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信号-滞留-释放序列介导噬菌体P1溶菌酶的输出与调控。

A signal-arrest-release sequence mediates export and control of the phage P1 endolysin.

作者信息

Xu Min, Struck Douglas K, Deaton John, Wang Ing-Nang, Young Ry

机构信息

Department of Biochemistry and Biophysics, Texas A&M University, College Station, TX 77843-2128, USA.

出版信息

Proc Natl Acad Sci U S A. 2004 Apr 27;101(17):6415-20. doi: 10.1073/pnas.0400957101. Epub 2004 Apr 16.

Abstract

The Lyz endolysin of bacteriophage P1 was found to cause lysis of the host without a holin. Induction of a plasmid-cloned lyz resulted in lysis, and the lytic event could be triggered prematurely by treatments that dissipate the proton-motive force. Instead of requiring a holin, export was mediated by an N-terminal transmembrane domain (TMD) and required host sec function. Exported Lyz of identical SDS/PAGE mobility was found in both the membrane and periplasmic compartments, indicating that periplasmic Lyz was not generated by the proteolytic cleavage of the membrane-associated form. In gene fusion experiments, the Lyz TMD directed PhoA to both the membrane and periplasmic compartments, whereas the TMD of the integral membrane protein FtsI restricts Lyz to the membrane. Thus, the N-terminal domain of Lyz is both necessary and sufficient not only for export of this endolysin to the membrane but also for its release into the periplasm. The unusual N-terminal domain, rich in residues that are weakly hydrophobic, thus functions as a signal-arrest-release sequence, which first acts as a normal signal-arrest domain to direct the endolysin to the periplasm in membrane-tethered form and then allows it to be released as a soluble active enzyme in the periplasm. Examination of the protein sequences of related bacteriophage endolysins suggests that the presence of an N-terminal signal-arrest-release sequence is not unique to Lyz. These observations are discussed in relation to the role of holins in the control of host lysis by bacteriophage encoding a secretory endolysin.

摘要

噬菌体P1的溶菌酶Lyz被发现可在没有穿孔素的情况下导致宿主细胞裂解。诱导质粒克隆的lyz会导致细胞裂解,并且通过耗散质子动力的处理可过早触发裂解事件。Lyz的输出不是由穿孔素介导,而是由N端跨膜结构域(TMD)介导,并且需要宿主的sec功能。在膜和周质区室中均发现了具有相同SDS/PAGE迁移率的输出型Lyz,这表明周质Lyz不是由膜相关形式的蛋白水解切割产生的。在基因融合实验中,Lyz的TMD将碱性磷酸酶(PhoA)导向膜和周质区室,而内膜蛋白FtsI的TMD则将Lyz限制在膜上。因此,Lyz的N端结构域不仅对于这种溶菌酶输出到膜上是必要且充分的,而且对于其释放到周质中也是如此。富含弱疏水性残基的异常N端结构域因此起到信号滞留释放序列的作用,它首先作为正常的信号滞留结构域,以膜结合形式将溶菌酶导向周质,然后使其作为可溶性活性酶在周质中释放。对相关噬菌体溶菌酶的蛋白质序列分析表明,N端信号滞留释放序列并非Lyz所特有。本文结合穿孔素在通过编码分泌型溶菌酶的噬菌体控制宿主裂解中的作用,对这些观察结果进行了讨论。

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