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通过 Halobacterium salinarum R1 中的 Pst 转运体调控磷酸盐摄取。

Regulation of phosphate uptake via Pst transporters in Halobacterium salinarum R1.

机构信息

Max-Planck-Institute of Biochemistry, Department of Membrane Biochemistry, Am Klopferspitz 18, 82152 Martinsried, Germany.

出版信息

Mol Microbiol. 2010 Apr;76(2):378-92. doi: 10.1111/j.1365-2958.2010.07101.x. Epub 2010 Mar 28.

Abstract

The genome of the archaeon Halobacterium salinarum contains two copies of the pst (phosphate-specific transport) operon, the genes of which are related to well-studied bacterial homologues. Both operons (pst1 and pst2) were shown to be polycistronic and, when under P(i)-limited conditions, transcription initiated 1 bp upstream of the translational starts. Under P(i) saturation, the pst1 operon utilized an additional transcription start site 59 bp upstream of the first one. The leaderless pst1 transcript was found to be more efficiently translated than the leadered transcript. Promoter strengths differed significantly between the two operons and when P(i) levels changed. The basal pst1 promoter activity in P(i)-saturated conditions was minimal while the pst2 promoter was active. In contrast, phosphate limitation induced the pst1 operon threefold more than the pst2 operon. We identified basic and phosphate-dependent cis-acting elements in both promoters. Phosphate-uptake assays conducted with several Pst1 and Pst2 mutant strains revealed differences in the substrate affinities between the two transporters and also suggested that the P(i)-binding proteins PstS1 and PstS2 can interact with either of the two permease subunits of the transporters. The tactic behaviour of wild type and pst-deletion strains showed that the Pst1 transporter plays an important role for phosphate-directed chemotaxis.

摘要

古菌盐杆菌的基因组包含两个 pst(磷酸特异性转运)操纵子,这些基因与研究充分的细菌同源物有关。两个操纵子(pst1 和 pst2)均为多顺反子,在 P(i)-有限条件下,转录起始于翻译起始点上游 1 bp。在 P(i)饱和条件下,pst1 操纵子利用了第一个转录起始点上游 59 bp 的另一个转录起始点。无启动子的 pst1 转录本比有启动子的转录本翻译效率更高。两个操纵子的启动子强度差异显著,且当 P(i)水平发生变化时也会发生变化。在 P(i)饱和条件下,基本的 pst1 启动子活性最小,而 pst2 启动子是活跃的。相比之下,磷酸盐限制诱导 pst1 操纵子的表达是 pst2 操纵子的三倍。我们在两个启动子中都鉴定了基本的和依赖于磷酸盐的顺式作用元件。对几种 Pst1 和 Pst2 突变株进行的磷酸盐摄取测定表明,两种转运体的底物亲和力存在差异,并且还表明 P(i)-结合蛋白 PstS1 和 PstS2 可以与转运体的两个渗透酶亚基之一相互作用。野生型和 pst 缺失菌株的策略行为表明,Pst1 转运体在磷酸盐导向的趋化作用中发挥重要作用。

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