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结核分枝杆菌 ftsZ 表达和最小启动子活性。

Mycobacterium tuberculosis ftsZ expression and minimal promoter activity.

机构信息

Biochemistry Department, The University of Texas Health Science Center @ Tyler, Tyler, TX 75708, USA.

出版信息

Tuberculosis (Edinb). 2009 Dec;89 Suppl 1(Suppl 1):S60-4. doi: 10.1016/S1472-9792(09)70014-9.

Abstract

Optimal levels of ftsZ gene product are shown to be required for initiation of the cell division process in Mycobacterium tuberculosis. Here, we report that the ftsZ gene expression is sharply down-regulated during starvation and hypoxia, conditions that are believed to result in growth arrest, but is restored upon dilution of cultures into fresh oxygen-rich media. Primer extension analysis identified four transcriptional start sites, designated as P1, P2, P3 and P4 at nucleotide positions -43, -101, -263, and -787, respectively, in the immediate upstream flanking region of the ftsZ initiation codon. Promoter deletion and homologous recombination experiments revealed that ftsZ expression from the 101-bp region is sufficient for M. tuberculosis viability. All promoter strains had reduced FtsZ levels compared to wild-type, although the loss of P4 severely compromised FtsZ levels during both the active and stationary phases. We propose that ftsZ expression from all promoters is required for optimal intracellular FtsZ levels and that the activities of P4 and possibly other promoters are down-regulated during growth-arrest conditions.

摘要

最佳水平的ftsZ 基因产物被证明是起始分枝杆菌细胞分裂过程所必需的。在这里,我们报告说ftsZ 基因表达在饥饿和缺氧期间急剧下调,这些条件被认为会导致生长停滞,但在将培养物稀释到富含新鲜氧气的培养基中时会恢复。引物延伸分析确定了四个转录起始位点,分别在 ftsZ 起始密码子的上游侧翼区域的核苷酸位置-43、-101、-263 和-787 处,指定为 P1、P2、P3 和 P4。启动子缺失和同源重组实验表明,ftsZ 从 101bp 区域的表达足以维持结核分枝杆菌的活力。与野生型相比,所有启动子菌株的 FtsZ 水平都降低了,尽管缺失 P4 在活性和静止期都会严重降低 FtsZ 水平。我们提出,ftsZ 从所有启动子的表达都需要最佳的细胞内 FtsZ 水平,并且在生长停滞条件下,P4 和可能其他启动子的活性被下调。

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Mycobacterium tuberculosis ftsZ expression and minimal promoter activity.结核分枝杆菌 ftsZ 表达和最小启动子活性。
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