中国医药工业杂志
中國醫藥工業雜誌
중국의약공업잡지
CHINESE JOURNAL OF PHARMACEUTICALS
2009年
12期
902-906
,共5页
刘艳%龚桂花%胡又佳%朱春宝%朱宝泉
劉豔%龔桂花%鬍又佳%硃春寶%硃寶泉
류염%공계화%호우가%주춘보%주보천
顶头孢霉%头孢菌素C%7-氨基头孢烷酸%头孢菌素C酰基转移酶
頂頭孢黴%頭孢菌素C%7-氨基頭孢烷痠%頭孢菌素C酰基轉移酶
정두포매%두포균소C%7-안기두포완산%두포균소C선기전이매
Acremonium chrysogenum%cephalosporin C:7-ACA%cephalosporin C acylase
以假单胞菌的头孢菌素C(CPC)酰基转移酶为基础,根据顶头孢霉密码子偏爱性及RNA二级结构预测分析,设计并合成了全长2349 bp的CPC酰基转移酶基因ecs,并将其在大肠杆菌中表达.结果证明,表达蛋白能将CPC转化为7-ACA.将ecs表达质粒转化CPC产生菌顶头他霉,通过PCR、Southern blotting以及Western blotting等方法验证,表明ecs基因已成功整合到顶头孢霉染色体上并得到表达,重组菌的发酵也显示部分CPC直接转化成了7-ACA.
以假單胞菌的頭孢菌素C(CPC)酰基轉移酶為基礎,根據頂頭孢黴密碼子偏愛性及RNA二級結構預測分析,設計併閤成瞭全長2349 bp的CPC酰基轉移酶基因ecs,併將其在大腸桿菌中錶達.結果證明,錶達蛋白能將CPC轉化為7-ACA.將ecs錶達質粒轉化CPC產生菌頂頭他黴,通過PCR、Southern blotting以及Western blotting等方法驗證,錶明ecs基因已成功整閤到頂頭孢黴染色體上併得到錶達,重組菌的髮酵也顯示部分CPC直接轉化成瞭7-ACA.
이가단포균적두포균소C(CPC)선기전이매위기출,근거정두포매밀마자편애성급RNA이급결구예측분석,설계병합성료전장2349 bp적CPC선기전이매기인ecs,병장기재대장간균중표체.결과증명,표체단백능장CPC전화위7-ACA.장ecs표체질립전화CPC산생균정두타매,통과PCR、Southern blotting이급Western blotting등방법험증,표명ecs기인이성공정합도정두포매염색체상병득도표체,중조균적발효야현시부분CPC직접전화성료7-ACA.
A 2 349 bp ecs gene was designed based on codon bias of Acremonium chrysogenum and analysis of RNA secondary structure prediction of cephalosporin C(CPC)acylase originated from Pseudomonas N176.The ecs was then synthesized and induced into E.coli BL21(DE3).The results showed that CPC could be converted to 7-ACA by purified recombinant ECS protein.A.chrysogenum expression plasmid containing ecs was transformed into this CPCproducing strain and the integration of heterologous genes was verified by PCR and Southern blotting.The expression of ECS in A.chrysogenum was verified by Western blotting.Fermentation of the transformats showed that a part of CPC had been converted to 7-ACA.
