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一种允许在肺炎链球菌中对重组质粒进行阳性选择的质粒载体。

A plasmid vector allowing positive selection of recombinant plasmids in Streptococcus pneumoniae.

作者信息

Prats H, Martin B, Pognonec P, Burger A C, Claverys J P

出版信息

Gene. 1985;39(1):41-8. doi: 10.1016/0378-1119(85)90105-2.

Abstract

A new plasmid, pSP2, was constructed as a cloning vector for use in Streptococcus pneumoniae. It allows direct selection of recombinant plasmids, even for DNA fragments not homologous to the S. pneumoniae chromosome, as based on the failure to maintain long inverted repeats (LIRs) hyphen-free in bacterial plasmids. Plasmid pSP2 contains a 1.4-kb BamHI fragment ("hyphen") flanked by 1.9-kb LIRs. The removal of the 1.4-kb BamHI fragment followed by ligation creates a plasmid containing a 1.9-kb insert-free LIR; plasmids with such non-hyphenated LIRs were not established when transferred into S. pneumoniae. Replacement of the original 1.4-kb insert by other restriction fragments restored plasmid viability. Investigation of plasmid transfer by transformation suggests that intrastrand synapsis between the LIRs could occur, thus facilitating plasmid establishment (a process we call self-facilitation). Such an intrastrand synapsis could also account for rare occurrences of insert-inversion noticed upon transfer as well as for the formation of palindrome-deleted derivatives at low frequency. Plasmid pSP2 carries two selectable genes, tet and ermC, and can be used for cloning of fragments produced by a variety of restriction enzymes (BamHI, Bg/II, Bc/I or Sau3A, and Sa/I or XhoI).

摘要

构建了一种新的质粒pSP2,用作肺炎链球菌的克隆载体。它允许直接筛选重组质粒,即使是与肺炎链球菌染色体非同源的DNA片段,这是基于细菌质粒中无法维持无间隔的长反向重复序列(LIR)。质粒pSP2包含一个1.4 kb的BamHI片段(“间隔”),两侧是1.9 kb的LIR。去除1.4 kb的BamHI片段后进行连接,会产生一个含有1.9 kb无插入片段LIR的质粒;当转入肺炎链球菌时,具有这种无间隔LIR的质粒无法建立。用其他限制性片段替换原来的1.4 kb插入片段可恢复质粒的活力。通过转化对质粒转移的研究表明,LIR之间可能发生链内联会,从而促进质粒的建立(我们称之为自我促进过程)。这种链内联会也可以解释转移时罕见的插入片段倒位现象以及低频下形成的回文缺失衍生物。质粒pSP2携带两个选择基因tet和ermC,可用于克隆由多种限制性酶(BamHI、Bg/II、Bc/I或Sau3A,以及Sa/I或XhoI)产生的片段。

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