)其免疫結(jié)合活性��。結(jié)果顯示�����,獲得了7株具有良好抗原結(jié)合活性的ScFv���。淘選到的DHV.1RdRp特異的基因工程ScFv�����,為鴨病毒性肝炎防制新策略研究奠定了基礎(chǔ)��。關(guān)鍵詞:1型鴨肝炎病毒�����;RdRp���;噬菌體抗體庫(kù);單鏈抗體中圖分類號(hào):$852.65文獻(xiàn)標(biāo)識(shí)碼:A文章編號(hào):1008.0589(2015)05.0334.05ConstructionoOftphagesingle.一chai
4�����、nantibody(scFl-v)1IibraryforRdRPproteinofduckhepatitisvirustype1andthespecificscFvpanningwANGYong-juan��,一����,LIBi-chun,SHENMing-jun��,HONGWei—ming2,ZUOWei—yonf(1CollegeofAnimalScienceandTechnology���,YangzhouUniversity����,Yangzhou225009����,China;2.JiangsuProvincialKeyLaboratoryof
5�、VeterinaryBio-pharmaceuticalHighTechResearch,JiangsuAgri—animalHusbandryVocationalCollege����,Taizhou225300,China)Abstract:Toconstructphagedisplaymurinesingle—chainantibodyvariablefragment(scFv)libraryforRdRpproteinofduckhepatitisvirustype1(DHV一1)andscreenthespecificsc
6�����、FvagainstRdRp�����,theRdRpgenewasamplifiedfromthegenomicRNAofDHV-1byRT—PCRmethodandclonedintopET一32avectorforexpressioninE.coil.Then����,micewereimmunizedwiththeexpressedrecombinantRdRp���,andtotalRNAwasextractedfromthespleenofimmunizedmicetoamplifythevariableregionsencodingse
7�����、quencesoftheheavy(VH)andlightchains(V0withdegenerateprimersbyRT—PCR.Inaddition�,thecompletesequenceofscFvwasamplifiedwithalinkersequencebySOE—PCR.Furthermore,scFvsequenceswereclonedintopCANTAB5EvectortoconstructthescFvphagedisplaylibrary.Eventually�,usingpurifiedreco
8、mbinantproteinRdRpaspanningantigen��,sevenScFvswiththebindingafinitytoRdRpwereidentifiedafter4roundsofprocedurebinding-elution—enrichmentbyELISA.In
