摘要
为了通过基因工程手段来增加苯丙氨酸的生物产量,利用PCR方法从大肠杆菌中克隆了抗反馈抑制突变型及野生型的pheA基因,进行了核苷酸序列分析,并利用高效的原核表达载体PBV220对pheA基因编码的突变型及野生型分支酸变位酶/预苯酸脱水酶(CM/PD)进行了表达。序列分析表明突变型基因碱基第580位由T变为C,相应氨基酸由Val变为Ala,SDS-PAGE图谱扫描分析表明目的蛋白CM/PD的表达量占全菌体蛋白的43%,占上清总蛋白的57%。酶活性测定表明其CM和 PD活性分别提高了 15.5和6.7倍,产酸量也有了一定的提高,为构建产苯丙氨酸的生物工程菌奠定了基础。
In order to improve the production of phenylalanine by bioengineering method, both the wild type and the feedback inhibition-resistant pheA gene were cloned. The result of DNA se- quencing indicated the T-580 in the wild type changed into C in the mutant, so the correspond amino acid changed from Val to Ala. The pheA gene of wild type and the feedback inhibition-re- sistant type encoding the double effect enzyme chorimate mutase/prephenate dehydratase (CM/ PD) were also high-level expressed in E. coli by PRPL promoter of pBV220. SDS-PAGE analysis indicated the yield of CM/PD is about 43% of total cellular proteins, and about 57% of total solvable protins. The specific activities of CM and PD were increased by 15. 5 and 6. 7 fold in strain harboring recombinant plasmid pBVpheA.
出处
《生物技术通讯》
CAS
1999年第4期250-253,共4页
Letters in Biotechnology
关键词
抗反馈抑制
分支酸变位酶/预苯酸脱水酶
基因表达
feedback inhibition-resistant
chorimate mutase/prephenate dehydratase
gene ex-pression
