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uvsX、uvsY和DNA拓扑异构酶对噬菌体T4中rII基因串联重复形成的影响。

Effects of uvsX, uvsY and DNA topoisomerase on the formation of tandem duplications of the rII gene in bacteriophage T4.

作者信息

Kumagai M, Yamashita T, Honda M, Ikeda H

机构信息

Department of Molecular Biology, University of Tokyo, Japan.

出版信息

Genetics. 1993 Oct;135(2):255-64. doi: 10.1093/genetics/135.2.255.

Abstract

We have characterized tandem duplications in the rII regions of phage T4. The rII deletion r1589 blocks only the function of the rIIA cistron, although it extends into the B cistron. Another rII deletion, r1236, blocks the function of the rIIB cistron and overlaps r1589. When a cross is made between r1589 and r1236, true rII+ progeny cannot form. Instead, anomalous phenotypically rII+ phages are detected carrying an rII region from each parent. Analyses of nucleotide sequences of the recombination junctions indicate that recombination takes place between short regions of homology (from 2 to 10 bp). Open reading frames of the recombinants deduced from the nucleotide sequences reveal that they contain a normal rIIA cistron and one of a variety of fused, duplicated rIIB cistrons. The T4 uvsX and uvsY genes, which participate in homologous recombination, are involved in this duplication formation. T4 DNA topoisomerase is encoded by genes 39, 52 and 60. Mutations in 52 and 60 reduced the frequency of such duplications, but mutations in gene 39 and some in gene 52 did not. Hence, the effects of topoisomerase mutations are allele-specific. Models are proposed in which these proteins are involved in tandem duplication.

摘要

我们已对噬菌体T4的rII区域中的串联重复进行了表征。rII缺失r1589仅阻断rIIA顺反子的功能,尽管它延伸到了B顺反子中。另一个rII缺失r1236阻断rIIB顺反子的功能并与r1589重叠。当r1589和r1236之间进行杂交时,真正的rII+子代无法形成。相反,检测到表型异常的rII+噬菌体携带来自每个亲本的一个rII区域。对重组连接点的核苷酸序列分析表明,重组发生在短的同源区域(2至10个碱基对)之间。从核苷酸序列推导的重组体的开放阅读框显示,它们包含一个正常的rIIA顺反子和多种融合、重复的rIIB顺反子中的一种。参与同源重组的T4 uvsX和uvsY基因与这种重复的形成有关。T4 DNA拓扑异构酶由基因39、52和60编码。52和60中的突变降低了这种重复的频率,但基因39中的突变和52中的一些突变则没有。因此,拓扑异构酶突变的影响是等位基因特异性的。提出了这些蛋白质参与串联重复的模型。

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本文引用的文献

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Modulation of mutation rates in bacteriophage T4 by a base-pair change a dozen nucleotides removed.
J Mol Biol. 1984 Jun 25;176(2):239-49. doi: 10.1016/0022-2836(84)90422-4.
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In vitro study of illegitimate recombination: involvement of DNA gyrase.非法重组的体外研究:DNA 回旋酶的作用
Cold Spring Harb Symp Quant Biol. 1981;45 Pt 1:399-408. doi: 10.1101/sqb.1981.045.01.054.
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The structure of rII diploids of phage T4.噬菌体T4的rII二倍体结构。
Mol Gen Genet. 1972;116(3):223-38. doi: 10.1007/BF00269767.

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