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利用phoA基因融合鉴定编码分泌蛋白的结核分枝杆菌DNA序列。

Identification of mycobacterium tuberculosis DNA sequences encoding exported proteins by using phoA gene fusions.

作者信息

Lim E M, Rauzier J, Timm J, Torrea G, Murray A, Gicquel B, Portnoi D

机构信息

Unité de Génétique Mycobactérienne, Centre National de la Recherche Scientifique, URA 1300, Institut Pasteur, Paris, France.

出版信息

J Bacteriol. 1995 Jan;177(1):59-65. doi: 10.1128/jb.177.1.59-65.1995.

Abstract

The activity of bacterial alkaline phosphatase (PhoA) is dependent on it being exported across the plasma membrane. A plasmid vector (pJEM11) allowing fusions between phoA and genes encoding exported proteins was constructed to study protein export in mycobacteria. Introduction of the Mycobacterium fortuitum beta-lactamase gene (blaF*) into this vector led to the production in M. smegmatis of protein fusions with PhoA activity. A genomic library from M. tuberculosis was constructed in pJEM11 and screened in M. smegmatis for clones with PhoA activity. Sequences of the M. tuberculosis inserts directing the production of protein fusions in these PhoA-positive clones were determined. They include part of the already-known exported 19-kDa lipoprotein, a sequence with similarities to the exported 28-kDa antigen from M. leprae, a sequence encoding a protein sharing conserved amino acid motifs with stearoyl-acyl-carrier-protein desaturases, and unknown sequences. This approach thus appears to identify sequences directing protein export, and we expect that more extensive screening of such libraries will lead to a better understanding of protein export in M. tuberculosis.

摘要

细菌碱性磷酸酶(PhoA)的活性取决于其被转运穿过质膜。构建了一种质粒载体(pJEM11),可使phoA与编码输出蛋白的基因融合,以研究分枝杆菌中的蛋白质输出。将偶然分枝杆菌β-内酰胺酶基因(blaF*)导入该载体,导致耻垢分枝杆菌产生具有PhoA活性的蛋白质融合体。用pJEM11构建了结核分枝杆菌的基因组文库,并在耻垢分枝杆菌中筛选具有PhoA活性的克隆。测定了这些PhoA阳性克隆中指导蛋白质融合体产生的结核分枝杆菌插入片段的序列。它们包括部分已知的19 kDa输出脂蛋白、一段与麻风分枝杆菌输出的28 kDa抗原相似的序列、一段编码与硬脂酰-酰基载体蛋白去饱和酶具有保守氨基酸基序的蛋白质的序列,以及未知序列。因此,这种方法似乎可以鉴定指导蛋白质输出的序列,并且我们预计对这类文库进行更广泛的筛选将有助于更好地理解结核分枝杆菌中的蛋白质输出。

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