資源描述:
《外切-β-葡聚糖酶基因重組里氏木霉的篩選及其產(chǎn)酶性能-論文.pdf》由會員上傳分享�,免費在線閱讀,更多相關(guān)內(nèi)容在應(yīng)用文檔-天天文庫�����。
1��、第65卷第8期化工學(xué)報V_01.65No.82014年8月CIESCJournalAugust2014菱3≥03j����;:;3j)jjjj外切-p一葡聚糖酶基因重組里氏木霉的篩選及其產(chǎn)酶性能孔芹�,方浩,夏黎明(浙江大學(xué)生物質(zhì)化工教育部重點實驗室��,化學(xué)工程與生物工程學(xué)系���,浙江杭州310027)摘要:外切.D一葡聚糖酶是纖維素酶的重要組分之一����,提高該組分的活力是增強纖維素酶協(xié)同降解性能���、降低纖維素水解成本的關(guān)鍵��。分別采用微晶纖維素瓊脂平板法和濾紙崩解法�,對己有的基因重組轉(zhuǎn)化子進行篩選試驗��,獲得了6個優(yōu)良
2����、轉(zhuǎn)化子,其濾紙崩解速率和微晶纖維素瓊脂平板上的生長速率都較大�����。進一步在搖瓶條件下進行復(fù)篩試驗��,獲得了外切.p.葡聚糖酶(C1)高產(chǎn)轉(zhuǎn)化子TrichodermareeseiZU.101���,液體培養(yǎng)48h����,其C1酶活力可達18.24U·ml~,是出發(fā)菌株的2.16倍�����;分析結(jié)果表明:重組轉(zhuǎn)化子的纖維素酶體系中內(nèi)切.D.葡聚糖酶和纖維二糖酶的活力與出發(fā)菌株相比變化不大�����,但由于外切.D一葡聚糖酶活力得到了大幅度提高����,纖維素酶的總活力(濾紙酶活力FPA)也提高了61.9%。采用纖維素酶對堿預(yù)處理玉米秸稈進行酶
3���、解試驗�,當(dāng)酶用量為20FPIU·(g底物����,水解48h,重組轉(zhuǎn)化子T.reeseiZU.101纖維素酶的酶解得率高達94.4%�。本文的研究結(jié)果在可再生纖維素資源的生物轉(zhuǎn)化與利用方面具有廣闊的應(yīng)用前景。關(guān)鍵詞:重組里氏木霉���;外切.D.葡聚糖酶���;轉(zhuǎn)化子篩選;玉米秸稈��;酶水解DOI:10.3969~.issn.0438-1t57.2014.08.037中圖分類號:TQ920文獻標(biāo)志碼:A文章編號:0438—1157(2014)O8—3l22—06Screeningandcellulaseproducti
4�、onofrecombinantTrichodermareeseiwithhighactivityexo-p-glucanasesKONGQin,F(xiàn)ANGHao���,XIALiming(KeyLaboratoryofBiomassChemicalEngineeringofMinistryofEducation����,DepartmentofChemicalEngineeringandBioengineeringZhejiangUniversity����,Hangzhou310027,Zh~iang,China)A
5��、bstract:Increasingtheactivitiesofexo—p—glucanases����,oneoftheimportantcomponentsofcellulase,isakeytostrengtheningthesynergisticdegradationofcellulaseandreducingthecostofcellulolytichydrolysis.ThemethodsofMCC—agarplatescreeningandliquidculturemediumoffil
6�、terpaperwereusedinthisworkrespectivelytoscreenTrichodermareeseitransformants�,obtaining6superiortransformantswithhigherfilterpapercollapsingrateandgrowingrateonMCC-agarplates.Furtherscreeningexperimentwasconductedundershakingflaskcondition�,obtainingth
7、ehighlyexo一~-glucanase(co-producingtransformantreeseiZU一101whoseC1activitywasl8.24U·ml—after48hliquidculture.2.16一foldhigherthantheoriginalstrain.Analysisresultsdemonstratedthatfilterpaperactivity(FPA)ofthecellulasesystemofthetransformant.representin
8����、gtotalactivity,increasedby61.9%asexo—p—glucanaseactivityascendedsignificantly,althoughendo一13-glucanaseandcellobiaseactivitiesvariedinsignificantlyfromtheoriginalstrain.TheenzymatichydrolysisyieldofreeseiZU一101’Scellulaseinthehydrolysisofalkalipretre
