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细胞生长和λ噬菌体发育受同一个必需的大肠杆菌基因ftsH/hflB控制。

Cell growth and lambda phage development controlled by the same essential Escherichia coli gene, ftsH/hflB.

作者信息

Herman C, Ogura T, Tomoyasu T, Hiraga S, Akiyama Y, Ito K, Thomas R, D'Ari R, Bouloc P

机构信息

Institut Jacques Monod (Centre National de la Recherche Scientifique, Université Paris 7), France.

出版信息

Proc Natl Acad Sci U S A. 1993 Nov 15;90(22):10861-5. doi: 10.1073/pnas.90.22.10861.

Abstract

The lambda phage choice between lysis and lysogeny is influenced by certain host functions in Escherichia coli. We found that the frequency of lambda lysogenization is markedly increased in the ftsH1 temperature-sensitive mutant. The ftsH gene, previously shown to code for an essential inner membrane protein with putative ATPase activity, is identical to hflB, a gene involved in the stability of the phage cII activator protein. The lysogenic decision controlled by FtsH/HflB is independent of that controlled by the protease HflA. Overproduction of FtsH/HflB suppresses the high frequency of lysogenization in an hflA null mutant. The FtsH/HflB protein, which stimulates cII degradation, may be a component of an HflA-independent proteolytic pathway, or it may act as a chaperone, maintaining cII in a conformation subject to proteolysis via such a pathway. Suppressor mutations of ftsH1 temperature-sensitive lethality, located in the fur gene (coding for the ferric uptake regulator), did not restore FtsH/HflB activity with respect to lambda lysogenization.

摘要

λ噬菌体在裂解和溶原化之间的选择受大肠杆菌中某些宿主功能的影响。我们发现,在ftsH1温度敏感突变体中,λ噬菌体溶原化的频率显著增加。ftsH基因先前已被证明编码一种具有假定ATP酶活性的必需内膜蛋白,它与hflB基因相同,hflB基因参与噬菌体cII激活蛋白的稳定性。由FtsH/HflB控制的溶原化决定独立于由蛋白酶HflA控制的溶原化决定。FtsH/HflB的过量表达抑制了hflA缺失突变体中的高溶原化频率。刺激cII降解的FtsH/HflB蛋白可能是不依赖HflA的蛋白水解途径的一个组成部分,或者它可能作为一种伴侣蛋白,通过这样的途径将cII维持在易于被蛋白水解的构象中。位于fur基因(编码铁摄取调节因子)中的ftsH1温度敏感致死性的抑制突变,在λ噬菌体溶原化方面并未恢复FtsH/HflB的活性。

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