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以反向排列携带两个Tn3衍生物拷贝的共整合体。

Cointegrates carrying two copies of a Tn3 derivative in an inverted orientation.

作者信息

McCormick M, Ohtsubo E

出版信息

Gene. 1985;34(2-3):197-206. doi: 10.1016/0378-1119(85)90128-3.

Abstract

We constructed a mutant of Tn3, Tn3 #2, that contains a 55-bp direct repeat of sequences near the amino-terminal coding region of the transposase, and an 8-bp EcoRI linker. This mutant transposase is functional. The plasmid carrying Tn3 #2, pMB8::Tn3 #2, recombines with the plasmid pHS1 at a frequency of 2.8 X 10(-7) recombinants per division cycle. This is similar to the recombination frequency of pHS1 and pMB8::Tn3+ (wild-type) which is 4.5 X 10(-6) recombinants per division cycle. One-third of the recombinants between pMB8::Tn3 #2 and pHS1 were approx. 22 kb in length. Restriction analysis and nucleotide sequencing showed that these large plasmids were Tn3 #2-mediated cointegrates formed by integration of pMB8::Tn3 #2 into pHS1. However, unlike Tn3 tnpR- -mediated cointegrates that contain direct repeats of the incoming element, Tn3 #2-mediated cointegrates carry two copies of Tn3 #2 in the form of inverted repeats. Like the tnpR- repeats, the Tn3 #2 repeats occur at both junctions between the parental plasmids, and are associated with a 5-bp direct duplication of the pHS1 target site. Furthermore, these recombinants contain a small deletion starting precisely at the end of Tn3 #2 and extending into pMB8 sequences. We propose a model for the generation of Tn3 #2-mediated cointegrates.

摘要

我们构建了Tn3的一个突变体Tn3 #2,它包含转座酶氨基末端编码区附近55个碱基对的序列直接重复,以及一个8个碱基对的EcoRI接头。这个突变体转座酶具有功能。携带Tn3 #2的质粒pMB8::Tn3 #2与质粒pHS1以每个分裂周期2.8×10⁻⁷个重组体的频率重组。这与pHS1和pMB8::Tn3⁺(野生型)的重组频率相似,后者是每个分裂周期4.5×10⁻⁶个重组体。pMB8::Tn3 #2和pHS1之间三分之一的重组体长度约为22 kb。限制性分析和核苷酸测序表明,这些大质粒是由pMB8::Tn3 #2整合到pHS1中形成的Tn3 #2介导的共合体。然而,与包含导入元件直接重复的Tn3 tnpR⁻⁻介导的共合体不同,Tn3 #2介导的共合体以反向重复的形式携带两个Tn3 #2拷贝。与tnpR⁻重复一样,Tn3 #2重复出现在亲本质粒之间的两个连接处,并与pHS1靶位点的5个碱基对直接重复相关。此外,这些重组体包含一个小缺失,精确地从Tn3 #2的末端开始并延伸到pMB8序列中。我们提出了一个关于Tn3 #2介导的共合体产生的模型。

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