首页> 外文OA文献 >Phylogenetic depth of S10 and spc operons: cloning and sequencing of a ribosomal protein gene cluster from the extremely thermophilic bacterium Thermotoga maritima.
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Phylogenetic depth of S10 and spc operons: cloning and sequencing of a ribosomal protein gene cluster from the extremely thermophilic bacterium Thermotoga maritima.

机译:S10和spc操纵子的系统发生深度:极端嗜热细菌马氏体(Thermotoga maritima)核糖体蛋白基因簇的克隆和测序。

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摘要

A segment of Thermotoga maritima DNA spanning 6,613 bp downstream from the gene tuf for elongation factor Tu was sequenced by use of a chromosome walking strategy. The sequenced region comprised a string of 14 tightly linked open reading frames (ORFs) starting 50 bp downstream from tuf. The first 11 ORFs were identified as homologs of ribosomal protein genes rps10, rpl3, rpl4, rpl23, rpl2, rps19, rpl22, rps3, rpl16, rpl29, and rps17 (which in Escherichia coli constitute the S10 operon, in that order); the last three ORFs were homologous to genes rpl14, rpl24, and rpl5 (which in E. coli constitute the three promoter-proximal genes of the spectinomycin operon). The 14-gene string was preceded by putative -35 and -10 promoter sequences situated 5' to gene rps10, within the 50-bp spacing between genes tuf and rps10; the same region exhibited a potential transcription termination signal for the upstream gene cluster (having tuf as the last gene) but displayed also the potential for formation of a hairpin loop hindering the terminator; this suggests that transcription of rps10 and downstream genes may start farther upstream. The similar organization of the sequenced rp genes in the deepest-branching bacterial phyla (T. maritima) and among Archaea has been interpreted as indicating that the S10-spc gene arrangement existed in the (last) common ancestor. The phylogenetic depth of the Thermotoga lineage was probed by use of r proteins as marker molecules: in all except one case (S3), Proteobacteria or the gram-positive bacteria, and not the genus Thermotoga, were the deepest-branching lineage; in only two cases, however, was the inferred branching order substantiated by bootstrap analysis.
机译:通过使用染色体行走策略,对延伸至Tuf基因的tuf基因下游6,613 bp下游的海栖嗜热菌DNA片段进行了测序。测序的区域包含一串14个紧密连接的开放阅读框(ORF),该开放阅读框位于tuf下游50 bp。前11个ORF被鉴定为核糖体蛋白基因rps10,rpl3,rpl4,rpl23,rpl2,rps19,rpl22,rps3,rpl16,rpl29和rps17的同源物(在大肠杆菌中按此顺序构成S10操纵子);最后三个ORF与rpl14,rpl24和rpl5基因(在大肠杆菌中构成大观霉素操纵子的三个启动子近端基因)同源。在14个基因串之前,位于基因rps10 5'端的推定的-35和-10启动子序列位于基因tuf和rps10之间50 bp的间隔内。同一区域显示出上游基因簇的潜在转录终止信号(以tuf作为最后一个基因),但也显示出可能形成阻碍终止子的发夹环;这表明rps10和下游基因的转录可能在更上游开始。在最深分支的细菌门(T. maritima)和古细菌之间,已测序的rp基因的相似组织已被解释为表明S10-spc基因排列存在于(最后一个)共同祖先中。通过使用r蛋白作为标记分子来探测嗜热菌谱​​系的系统发育深度:在除一种情况(S3)以外的所有病例中,变形杆菌或革兰氏阳性细菌而非嗜热菌属都是最深的分支谱系;但是,在只有两种情况下,引导分析证实了推论的分支顺序。

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