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大肠杆菌厌氧C4-二羧酸转运蛋白DcuA的拓扑分析

Topological analysis of DcuA, an anaerobic C4-dicarboxylate transporter of Escherichia coli.

作者信息

Golby P, Kelly D J, Guest J R, Andrews S C

机构信息

School of Animal and Microbial Sciences, University of Reading, Reading RG6 6AJ, United Kingdom.

出版信息

J Bacteriol. 1998 Sep;180(18):4821-7. doi: 10.1128/JB.180.18.4821-4827.1998.

Abstract

Escherichia coli possesses three independent anaerobic C4-dicarboxylate transport systems encoded by the dcuA, dcuB, and dcuC genes. The dcuA and dcuB genes encode related integral inner-membrane proteins, DcuA and DcuB (433 and 446 amino acid residues), which have 36% amino acid sequence identity. A previous amino acid sequence-based analysis predicted that DcuA and DcuB contain either 12 or 14 transmembrane helices, with the N and C termini located in the cytoplasm or periplasm (S. Six, S. C. Andrews, G. Unden, and J. R. Guest, J. Bacteriol. 176:6470-6478, 1994). These predictions were tested by constructing and analyzing 66 DcuA-BlaM fusions in which C terminally truncated forms of DcuA are fused to a beta-lactamase protein lacking the N-terminal signal peptide. The resulting topological model differs from those previously predicted. It has just 10 transmembrane helices and a central, 80-residue cytoplasmic loop between helices 5 and 6. The N and C termini are located in the periplasm and the predicted orientation is consistent with the "positive-inside rule." Two highly hydrophobic segments are not membrane spanning: one is in the cytoplasmic loop; the other is in the C-terminal periplasmic region. The topological model obtained for DcuA can be applied to DcuA homologues in other bacteria as well as to DcuB. Overproduction of DcuA to 15% of inner-membrane protein was obtained with the lacUV5-promoter-based plasmid, pYZ4.

摘要

大肠杆菌拥有由dcuA、dcuB和dcuC基因编码的三种独立的厌氧C4 - 二羧酸转运系统。dcuA和dcuB基因编码相关的内膜整合蛋白DcuA和DcuB(分别为433和446个氨基酸残基),它们具有36%的氨基酸序列同一性。先前基于氨基酸序列的分析预测,DcuA和DcuB含有12个或14个跨膜螺旋,N端和C端位于细胞质或周质中(S. Six、S. C. Andrews、G. Unden和J. R. Guest,《细菌学杂志》176:6470 - 6478,1994年)。通过构建和分析66个DcuA - BlaM融合体对这些预测进行了验证,其中DcuA的C端截短形式与缺乏N端信号肽的β - 内酰胺酶蛋白融合。所得的拓扑模型与先前预测的不同。它只有10个跨膜螺旋,在螺旋5和6之间有一个80个残基的中央细胞质环。N端和C端位于周质中,预测的方向与“正内规则”一致。两个高度疏水的片段不跨膜:一个在细胞质环中;另一个在C端周质区域。为DcuA获得的拓扑模型可应用于其他细菌中的DcuA同源物以及DcuB。使用基于lacUV5启动子的质粒pYZ4,DcuA的过量表达量达到内膜蛋白的15%。

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