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痢疾志贺菌1型中rfb基因簇和rfe基因在O抗原合成中的作用。

Function of the rfb gene cluster and the rfe gene in the synthesis of O antigen by Shigella dysenteriae 1.

作者信息

Klena J D, Schnaitman C A

机构信息

Department of Microbiology, Arizona State University, Tempe 85287.

出版信息

Mol Microbiol. 1993 Jul;9(2):393-402. doi: 10.1111/j.1365-2958.1993.tb01700.x.

Abstract

A plasmid that included both an 8.9 kb chromosomal DNA insert containing genes from the rfb cluster of Shigella dysenteriae 1 and a smaller insert containing the rfp gene from a S. dysenteriae 1 multicopy plasmid resulted in efficient expression of O antigen in an rfb-deleted strain of Escherichia coli K-12. Eight genes were identified in the rfb fragment: the rfbB-CAD cluster which encodes dTDP-rhamnose synthesis, rfbX which encodes a hydrophobic protein involved in assembly of the O antigen, rfc which encodes the O antigen polymerase, and two sugar transferase genes. The production of an O antigen also required the E. coli K-12 rfe gene, which is known to encode a transferase which adds N-acetylglucosamine phosphate to the carrier lipid undecaprenol phosphate. Thus Rfe protein appears to function as an analogue of the Salmonella RfbP protein to provide the first sugar of the O unit. Functional analysis of the other genes was facilitated by the fact that partial O units of one, two or three sugars were efficiently transferred to the lipopolysaccharide core. This analysis indicated that the plasmid-encoded Rfp protein is the transferase that adds the second sugar of the O unit while the two rfb transferases add the distal sugars to make an O antigen whose structure is (Rha-Rha-Gal-GlcNAc)n. The use of the rfe gene product as the transferase that adds the first sugar of an O unit is a novel mechanism which may be used for the synthesis of other enteric O antigens.

摘要

一种质粒,它既包含一个8.9 kb的染色体DNA插入片段,该片段含有痢疾志贺氏菌1型rfb簇的基因,又包含一个较小的插入片段,该片段含有来自痢疾志贺氏菌1型多拷贝质粒的rfp基因,该质粒能在大肠杆菌K - 12的rfb缺失菌株中高效表达O抗原。在rfb片段中鉴定出了8个基因:编码dTDP - 鼠李糖合成的rfbB - CAD簇、编码参与O抗原组装的疏水蛋白的rfbX、编码O抗原聚合酶的rfc以及两个糖基转移酶基因。O抗原的产生还需要大肠杆菌K - 12的rfe基因,已知该基因编码一种转移酶,可将N - 乙酰葡糖胺磷酸添加到载体脂质十一异戊烯磷酸上。因此,Rfe蛋白似乎起着沙门氏菌RfbP蛋白类似物的作用,为O单元提供第一个糖。由于一、二或三个糖的部分O单元能有效地转移到脂多糖核心,这一事实便于对其他基因进行功能分析。该分析表明,质粒编码的Rfp蛋白是添加O单元第二个糖的转移酶,而两个rfb转移酶添加远端糖以形成结构为(Rha - Rha - Gal - GlcNAc)n的O抗原。利用rfe基因产物作为添加O单元第一个糖的转移酶是一种新机制,可用于合成其他肠道O抗原。

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