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5.2.2—5.2.2—••••1)FunctionalactivityoftherecombinantproteinTheBEVStypicallyproducesoverexpressedrecombinantproteinscontainingproperfolding,disulfidebondformationandoligomerization.Additionally,thissystemiscapableofperformingseveralpost-translationalmodifications.Thisleadstoaproteinthatissimilartoitsnativecounterpart,bothstructurallyandfunctionally.However,incaseswheretheauthenticproteinfunctionsasaheterodimerorreliesontissue-orspecies-specificmodifications,therecombinantBaculovirus-expressedproteinmaynotbefunctionallyactive,unlessitsbindingpartnerormodifyingenzymeisco-expressed.2)Post-translationalmodifications2)Post-translationalmodificationsSeveralpost-translationalmodificationshavebeenreportedtooccurintheBEVS,includingN-andO-linkedglycosylation,phosphorylation,acylation,amidation,carboxymethylation,isoprenylation,signalpeptidecleavageandproteolyticcleavage.Thesiteswherethesemodificationsoccurareoftenidenticaltothoseoftheauthenticproteininitsnativecellularenvironment.Severalpost-translationalmodificationshavebeenreportedtooccurintheBEVS,includingN-andO-linkedglycosylation,phosphorylation,acylation,amidation,carboxymethylation,isoprenylation,signalpeptidecleavageandproteolyticcleavage.Thesiteswherethesemodificationsoccurareoftenidenticaltothoseoftheauthenticproteininitsnativecellularenvironment.3)Highexpressionlevels3)HighexpressionlevelsComparedtootherhighereukaryoticexpressionsystems,themostdistinguishingfeatureoftheBEVSisitspotentialtoachievehighlevelsofexpressionofaclonedgene.TheBEVSsystemhasprovenparticularlyusefulinthegenerationoflargequantitiesofproteinsforstructuralanalysis.Thehighestexpressionlevelreportedis50%ofthetotalcellularproteinofaninfectedinsectcellcorrespondingtoapproximately1gofrecombinantproteinper1109cells.However,manyrecombinantproteinsarenotproducedatsuchhighamountsanditisusuallydifficulttopredicttheamountofproteinexpression.Therearesomeguidelinesonecanfollowtooptimizeproteinproduction.OfprimaryimportanceisoptimizingthedesignoftherecombinantBaculovirusTransferVector.Comparedtootherhighereukaryoticexpressionsystems,themostdistinguishingfeatureoftheBEVSisitspotentialtoachievehighlevelsofexpressionofaclonedgene.TheBEVSsystemhasprovenparticularlyusefulinthegenerationoflargequantitiesofproteinsforstructuralanalysis.Thehighestexpressionlevelreportedis50%ofthetotalcellularproteinofaninfectedinsectcellcorrespondingtoapproximately1gofrecombinantproteinper1109cells.However,manyrecombinantproteinsarenotproducedatsuchhighamountsanditisusuallydifficulttopredicttheamountofproteinexpression.Therearesomeguidelinesonecanfollowtooptimizeproteinproduction.OfprimaryimportanceisoptimizingthedesignoftherecombinantBaculovirusTransferVector.4)Capacityforlargeinserts4)CapacityforlargeinsertsTheexpandabilityofthecapsidstructureofBaculovirusesallowsthepackagingandexpressionofverylargegenes.ThereisnoknownuppersizelimitfortheinsertionofforeignsequencesintotheBVgenome.TheexpandabilityofthecapsidstructureofBaculovirusesallowsthepackagingandexpressionofverylargegenes.ThereisnoknownuppersizelimitfortheinsertionofforeignsequencesintotheBVgenome.5)Capacitytoexpressunsplicedgenes5)CapacitytoexpressunsplicedgenesInsectcellshavethecapabilitytoperformintron/exonsplicing.However,certainvirus-,tissue-orspecies-specificsplicingpatternswillnotbeobtainediftheyrequirethepresenceofparticularsplicingfactorswhicharenotavailableintheinfectedinsectcellenvironment.Ingeneral,forhighproteinexpressionlevels,acDNAinsertratherthanagenomicDNAfragmentisrecommended.Insectcellshavethecapabilitytoperformintron/exonsplicing.However,certainvirus-,tissue-orspecies-specificsplicingpatternswillnotbeobtainediftheyrequirethepresenceofparticularsplicingfactorswhicharenotavailableintheinfectedinsectcellenvironment.Ingeneral,forhighproteinexpressionlevels,acDNAinsertratherthanagenomicDNAfragmentisrecommended.6)Simplicityoftechnology6)SimplicityoftechnologyThistechnologyhasmadeexpressionoffull-lengthproteinsfast,easyandreliable.RecombinantBaculoviruscanbeobtainedintwosimplesteps–cloningandco-transfection–inaslittleas5days.TheeaseofusenowrivalsthatofbacterialexpressionsystemsandBEVStechnologydoesnotrequirethattherecombinantproteinbeexpressedasafusionprotein.Thistechnologyhasmadeexpressionoffull-lengthproteinsfast,easyandreliable.RecombinantBaculoviruscanbeobtainedintwosimplesteps–cloningandco-transfection–inaslittleas5days.TheeaseofusenowrivalsthatofbacterialexpressionsystemsandBEVStechnologydoesnotrequirethattherecombinantproteinbeexpressedasafusionprotein.7)Simultaneousexpressionofmultiplegenes7)SimultaneousexpressionofmultiplegenesBEVShasthecapabilitytoexpresstwoormoregenessimultaneouslywithinsingleinfectedinsectcells.Proteincomplexesthatdependondimerormultidimerformationforactivitycanbeassembled.Awellknownexampleistheformationofcompleteviruscapsidsfromavarietyofviruseswhichhavebeenassembledinvitro,usingBEVS,bycoexpressingthecapsidsubunitssimultaneously.BEVShasthecapabilitytoexpresstwoormoregenessimultaneouslywithinsingleinfe
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李剑雄
本文标题:昆虫杆状病毒细胞表达系统-课件
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