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[发光杆菌属Zm1菌株lux操纵子的克隆与表达:luxAB基因的核苷酸序列及荧光素酶的基本特性]

[Cloning and expression of the lux-operon of Photorhabdus luminescens, strain Zm1: nucleotide sequence of luxAB genes and basic properties of luciferase].

作者信息

Manukhov I V, Rastorguev S M, Eroshnikov G E, Zarubina A P, Zavil'gel'skiĭ G B

机构信息

State Research Institute of Genetics, Moscow, Russia.

出版信息

Genetika. 2000 Mar;36(3):322-30.

PMID:10779906
Abstract

A chromosomal fragment of bacteria Photorhabdus luminescence Zm1, which contains the lux operon, was cloned into the vector pUC18. The hybrid clone containing plasmid pXen7 with the EcoRI fragment approximately 7-kb was shown to manifest a high level of bioluminescence. By subcloning and restriction analysis of the EcoRI fragment, the location of luxCDABE genes relative to restriction sites was determined. The nucleotide sequence of the DNA fragment containing the luxA and luxB genes encoding alpha- and beta-subunits of luciferase was determined. A comparison with the nucleotide sequences of luxAB genes in Hm and Hw strains of Ph. luminescence revealed 94.5 and 89.7% homology, respectively. The enterobacterial repetitive intergenic sequence (ERIC) of 126 bp typical for Hw strains was identified in the spacer between the luxD and luxA genes. The lux operon of Zm1 is assumed to emerge through recombination between Hm and Hw strains. Luciferase of Ph. luminescence was shown to possess a high thermal stability: its activity decreased by a factor of 10 at 44 degrees C for 30 min, whereas luciferases of marine bacteria Vibrio fischeri and Vibrio harveyi were inactivated by one order of magnitude at 44 degrees C for 1 and 6 min, respectively. The lux genes of Ph. luminescence are suggested for use in gene engineering and biotechnology.

摘要

将含有lux操纵子的发光光杆状菌Zm1的染色体片段克隆到载体pUC18中。含有质粒pXen7和大约7kb EcoRI片段的杂交克隆显示出高水平的生物发光。通过对EcoRI片段进行亚克隆和限制性分析,确定了luxCDABE基因相对于限制性酶切位点的位置。测定了包含编码荧光素酶α亚基和β亚基的luxA和luxB基因的DNA片段的核苷酸序列。与发光光杆状菌Hm和Hw菌株中luxAB基因的核苷酸序列比较,分别显示出94.5%和89.7%的同源性。在luxD和luxA基因之间的间隔区鉴定出了Hw菌株典型的126bp肠杆菌重复基因间序列(ERIC)。推测Zm1的lux操纵子是通过Hm和Hw菌株之间的重组产生的。已证明发光光杆状菌的荧光素酶具有很高的热稳定性:在44℃下30分钟其活性降低10倍,而海洋细菌费氏弧菌和哈维氏弧菌的荧光素酶在44℃下分别1分钟和6分钟就失活一个数量级。发光光杆状菌的lux基因被建议用于基因工程和生物技术。

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[Cloning and expression of the lux-operon of Photorhabdus luminescens, strain Zm1: nucleotide sequence of luxAB genes and basic properties of luciferase].[发光杆菌属Zm1菌株lux操纵子的克隆与表达:luxAB基因的核苷酸序列及荧光素酶的基本特性]
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