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五个在感染的哺乳动物细胞中优先表达的单核细胞增生李斯特菌基因:plcA、purH、purD、pyrE和一个精氨酸ABC转运蛋白基因arpJ。

Five Listeria monocytogenes genes preferentially expressed in infected mammalian cells: plcA, purH, purD, pyrE and an arginine ABC transporter gene, arpJ.

作者信息

Klarsfeld A D, Goossens P L, Cossart P

机构信息

Unité des Interactions Bactéries-Cellules, CNRS URA 1300, Institut Pasteur, Paris, France.

出版信息

Mol Microbiol. 1994 Aug;13(4):585-97. doi: 10.1111/j.1365-2958.1994.tb00453.x.

DOI:10.1111/j.1365-2958.1994.tb00453.x
PMID:7997171
Abstract

Listeria monocytogenes is a bacterial pathogen that multiplies within the cytosol of eukaryotic cells. To identify Listeria genes with preferentially intracellular expression (pic genes), a library of Tn917-lac insertion mutants was screened for transcriptional fusions to lacZ with higher expression inside a macrophage-like cell line than in a rich broth medium. Five pic genes with up to 100-fold induction inside cells were identified. Three of them (purH, purD and pyrE) were involved in nucleotide biosynthesis. One was part of an operon encoding an ABC (ATP-binding cassette) transporter for arginine. The corresponding mutants were not affected in intracellular growth, cell-to-cell spread or virulence, except for the transporter mutant, whose LD50 after intravenous infection of mice was twofold higher than the wild-type. The fifth gene was plcA, a previously identified virulence gene that encodes a phosphatidylinositol-phospholipase C, and is cotranscribed with prfA, a gene encoding a pleiotropic transcriptional activator of known virulence genes. Although plcA expression is known to depend on PrfA, a prfA promoter-lacZ fusion was highly expressed both inside and outside cells. Furthermore, in the presence of cellobiose, a disaccharide recently shown to repress plcA and hly expression, plcA and hly mRNA levels were dramatically reduced without any decrease in the monocistronic prfA mRNA levels. These results demonstrate that virulence gene activation does not depend only on prfA transcript accumulation.

摘要

单核细胞增生李斯特菌是一种在真核细胞胞质溶胶中繁殖的细菌病原体。为了鉴定具有优先细胞内表达的李斯特菌基因(pic基因),对Tn917-lac插入突变体文库进行筛选,寻找与lacZ的转录融合体,其在巨噬细胞样细胞系内的表达高于在丰富肉汤培养基中的表达。鉴定出了五个在细胞内诱导高达100倍的pic基因。其中三个(purH、purD和pyrE)参与核苷酸生物合成。一个是编码精氨酸ABC(ATP结合盒)转运蛋白的操纵子的一部分。除了转运蛋白突变体外,相应的突变体在细胞内生长、细胞间传播或毒力方面均未受到影响,该转运蛋白突变体经静脉感染小鼠后的半数致死剂量比野生型高两倍。第五个基因是plcA,一个先前鉴定的毒力基因,编码磷脂酰肌醇磷脂酶C,并与prfA共转录,prfA是一个编码已知毒力基因的多效性转录激活因子的基因。尽管已知plcA的表达依赖于PrfA,但prfA启动子-lacZ融合体在细胞内外均高表达。此外,在存在纤维二糖(一种最近显示可抑制plcA和hly表达的二糖)的情况下,plcA和hly的mRNA水平显著降低,而单顺反子prfA的mRNA水平没有任何下降。这些结果表明,毒力基因的激活不仅仅取决于prfA转录本的积累。

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