首页> 美国卫生研究院文献>Journal of Bacteriology >Transcript analysis of the c-vac region and differential synthesis of the two regulatory gas vesicle proteins GvpD and GvpE in Halobacterium salinarium PHH4.
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Transcript analysis of the c-vac region and differential synthesis of the two regulatory gas vesicle proteins GvpD and GvpE in Halobacterium salinarium PHH4.

机译:盐杆菌PHH4中c-vac区的转录本分析和两种调节性气体囊泡蛋白GvpD和GvpE的差异合成。

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摘要

Halobacterium salinarium PHH4 synthesizes gas vesicles in the stationary growth phase by the expression of 14 gyp genes arranged in two clusters. The chromosomal gvpACNO (c-gvpACNO) gene cluster (encoding the major structural gas vesicle protein GvpA and the minor structural protein GvpC was transcribed as three mRNA species starting at one promoter during the stationary phase of growth. The second gene cluster, c-gvpDEFGHIKLM), was transcribed during all stages of growth as a relatively unstable, single mRNA with a maximal length of 6 kb. In addition, a 1.7-kb c-gvpD transcript was synthesized during stationary growth starting at the same promotor as that of the cgvpDEFGHIJKLM mRNA. The expression of the first two genes located in this unit (c-gvpD and c-gvpE) was also monitored by Western blot (immunoblot) analyses using antisera raised against these proteins synthesized in Escherichia coli. While the cGvpD protein was present only during early exponential growth and disappeared during gas vesicle formation, the cGvpE protein was present during cGvpA and gas vesicle synthesis in the early stationary phase of growth. Previous data indicated that cGvpD is involved in repression of gas vesicle formation, whereas cGvpE is a transcriptional activator for the c-gvpA promoter. The appearance of both proteins during the growth cycle is in line with the functions of these proteins in gas vesicle synthesis. The mechanism of the differential translation of cGvpD and cGvpE from the c-gvpDEFGHIJKLM rnRNA still has to be elucidated, but antisense RNAs complementary to the 5' terminus as well as the 3' portion of the c-gvpD mRNA might be involved in this regulation. Such RNAs occurred during early stationary growth when the cGvpD protein level decreased and may possibly inhibit the translation of the c-gvpD mRNA.
机译:盐杆菌盐藻PHH4通过表达排列在两个簇中的14个gyp基因来合成处于静止生长期的气体囊泡。染色体gvpACNO(c-gvpACNO)基因簇(编码主要结构气体小泡蛋白GvpA和次要结构蛋白GvpC被转录为三个mRNA物种,在生长的稳定阶段从一个启动子开始转录。第二个基因簇c-gvpDEFGHIKLMLM ),在生长的所有阶段均转录为相对不稳定的,最大长度为6 kb的单一mRNA。另外,在稳定生长期间以与cgvpDEFGHIJKLM mRNA相同的启动子开始合成了1.7-kb c-gvpD转录本。还通过Western blot(免疫印迹)分析,使用针对大肠杆菌中合成的这些蛋白的抗血清,通过Western blot(免疫印迹)分析监测位于该单元中的前两个基因(c-gvpD和c-gvpE)的表达。虽然cGvpD蛋白仅在早期指数生长期间存在,并在气囊形成过程中消失,但cGvpE蛋白在cGvpA和生长早期稳定期的气囊合成期间存在。以前的数据表明,cGvpD参与了气囊形成的抑制,而cGvpE是c-gvpA启动子的转录激活因子。两种蛋白质在生长周期中的出现与这些蛋白质在气泡合成中的功能一致。来自c-gvpDEFGHIJKLM rnRNA的cGvpD和cGvpE差异翻译的机制仍然有待阐明,但是与c-gvpD mRNA的5'末端和3'部分互补的反义RNA可能与该调控有关。 。当cGvpD蛋白水平降低并且可能抑制c-gvpD mRNA的翻译时,此类RNA发生在早期静止生长期间。

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