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从环境样本中纯化游离志贺毒素产生菌噬菌体的方法的开发和应用。

Development and application of a method for the purification of free shigatoxigenic bacteriophage from environmental samples.

机构信息

Microbiology Research Group, Institute of Integrative Biology, University of Liverpool, Liverpool, L69 7ZB, United Kingdom.

出版信息

J Microbiol Methods. 2012 Nov;91(2):240-5. doi: 10.1016/j.mimet.2012.08.017. Epub 2012 Sep 4.

Abstract

Shiga toxin producing Escherichia coli (STEC) strains are foodborne pathogens whose ability to produce Shiga toxin (Stx) is due to the integration of Stx-encoding lambdoid bacteriophage (Stx phage). Circulating, infective Stx phages are very difficult to isolate, purify and propagate such that there is no information on their genetic composition and properties. Here we describe a novel approach that exploits the phage's ability to infect their host and form a lysogen, thus enabling purification of Stx phages by a series of sequential lysogen isolation and induction steps. A total of 15 Stx phages were rigorously purified from water samples in this way, classified by TEM and genotyped using a PCR-based multi-loci characterisation system. Each phage possessed only one variant of each target gene type, thus confirming its purity, with 9 of the 15 phages possessing a short tail-spike gene and identified by TEM as Podoviridae. The remaining 6 phages possessed long tails, four of which appeared to be contractile in nature (Myoviridae) and two of which were morphologically very similar to bacteriophage lambda (Siphoviridae).

摘要

产志贺毒素大肠杆菌(STEC)菌株是食源性病原体,其产生志贺毒素(Stx)的能力是由于 Stx 编码的 lambda 噬菌体(Stx 噬菌体)的整合。循环的、感染性的 Stx 噬菌体非常难以分离、纯化和繁殖,因此没有关于它们遗传组成和特性的信息。在这里,我们描述了一种新方法,该方法利用噬菌体感染其宿主并形成溶原菌的能力,从而能够通过一系列连续的溶原菌分离和诱导步骤来纯化 Stx 噬菌体。总共从水样中严格纯化了 15 种 Stx 噬菌体,通过 TEM 分类,并使用基于 PCR 的多基因座特征系统进行基因分型。每种噬菌体仅具有一种靶基因类型的一种变体,从而确认了其纯度,其中 15 种噬菌体中的 9 种具有短尾刺基因,并且通过 TEM 鉴定为 Podoviridae。其余 6 种噬菌体具有长尾,其中 4 种似乎具有收缩性质(肌病毒科),2 种在形态上非常类似于噬菌体 lambda(长尾噬菌体科)。

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