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噬菌体对大肠杆菌志贺毒素1产生和释放的控制

Bacteriophage control of Shiga toxin 1 production and release by Escherichia coli.

作者信息

Wagner Patrick L, Livny Jonathan, Neely Melody N, Acheson David W K, Friedman David I, Waldor Matthew K

机构信息

Howard Hughes Medical Institute and Division of Geographic Medicine and Infectious Diseases, New England Medical Center and Tufts University School of Medicine, Boston, MA 02111, USA.

出版信息

Mol Microbiol. 2002 May;44(4):957-70. doi: 10.1046/j.1365-2958.2002.02950.x.

DOI:10.1046/j.1365-2958.2002.02950.x
PMID:12010491
Abstract

The stx genes of many Shiga toxin-encoding Escherichia coli (STEC) strains are encoded by prophages of the lambda bacteriophage family. In the genome of the Stx1-encoding phage H-19B, the stx(1)AB genes are found approximately 1 kb downstream of the late phage promoter, p(R)', but are known to be regulated by the associated iron-regulated promoter, p(Stx1). Growth of H-19B lysogens in low iron concentrations or in conditions that induce the prophage results in increased Stx1 production. Although the mechanism by which low iron concentration induces Stx1 production is well understood, the mechanisms by which phage induction enhances toxin production have not been extensively characterized. The studies reported here identify the factors that contribute to Stx1 production after induction of the H-19B prophage. We found that replication of the phage genome, with the associated increase in stx(1)AB copy number, is the most quantitatively important mechanism by which H-19B induction increases Stx1 production. Three promoters are shown to be involved in stx(1)AB transcription after phage induction, the iron-regulated p(Stx1) and the phage-regulated p(R) and p(R)' promoters, the relative importance of which varies with environmental conditions. Late phage transcription initiating at the p(R)' promoter, contrary to previous findings in the related Stx2-encoding phage phi 361, was found to be unnecessary for high-level Stx1 production after phage induction. Finally, we present evidence that phage-mediated lysis regulates the quantity of Stx1 produced by determining the duration of Stx1 accumulation and provides a mechanism for Stx1 release. By amplifying stx(1)AB copy number, regulating stx(1)AB transcription and allowing for Stx1 release, the biology of the Stx-encoding phages contributes greatly to the production of Stx, the principal virulence factor of STEC.

摘要

许多产志贺毒素大肠杆菌(STEC)菌株的stx基因由λ噬菌体家族的前噬菌体编码。在编码Stx1的噬菌体H - 19B的基因组中,stx(1)AB基因位于晚期噬菌体启动子p(R)'下游约1 kb处,但已知受相关的铁调节启动子p(Stx1)调控。H - 19B溶原菌在低铁浓度或诱导前噬菌体的条件下生长会导致Stx1产量增加。尽管低铁浓度诱导Stx1产生的机制已得到充分了解,但噬菌体诱导增强毒素产生的机制尚未得到广泛研究。本文报道的研究确定了H - 19B前噬菌体诱导后导致Stx1产生的因素。我们发现噬菌体基因组的复制以及stx(1)AB拷贝数的相应增加,是H - 19B诱导增加Stx1产生的最主要定量机制。研究表明,噬菌体诱导后,有三个启动子参与stx(1)AB转录,即铁调节的p(Stx1)以及噬菌体调节的p(R)和p(R)'启动子,它们的相对重要性随环境条件而变化。与之前在相关的编码Stx2的噬菌体phi 361中的发现相反,发现在噬菌体诱导后高水平的Stx1产生并不需要从p(R)'启动子起始的晚期噬菌体转录。最后,我们提供证据表明噬菌体介导的裂解通过确定Stx1积累的持续时间来调节Stx1产生的量,并为Stx1释放提供了一种机制。通过扩增stx(1)AB拷贝数、调节stx(1)AB转录并允许Stx1释放,编码Stx的噬菌体生物学特性对Stx(STEC的主要毒力因子)的产生有很大贡献。

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