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鼠伤寒沙门氏菌外膜磷脂酶A的拓扑结构

Topology of the outer membrane phospholipase A of Salmonella typhimurium.

作者信息

Merck K B, de Cock H, Verheij H M, Tommassen J

机构信息

Department of Molecular Cell Biology, Institute of Biomembranes, Utrecht University, The Netherlands.

出版信息

J Bacteriol. 1997 Jun;179(11):3443-50. doi: 10.1128/jb.179.11.3443-3450.1997.

Abstract

The outer membrane phospholipase A (OMPLA) of Enterobacteriaceae has been proposed to span the membrane 14 times as antiparallel amphipathic beta-strands, thereby exposing seven loops to the cell surface. We have employed the epitope insertion method to probe the topology of OMPLA of Salmonella typhimurium. First, missense mutations were introduced at various positions in the pldA gene, encoding OMPLA, to create unique BamHI sites. These BamHI sites were subsequently used to insert linkers, encoding a 16-amino-acid B-cell epitope. Proper assembly of all mutant proteins was revealed by their heat modifiability in sodium dodecyl sulfate-polyacrylamide gel electrophoresis. The accessibility of the inserted epitopes was assessed. Immunofluorescence analysis of intact cells with antibodies against the inserted epitope showed that three of seven predicted loops are indeed cell surface exposed. Trypsin accessibility experiments verified the cell surface exposure of two additional loops and provided support for the proposed periplasmic localization of three predicted turns. For two other predicted exposed loops, the results were not conclusive. These results support to a large extent the proposed topology model of OMPLA. Furthermore, the observation that the substitutions Glu66Pro and Glu247Gly virtually abolished enzymatic activity indicates that these residues might play a major role in catalysis.

摘要

肠杆菌科的外膜磷脂酶A(OMPLA)被认为以反平行两亲性β链跨膜14次,从而使七个环暴露于细胞表面。我们采用表位插入法来探究鼠伤寒沙门氏菌OMPLA的拓扑结构。首先,在编码OMPLA的pldA基因的各个位置引入错义突变,以创建独特的BamHI位点。随后利用这些BamHI位点插入编码16个氨基酸的B细胞表位的接头。通过它们在十二烷基硫酸钠-聚丙烯酰胺凝胶电泳中的热可修饰性揭示了所有突变蛋白的正确组装。评估了插入表位的可及性。用针对插入表位的抗体对完整细胞进行免疫荧光分析表明,七个预测环中的三个确实暴露于细胞表面。胰蛋白酶可及性实验证实了另外两个环的细胞表面暴露,并为三个预测转角的拟周质定位提供了支持。对于另外两个预测的暴露环,结果尚无定论。这些结果在很大程度上支持了所提出的OMPLA拓扑模型。此外,Glu66Pro和Glu247Gly取代几乎消除酶活性这一观察结果表明,这些残基可能在催化中起主要作用。

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