生物加工过程
生物加工過程
생물가공과정
CHINESE JOURNAL OF BIOPROCESS ENGINEERING
2014年
4期
1-6
,共6页
枯草芽胞杆菌%发酵%脂肪酶%粘质沙雷氏菌
枯草芽胞桿菌%髮酵%脂肪酶%粘質沙雷氏菌
고초아포간균%발효%지방매%점질사뢰씨균
Bacillus subtilis%fermentation%lipase%Serratia marcescens
笔者所在实验室前期筛选到1株产脂肪酶粘质沙雷氏菌,克隆其脂肪酶基因,构建重组枯草芽胞杆菌Bacillus subtilis 168/pMA5 lipA,成功实现了来源于粘质沙雷氏菌的脂肪酶基因在枯草芽胞杆菌中的表达。基于以上工作基础上,对B?subtilis 168/pMA5 lipA进行了摇瓶水平上的产酶发酵优化。首先通过单因素和正交试验确定了有利于产脂肪酶的最佳培养基成分,并对发酵条件进行了优化。结果表明:优化后的培养基组分为蔗糖35 g/L,玉米浆27?5 g/L,( NH4)2 SO41?25 g/L,CaCl24 g/L,pH 7?0。在最优发酵培养基的条件下,37℃、160 r/min摇床培养33 h,每毫升发酵液中重组菌脂肪酶酶活可达98?6 U,是优化前的3倍。
筆者所在實驗室前期篩選到1株產脂肪酶粘質沙雷氏菌,剋隆其脂肪酶基因,構建重組枯草芽胞桿菌Bacillus subtilis 168/pMA5 lipA,成功實現瞭來源于粘質沙雷氏菌的脂肪酶基因在枯草芽胞桿菌中的錶達。基于以上工作基礎上,對B?subtilis 168/pMA5 lipA進行瞭搖瓶水平上的產酶髮酵優化。首先通過單因素和正交試驗確定瞭有利于產脂肪酶的最佳培養基成分,併對髮酵條件進行瞭優化。結果錶明:優化後的培養基組分為蔗糖35 g/L,玉米漿27?5 g/L,( NH4)2 SO41?25 g/L,CaCl24 g/L,pH 7?0。在最優髮酵培養基的條件下,37℃、160 r/min搖床培養33 h,每毫升髮酵液中重組菌脂肪酶酶活可達98?6 U,是優化前的3倍。
필자소재실험실전기사선도1주산지방매점질사뢰씨균,극륭기지방매기인,구건중조고초아포간균Bacillus subtilis 168/pMA5 lipA,성공실현료래원우점질사뢰씨균적지방매기인재고초아포간균중적표체。기우이상공작기출상,대B?subtilis 168/pMA5 lipA진행료요병수평상적산매발효우화。수선통과단인소화정교시험학정료유리우산지방매적최가배양기성분,병대발효조건진행료우화。결과표명:우화후적배양기조분위자당35 g/L,옥미장27?5 g/L,( NH4)2 SO41?25 g/L,CaCl24 g/L,pH 7?0。재최우발효배양기적조건하,37℃、160 r/min요상배양33 h,매호승발효액중중조균지방매매활가체98?6 U,시우화전적3배。
A lipase-production Serratia marcescens was screened and its lipase coding gene was cloned to construct the recombinant Bacillus subtilis 168/pMA5-lipA.Lipase from Serratia marcescens was expressed in B.subtilis for the first time.In this study,fermentation optimization of B.subtilis 168/pMA5-lipA was carried out at the shake flask level.Medium compositions were optimized using single factor and orthogonal experiment.Furthermore, the optimization of culture conditions was performed.The optimal fermentation medium was as follows:sucrose 35 g/L,corn syrup 27.5 g/L,( NH4 ) 2 SO4 1.25 g/L,CaCl2 4 g/L, and pH 7.0.The lipase yield reached 98.6 U/mL in the optimal fermentation medium and culture conditions,it was 3 times before the optimization.
