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首页> 外文期刊>Molecular Microbiology >Modulation of Lactobacillus casei bacteriophage A2 lytic/lysogenic cycles by binding of Gp25 to the early lytic mRNA
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Modulation of Lactobacillus casei bacteriophage A2 lytic/lysogenic cycles by binding of Gp25 to the early lytic mRNA

机译:通过将GP25结合到早期裂变mRNA,调节乳杆菌菌株A2裂解/溶血性循环

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摘要

The genetic switch of Lactobacillus casei bacteriophage A2 is regulated by the CI protein, which represses the early lytic promoter P-R and Cro that abolishes expression from the lysogenic promoter P-L. Lysogens contain equivalent cI and cro-gp25 mRNA concentrations, i.e., CI only partially represses P-R, predicting a lytic cycle dominance. However, A2 generates stable lysogens. This may be due to Gp25 binding to the cro-gp25 mRNA between the ribosomal binding site and the cro start codon, which abolishes its translation. Upon lytic cycle induction, CI is partially degraded, cro-gp25 mRNA levels increase, and Cro accumulates, launching viral progeny production. The concomitant concentration increase of Gp25 restricts cro mRNA translation, which, together with the low but detectable levels of CI late during the lytic cycle, promotes reentry of part of the cell population into the lysogenic cycle, thus explaining the low proportion of L. casei lysogens that become lysed (similar to 1%). A2 shares its genetic switch structure with many other Firmicutes phages. The data presented may constitute a model of how these phages make the decision for lysis versus lysogeny.
机译:乳酸杆菌菌株A2的遗传开关由CI蛋白调节,其抑制早期的裂解启动子P-R和CRO,其消除了溶酶体启动子P-L的表达。溶血菌含有当量CI和CRO-GP25 mRNA浓度,即CI仅部分抑制P-R,预测裂解循环的优势。然而,A2产生稳定的溶血性。这可能是由于GP25与核糖体结合位点和CRO开始密码子之间的CRO-GP25 mRNA结合,这消除了其翻译。在裂变循环诱导后,CI部分降解,CRO-GP25 mRNA水平增加,CRO积聚,发动病毒后代生产。 GP25的综合浓度增加限制了CRO mRNA翻译,该翻译与在裂解循环期间晚期的低但可检测水平的CI,将部分细胞群的再入性促进到溶血性循环中,从而解释了L.酪虫的低比例裂解的溶血剂(类似于1%)。 A2与许多其他常规噬菌体共用其遗传开关结构。所提出的数据可以构成这些噬菌体如何做出裂解裂解与溶解的模型。

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