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大肠杆菌中由木糖基因xylF编码的D-木糖受体蛋白的分子遗传学。

Molecular genetics of a receptor protein for D-xylose, encoded by the gene xylF, in Escherichia coli.

作者信息

Sumiya M, Davis E O, Packman L C, McDonald T P, Henderson P J

机构信息

Department of Biochemistry, University of Cambridge, UK.

出版信息

Recept Channels. 1995;3(2):117-28.

PMID:8581399
Abstract

Mutants of Escherichia coli K12 have been isolated containing either the 'XylF' or the 'XylE' transport systems for D-xylose. This enabled the XylF system containing a D-xylose receptor-binding protein to be associated with high-affinity transport, apparent Km 0.2-4 microM, while the XylE sugar-H+ symporter system exhibited relatively low affinity, apparent Km 63-169 microM. Their apparent Vmax values were similar. Isolation of a xylose transport-negative mutation in a downstream gene, xylG, and a series of transduction experiments enabled the gene order xylB xylA p/o xyl(FG) mtlA to be proposed near 80 min on the E. coli chromosome. The xylose receptor protein (XylF) was highly purified from the periplasm and the sequence of its N-terminal 44 amino acids determined. From this a mixed oligonucleotide (14 mer) was synthesised of corresponding DNA sequence, hybridisation of which to restriction fragments from the ColE I hybrid plasmid, pLC32-9, which conferred xylose transport activity on a xylE- xylF- double mutant, enabled precise location of the xylF gene next to the xylose isomerase gene, xylA (3984 kbp on the Kohara physical map). The DNA sequence of the 2.5 kb Bgl II fragment containing the xylF gene was then determined, which confirmed the above gene order and revealed two divergent operons, probably regulated in a co-ordinate manner, one containing enzymes for catabolism of D-xylose, and the other proteins comprising the XylFG receptor-transport system. Analysis of the 330 amino acid sequence of the XylF receptor protein located the scission point of its leader peptide between Ala23 and Lys24, and revealed significant homologies with the other sugar receptor proteins for ribose (RbsB), galactose (MglB) and arabinose (AraF).

摘要

已分离出大肠杆菌K12的突变体,其含有用于D-木糖的“XylF”或“XylE”转运系统。这使得含有D-木糖受体结合蛋白的XylF系统与高亲和力转运相关,表观Km为0.2 - 4微摩尔,而XylE糖-H⁺同向转运体系统表现出相对较低的亲和力,表观Km为63 - 169微摩尔。它们的表观Vmax值相似。在下游基因xylG中分离出木糖转运阴性突变,并进行了一系列转导实验,从而提出在大肠杆菌染色体上接近80分钟处的基因顺序为xylB xylA p/o xyl(FG) mtlA。木糖受体蛋白(XylF)从周质中高度纯化,并确定了其N端44个氨基酸的序列。据此合成了相应DNA序列的混合寡核苷酸(14聚体),将其与来自ColE I杂交质粒pLC32 - 9的限制性片段杂交,该质粒赋予木糖转运活性给xylE⁻ xylF⁻双突变体,从而能够将xylF基因精确定位在木糖异构酶基因xylA旁边(在小原物理图谱上为3984千碱基对)。然后确定了包含xylF基因的2.5千碱基Bgl II片段的DNA序列,这证实了上述基因顺序,并揭示了两个不同的操纵子,可能以协调方式调控,一个包含用于D-木糖分解代谢的酶,另一个包含构成XylFG受体-转运系统的蛋白质。对XylF受体蛋白的330个氨基酸序列进行分析,确定了其前导肽在Ala23和Lys24之间的切割点,并揭示了与核糖(RbsB)、半乳糖(MglB)和阿拉伯糖(AraF)的其他糖受体蛋白有显著同源性。

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