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鼠伤寒沙门氏菌LT2中脂多糖合成的rfaLK区域的克隆、特性鉴定及DNA序列分析

Cloning, characterization, and DNA sequence of the rfaLK region for lipopolysaccharide synthesis in Salmonella typhimurium LT2.

作者信息

MacLachlan P R, Kadam S K, Sanderson K E

机构信息

Department of Biological Sciences, University of Calgary, Alberta, Canada.

出版信息

J Bacteriol. 1991 Nov;173(22):7151-63. doi: 10.1128/jb.173.22.7151-7163.1991.

Abstract

We have cloned and sequenced the rfaL and rfaK genes for lipopolysaccharide synthesis in Salmonella typhimurium LT2 on a 4.28-kb HindIII fragment from the previously described R' factor pKZ3 (S. K. Kadam, A. Rehemtulla, and K. E. Sanderson, J. Bacteriol. 161:277-284, 1985). rfaL is thought to encode a component of the O-antigen ligase, and rfaK is believed to encode the N-acetylglucosamine transferase. The genes were identified by the loss of complementation of prototype rfaL and rfaK mutations after Tn1000 mutagenesis. Translation of the nucleotide sequence predicted sizes of 45.9 and 43.1 kDa for the rfaL and rfaK gene products, respectively. Hydropathy analysis of the rfaL product suggested that it was an integral membrane protein. A third gene, rfaZ, was found to be an 808-bp open reading frame on the pyrE side of rfaK. Insertions into rfaZ reduced rfaK complementation, suggesting cotranscription in the pyrE-cysE direction. The rfaL gene is transcribed in the opposite direction in a separate operon which may also include rfaC. An incomplete open reading frame with homology to an Escherichia coli gene in the same region, rfaY, was found on the pyrE side of rfaZ. Complementation studies with Tn1000 insertions in rfaL showed that rfaL446 and rfaL447 are allelic. With the cloning of the rfaL and -K genes, the order of genes within the rfa cluster at 79 units on the linkage map was found to be cysE-rfaDFCLKZYJIBG-pyrE.

摘要

我们从先前描述的R'因子pKZ3(S.K.卡丹、A.雷赫姆图拉和K.E.桑德森,《细菌学杂志》161:277 - 284,1985年)的一个4.28 kb HindIII片段中克隆并测序了鼠伤寒沙门氏菌LT2中参与脂多糖合成的rfaL和rfaK基因。rfaL被认为编码O抗原连接酶的一个组分,rfaK据信编码N - 乙酰葡糖胺转移酶。通过Tn1000诱变后原型rfaL和rfaK突变互补性的丧失鉴定出了这些基因。核苷酸序列翻译预测rfaL和rfaK基因产物的大小分别为45.9 kDa和43.1 kDa。对rfaL产物的亲水性分析表明它是一种整合膜蛋白。发现第三个基因rfaZ是rfaK的pyrE侧一个808 bp的开放阅读框。插入rfaZ会降低rfaK的互补性,表明在pyrE - cysE方向上共转录。rfaL基因在一个单独的操纵子中以相反方向转录,该操纵子可能还包括rfaC。在rfaZ的pyrE侧发现了一个与同一区域大肠杆菌基因rfaY具有同源性的不完整开放阅读框。用rfaL中Tn1000插入进行的互补研究表明rfaL446和rfaL447是等位基因。随着rfaL和 - K基因的克隆,发现在连锁图上79单位处rfa簇内基因的顺序为cysE - rfaDFCLKZYJIBG - pyrE。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/af84/209221/f2a2823f3697/jbacter01040-0104-a.jpg

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