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一系列允许对重组体进行直接筛选的广宿主范围低拷贝数载体。

A series of wide-host-range low-copy-number vectors that allow direct screening for recombinants.

作者信息

Morales V M, Bäckman A, Bagdasarian M

机构信息

Unit for Applied Cell and Molecular Biology, Umeå University, Sweden.

出版信息

Gene. 1991 Jan 2;97(1):39-47. doi: 10.1016/0378-1119(91)90007-x.

DOI:10.1016/0378-1119(91)90007-x
PMID:1847347
Abstract

A series of controlled expression vectors was constructed based on the wide-host-range plasmid pMMB66EH. Some of these new vectors code for the alpha-peptide of beta-galactosidase and allow the direct screening of recombinant clones by inactivation of alpha-complementation. The bla gene was replaced in some plasmids by the cat gene of Tn9 coding for chloramphenicol resistance, extending the use into beta-lactam-resistant strains. They all feature either the tac or taclac (tac-lac UV5 in tandem) promoters in front of a polylinker followed by the rrnB transcriptional stop point. These vectors were tested by subcloning the xylE gene coding for the Pseudomonas putida catechol 2,3-oxygenase and the Escherichia coli lamB gene coding for the lambda receptor. The expression of these genes in E. coli indicated that the tac promoter is five times stronger than the taclac promoter and that both were tightly regulated. The tac promoter in Pseudomonas syringae pv glycinea and Xanthomonas campestris pv vesicatoria had a strength similar to that in E. coli, while the taclac promoter was much weaker, reaching only 6.5 and 3% of the level of expression of the tac promoter, respectively. The taclac promoter, however, proved to be useful for the cloning in E. coli of DNA fragments that were unstable in vectors with stronger promoters and higher copy number. Expression of the lamB gene in Vibrio cholerae strain TRH7000 was not sufficient to permit cosmid transduction. Two subunits of the E. coli mannose permease, coded by the ptsP and ptsM genes, are also required for cosmid DNA penetration into the recipient cells.

摘要

基于广宿主范围质粒pMMB66EH构建了一系列可控表达载体。其中一些新载体编码β-半乳糖苷酶的α-肽,并允许通过α-互补失活直接筛选重组克隆。在一些质粒中,bla基因被编码氯霉素抗性的Tn9的cat基因取代,从而将其应用扩展到β-内酰胺抗性菌株。它们都在多克隆位点前具有tac或taclac(串联的tac-lac UV5)启动子,随后是rrnB转录终止点。通过亚克隆编码恶臭假单胞菌儿茶酚2,3-加氧酶的xylE基因和编码λ受体的大肠杆菌lamB基因对这些载体进行了测试。这些基因在大肠杆菌中的表达表明,tac启动子比taclac启动子强五倍,并且两者都受到严格调控。丁香假单胞菌大豆致病变种和野油菜黄单胞菌辣椒斑点病菌中的tac启动子强度与大肠杆菌中的相似,而taclac启动子则弱得多,分别仅达到tac启动子表达水平的6.5%和3%。然而,事实证明,taclac启动子对于在大肠杆菌中克隆在具有更强启动子和更高拷贝数的载体中不稳定的DNA片段很有用。霍乱弧菌TRH7000菌株中lamB基因的表达不足以允许黏粒转导。黏粒DNA渗透到受体细胞中还需要由ptsP和ptsM基因编码的大肠杆菌甘露糖通透酶的两个亚基。

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