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转座子Tn5插入的特异性

Specificity of transposon Tn5 insertion.

作者信息

Berg D E, Schmandt M A, Lowe J B

出版信息

Genetics. 1983 Dec;105(4):813-28. doi: 10.1093/genetics/105.4.813.

Abstract

Genetic mapping studies had shown that the bacterial transposon Tn5 can insert into many sites in a gene, but that some sites are preferred. To begin understanding Tn5's insertion specificity at the molecular level, we selected transpositions of Tn5 from the Escherichia coli chromosome to the plasmid pBR322 and analyzed the resultant pBR322::Tn5 plasmids by restriction endonuclease digestion and DNA sequencing. Seventy-five insertions in the tet gene were found at 28 sites including one major hotspot (with 21 insertions) and four lesser hotspots (with four to ten insertions each). All five hotspots are within the first 300 of the 1250-base pair (bp) tet gene. In contrast, 31 independent insertions in the amp gene were found in at least 27 distinct sites.--Tn5 generates 9 bp target sequence duplications when it transposes. Such transposon-induced duplications are generally taken to indicate that cleavages of complementary target DNA strands are made 9 bp apart during transposition. DNA sequence analysis indicated that GC base pairs occupy positions 1 and 9 in the duplications at each of the five hotspots examined, suggesting a GC-cutting preference during Tn5 transposition.

摘要

遗传图谱研究表明,细菌转座子Tn5可插入基因中的多个位点,但有些位点更受青睐。为了从分子水平开始了解Tn5的插入特异性,我们选择了从大肠杆菌染色体到质粒pBR322的Tn5转座,并通过限制性内切酶消化和DNA测序分析了所得的pBR322::Tn5质粒。在tet基因中发现了75个插入位点,分布在28个位置,包括一个主要热点(有21个插入)和四个次要热点(每个有4到10个插入)。所有五个热点都在1250个碱基对(bp)的tet基因的前300个碱基对范围内。相比之下,在amp基因中发现的31个独立插入至少分布在27个不同的位点。——Tn5转座时会产生9个碱基对的靶序列重复。这种转座子诱导的重复通常被认为表明在转座过程中互补靶DNA链的切割相隔9个碱基对。DNA序列分析表明,在所检查的五个热点中的每一个热点的重复序列中,GC碱基对占据第1位和第9位,这表明Tn5转座过程中有切割GC的偏好。

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