首页> 美国卫生研究院文献>Journal of Bacteriology >Identification of esg a genetic locus involved in cell-cell signaling during Myxococcus xanthus development.
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Identification of esg a genetic locus involved in cell-cell signaling during Myxococcus xanthus development.

机译:esg的鉴定它是在黄色粘球菌发展过程中参与细胞信号传导的遗传基因座。

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摘要

JD258, a Tn5 insertion mutant of Myxococcus xanthus, was shown to have major defects in three development-associated properties: expression of the developmentally regulated tps gene, spore formation, and production of multicellular fruiting bodies. The defects in tps gene expression and sporulation could be substantially corrected, at the phenotypic level, by mixing JD258 with wild-type cells (extracellular complementation). By this criterion, JD258 appeared to be a new member of a group of conditional developmental mutants that were previously characterized and placed in four extracellular complementation groups (A to D) based on the ability of mutants in one group to stimulate development in mutants belonging to a different group (D. C. Hagen, A. P. Bretscher, and D. Kaiser, Dev. Biol. 64:284-296, 1978). Mutants from groups A, B, C, and D all displayed extracellular complementation activity when mixed with JD258. These results, and other aspects of the phenotype of JD258, indicate that this mutant defines a fifth extracellular complementation group, group E. The M. xanthus esg locus identified by the Tn5 insertion in JD258 was cloned in Escherichia coli and used for further genetic analysis of the locus. These studies indicated that the esg locus resides within a 2.5-kb region of the M. xanthus chromosome and that the locus contains at least two genetic complementation groups. Our results are consistent with a model in which the esg locus controls the production of a previously unrecognized extracellular signal that must be transmitted between cells for the completion of M. xanthus development.
机译:JD258,一种黄色粘球菌的Tn5插入突变体,在三个与发育相关的特性中显示出主要缺陷:发育调控的tps基因的表达,孢子形成和多细胞子实体的产生。通过将JD258与野生型细胞混合(细胞外互补),可以在表型水平上基本上纠正tps基因表达和孢子形成的缺陷。按照这一标准,JD258似乎是一组条件发育突变体的新成员,这些条件发育突变体先前已被鉴定并根据一组中的突变体刺激属于突变体的发育的能力而置于四个细胞外互补组(A至D)中。另一组(DC Hagen,AP Bretscher和D.Kaiser,Dev.Biol.64:284-296,1978)。与JD258混合时,A,B,C和D组的突变体均显示出细胞外互补活性。这些结果以及JD258表型的其他方面表明,该突变体定义了第五个细胞外互补组,即E组。通过在JD258中插入Tn5鉴定的X.anthus esg基因座已克隆到大肠杆菌中,并用于进一步的遗传分析的位置。这些研究表明,esg基因座位于黄单胞菌染色体的2.5-kb区域内,并且该基因座含有至少两个遗传互补基团。我们的结果与其中esg基因座控制先前无法识别的细胞外信号的产生的模型相符,该信号必须在细胞之间传递以完成黄腐支原体的发育。

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