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李斯特菌中隐秘原噬菌体(单链菌素)的特征分析及一个孔蛋白/内溶素基因的序列分析

Characterization of cryptic prophages (monocins) in Listeria and sequence analysis of a holin/endolysin gene.

作者信息

Zink R, Loessner M J, Scherer S

机构信息

Institut für Mikrobiologie, Technische Universität München, Freising, Germany.

出版信息

Microbiology (Reading). 1995 Oct;141 ( Pt 10):2577-84. doi: 10.1099/13500872-141-10-2577.

DOI:10.1099/13500872-141-10-2577
PMID:7582018
Abstract

Monocins in Listeria were induced by UV-irradiation of liquid cultures, and defective phage particles were purified from the lysates. Electron microscopy showed flexible, non-contractile bacteriophage-tail-like particles, consisting of specific proteins of molecular mass 20-45 kDa and pI 4.6-6.7. These particles were able to lyse listerial cells. DNA sequence homologies between chromosomal DNA of monocin-producing strains and labelled Listeria phage DNAs were inferred from DNA/DNA hybridizations, suggesting that most of the prophage DNA is still present in the listerial chromosome. An endolysin gene cpl2438 was cloned from listerial chromosomal DNA and was identified by its expression of lytic activity against Listeria cells in a bioassay. The gene consists of 864 nt encoding a protein of 287 aa with a calculated molecular mass of 32975 Da (CPL2438). This is in good agreement with the size of a protein observed in SDS-PAGE after overexpression of the lytic protein in Escherichia coli. The nucleotide sequence of a putative holin gene (hol2438, 291 nt) upstream of cpl2438 was determined after PCR-amplification of listerial DNA and it shows typical features common to the holin gene family. Expression of the encoded protein (HOL2438, 95 aa, 10.1 kDa) in E. coli was found to be lethal for the host cells. The results underline the close relationship between monocins and intact Listeria bacteriophages, indicating that monocins are incompletely assembled phage particles derived from cryptic prophages of Listeria, probably including the phage lysin.

摘要

通过对李斯特菌液体培养物进行紫外线照射诱导产生单霉素,并从裂解物中纯化出有缺陷的噬菌体颗粒。电子显微镜显示有柔性、非收缩性的噬菌体尾状颗粒,由分子量为20 - 45 kDa、等电点为4.6 - 6.7的特定蛋白质组成。这些颗粒能够裂解李斯特菌细胞。通过DNA/DNA杂交推断产单霉素菌株的染色体DNA与标记的李斯特菌噬菌体DNA之间的DNA序列同源性,表明大多数前噬菌体DNA仍存在于李斯特菌染色体中。从李斯特菌染色体DNA中克隆出一种内溶素基因cpl2438,并通过其在生物测定中对李斯特菌细胞的裂解活性表达来鉴定。该基因由864个核苷酸组成,编码一个287个氨基酸的蛋白质,计算分子量为32975 Da(CPL2438)。这与在大肠杆菌中过表达裂解蛋白后在SDS - PAGE中观察到的蛋白质大小高度一致。在对李斯特菌DNA进行PCR扩增后,确定了cpl2438上游假定的穿孔素基因(hol2438,291个核苷酸)的核苷酸序列,它显示出穿孔素基因家族共有的典型特征。发现编码的蛋白质(HOL2438,95个氨基酸,10.1 kDa)在大肠杆菌中的表达对宿主细胞是致死的。结果强调了单霉素与完整的李斯特菌噬菌体之间的密切关系,表明单霉素是源自李斯特菌隐蔽前噬菌体的不完全组装的噬菌体颗粒,可能包括噬菌体溶素。

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