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大肠杆菌O9多糖的表达:大肠杆菌O9 rfb基因簇的测序、甘露糖基转移酶的特性分析以及ATP结合盒转运系统的证据

Expression of the O9 polysaccharide of Escherichia coli: sequencing of the E. coli O9 rfb gene cluster, characterization of mannosyl transferases, and evidence for an ATP-binding cassette transport system.

作者信息

Kido N, Torgov V I, Sugiyama T, Uchiya K, Sugihara H, Komatsu T, Kato N, Jann K

机构信息

Max-Planck-Institute für Immunobiologie, Freiburg, Germany.

出版信息

J Bacteriol. 1995 Apr;177(8):2178-87. doi: 10.1128/jb.177.8.2178-2187.1995.

Abstract

The rfb gene cluster of Escherichia coli O9 directs the synthesis of the O9-specific polysaccharide which has the structure -->2-alpha-Man-(1-->2)-alpha-Man-(1-->2)-alpha-Man-(1-->3)-alpha- Man-(1-->. The E. coli O9 rfb cluster has been sequenced, and six genes, in addition to the previously described rfbK and rfbM, were identified. They correspond to six open reading frames (ORFs) encoding polypeptides of 261, 431, 708, 815, 381, and 274 amino acids. They are all transcribed in the counter direction to those of the his operon. No gene was found between rfb and his. A higher G+C content indicated that E. coli O9 rfb evolved independently of the rfb clusters from other E. coli strains and from Shigella and Salmonella spp. Deletion mutagenesis, in combination with analysis of the in vitro synthesis of the O9 mannan in membranes isolated from the mutants, showed that three genes (termed mtfA, -B, and -C, encoding polypeptides of 815, 381, and 274 amino acids, respectively) directed alpha-mannosyl transferases. MtfC (from ORF274), the first mannosyl transferase, transfers a mannose to the endogenous acceptor. It critically depended on a functional rfe gene (which directs the synthesis of the endogenous acceptor) and initiates the growth of the polysaccharide chain. MtfB (from ORF381) then transfers two mannoses into the 3 position of the previous mannose, and MtfA (from ORF815) transfers three mannoses into the 2 position. Further chain growth needs only the two transferases MtfA and MtfB. Thus, there are fewer transferases needed than the number of sugars in the repeating unit. Analysis of the predicted amino acid sequence of the ORF261 and ORF431 proteins indicated that they function as components of an ATP-binding cassette transport system. A possible correlation between the mechanism of polymerization and mode of membrane translocation of the products is discussed.

摘要

大肠杆菌O9的rfb基因簇指导合成具有结构-->2-α-甘露糖-(1-->2)-α-甘露糖-(1-->2)-α-甘露糖-(1-->3)-α-甘露糖-(1-->的O9特异性多糖。已对大肠杆菌O9的rfb簇进行了测序,除了先前描述的rfbK和rfbM外,还鉴定出六个基因。它们对应于六个开放阅读框(ORF),分别编码261、431、708、815、381和274个氨基酸的多肽。它们都与组氨酸操纵子的转录方向相反。在rfb和his之间未发现基因。较高的G+C含量表明大肠杆菌O9的rfb是独立于其他大肠杆菌菌株以及志贺氏菌和沙门氏菌属的rfb簇进化而来的。缺失诱变结合对从突变体中分离的膜中O9甘露聚糖体外合成的分析表明,三个基因(分别称为mtfA、-B和-C,编码815、381和274个氨基酸的多肽)指导α-甘露糖基转移酶。MtfC(来自ORF274),即第一个甘露糖基转移酶,将一个甘露糖转移到内源性受体上。它严重依赖于功能性的rfe基因(指导内源性受体的合成)并启动多糖链的生长。然后MtfB(来自ORF381)将两个甘露糖转移到前一个甘露糖的3位,而MtfA(来自ORF815)将三个甘露糖转移到2位。进一步的链生长仅需要两种转移酶MtfA和MtfB。因此,所需的转移酶比重复单元中的糖数量少。对ORF261和ORF431蛋白质预测氨基酸序列的分析表明,它们作为ATP结合盒转运系统发挥作用。讨论了聚合机制与产物膜转运模式之间的可能相关性。

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