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大肠杆菌K-12渗透压调节的依赖结合蛋白的甘氨酸甜菜碱转运系统(ProU)的克隆结构基因。

Cloned structural genes for the osmotically regulated binding-protein-dependent glycine betaine transport system (ProU) of Escherichia coli K-12.

作者信息

Faatz E, Middendorf A, Bremer E

机构信息

Department of Biology, University of Konstanz, Federal Republic of Germany.

出版信息

Mol Microbiol. 1988 Mar;2(2):265-79. doi: 10.1111/j.1365-2958.1988.tb00028.x.

Abstract

The proU locus of Escherichia coli encodes a high-affinity, binding-protein-dependent transport system (ProU) for the osmoprotectant glycine betaine. We cloned this locus into both low-copy-number lambda vectors and multicopy plasmids and demonstrated that these clones restore osmotically controlled synthesis of the periplasmic glycine betaine binding protein (GBBP) and the transport of glycine betaine in a delta (proU) strain. These clones allowed us to investigate the influence of osmolarity on ProU transport activity independent of the osmotically controlled expression of proU. ProU activity was strongly stimulated by a moderate increase in osmolarity and was partially inhibited by high osmolarity. This activity profile differs from the profile of the osmotically regulated proU expression. The proU locus is organized in an operon and the position of the structural gene (proV) for GBBP is defined using a minicell system. We determined that at least three proteins (in addition to GBBP) are encoded by the proU locus. We also investigated the permeation of glycine betaine across the outer membrane. At low substrate concentration (0.7 microM), permeation of glycine betaine was entirely dependent on the OmpF and OmpC porins.

摘要

大肠杆菌的proU基因座编码一种用于渗透保护剂甘氨酸甜菜碱的高亲和力、依赖结合蛋白的转运系统(ProU)。我们将该基因座克隆到低拷贝数的λ载体和多拷贝质粒中,并证明这些克隆可恢复δ(proU)菌株中受渗透压控制的周质甘氨酸甜菜碱结合蛋白(GBBP)的合成以及甘氨酸甜菜碱的转运。这些克隆使我们能够研究渗透压对ProU转运活性的影响,而不受proU渗透压控制表达的影响。适度增加渗透压可强烈刺激ProU活性,而高渗透压则会部分抑制该活性。这种活性模式与渗透压调节的proU表达模式不同。proU基因座以操纵子形式组织,使用小细胞系统确定了GBBP结构基因(proV)的位置。我们确定proU基因座至少编码三种蛋白质(除GBBP外)。我们还研究了甘氨酸甜菜碱在外膜中的通透情况。在低底物浓度(0.7 microM)下,甘氨酸甜菜碱的通透完全依赖于OmpF和OmpC孔蛋白。

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