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灰色链霉菌链霉素磷酸转移酶:其基因在大肠杆菌中的表达以及与其他抗生素磷酸转移酶和真核蛋白激酶的序列同源性。

Streptomyces griseus streptomycin phosphotransferase: expression of its gene in Escherichia coli and sequence homology with other antibiotic phosphotransferases and with eukaryotic protein kinases.

作者信息

Lim C K, Smith M C, Petty J, Baumberg S, Wootton J C

机构信息

Department of Genetics, University of Leeds, UK.

出版信息

J Gen Microbiol. 1989 Dec;135(12):3289-302. doi: 10.1099/00221287-135-12-3289.

Abstract

The aphD gene of Streptomyces griseus, encoding a streptomycin 6-phosphotransferase (SPH), was sub-cloned in the pBR322-based expression vector pRK9 (which contains the Serratia marcescens trp promoter) with selection for expression of streptomycin resistance in Escherichia coli. Two hybrid plasmids, pCKL631 and pCKL711, were isolated which conferred resistance. Both contained a approximately 2 kbp fragment already suspected to include aphD. The properties of in vitro deletion derivatives of these plasmids were consistent with the presumed location of aphD. In vitro deletion of a sequence including most of the trp promoter largely, but not quite completely, abolished the ability of the plasmid to confer streptomycin resistance, confirming that expression was indeed principally from the trp promoter. A polypeptide of approximately 34.5 kDa was present in minicells containing plasmids that conferred streptomycin resistance, but was absent when the plasmids contained in vitro deletions removing streptomycin resistance. Part of the fragment was sequenced and an open reading frame corresponding to aphD identified. A computer-assisted comparison of the deduced SPH sequence with those of other antibiotic phosphotransferases suggested a common structure A-B-C-D-E, where B and D were conserved between all sequences compared while A, C and E divided between the streptomycin and hygromycin B phosphotransferases on one hand and kanamycin/neomycin ones on the other. A composite sequence data base was searched for homologues to consensus matrices constructed from five approximately 12-residue subsequences within blocks B and D. For one subsequence, corresponding to the N-terminal portion of block D, those sequences from the database that yielded the highest homology scores comprised almost entirely either antibiotic phosphotransferases or eukaryotic protein kinases. Possible evolutionary implications of this homology, previously described by other groups, are discussed.

摘要

灰色链霉菌的aphD基因编码链霉素6 - 磷酸转移酶(SPH),该基因被亚克隆到基于pBR322的表达载体pRK9(其含有粘质沙雷氏菌色氨酸启动子)中,用于在大肠杆菌中筛选链霉素抗性的表达。分离出了两个赋予抗性的杂交质粒pCKL631和pCKL711。两者都含有一个约2 kbp的片段,该片段已被怀疑包含aphD。这些质粒的体外缺失衍生物的特性与aphD的推测位置一致。体外缺失包括大部分色氨酸启动子的序列在很大程度上但并非完全消除了质粒赋予链霉素抗性的能力,证实表达确实主要来自色氨酸启动子。在含有赋予链霉素抗性的质粒的小细胞中存在一种约34.5 kDa的多肽,但当质粒含有去除链霉素抗性的体外缺失片段时该多肽不存在。对该片段的一部分进行了测序,并鉴定出了与aphD对应的开放阅读框。通过计算机辅助将推导的SPH序列与其他抗生素磷酸转移酶的序列进行比较,发现了一个共同的结构A - B - C - D - E,其中B和D在所有比较的序列中是保守的,而A、C和E一方面在链霉素和潮霉素B磷酸转移酶之间划分,另一方面在卡那霉素/新霉素磷酸转移酶之间划分。在一个复合序列数据库中搜索与由B和D区域内五个约12个残基的子序列构建的共有矩阵的同源物。对于一个对应于D区域N端部分的子序列,数据库中产生最高同源性得分的那些序列几乎完全由抗生素磷酸转移酶或真核蛋白激酶组成。讨论了先前其他研究小组描述的这种同源性可能的进化意义。

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