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鉴定炭疽保护性抗原中与致死因子结合相关的氨基酸残基。

Identification of amino acid residues of anthrax protective antigen involved in binding with lethal factor.

作者信息

Chauhan Vibha, Bhatnagar Rakesh

机构信息

Centre For Biotechnology, Jawaharlal Nehru University, New Delhi 110067, India.

出版信息

Infect Immun. 2002 Aug;70(8):4477-84. doi: 10.1128/IAI.70.8.4477-4484.2002.

Abstract

Protective antigen (PA) and lethal factor (LF) are the two components of anthrax lethal toxin. PA is responsible for the translocation of LF to the cytosol. The binding of LF to cell surface receptor-bound PA is a prerequisite for the formation of lethal toxin. It has been hypothesized that hydrophobic residues P184, L187, F202, L203, P205, I207, I210, W226, and F236 of domain 1b of PA play an important role in the binding of PA to LF. These residues are normally buried in the 83-kDA version of PA, PA83, as determined by the crystal structure of PA. However, they become exposed due to the conformational change brought about by the cleavage of PA83 to PA63 by a cell surface protease. Mutation of the above-mentioned residues to alanine resulted in mutant proteins that were able to bind to the cell surface receptors and also to be specifically cleaved by the cellular proteases. All the mutant proteins except the F202A, L203A, P205A, and I207A mutants were able to bind to LF and were also toxic to macrophage cells in combination with LF. It was concluded that residues 202, 203, 205, and 207 of PA are essential for the binding of LF to PA.

摘要

保护性抗原(PA)和致死因子(LF)是炭疽致死毒素的两个组成部分。PA负责将LF转运至细胞质溶胶。LF与细胞表面受体结合的PA相结合是致死毒素形成的前提条件。据推测,PA 1b结构域的疏水性残基P184、L187、F202、L203、P205、I207、I210、W226和F236在PA与LF的结合中起重要作用。根据PA的晶体结构测定,这些残基通常埋藏在83-kDA版本的PA即PA83中。然而,由于细胞表面蛋白酶将PA83切割为PA63所带来的构象变化,它们会暴露出来。将上述残基突变为丙氨酸会产生能够与细胞表面受体结合且能被细胞蛋白酶特异性切割的突变蛋白。除F202A、L203A、P205A和I207A突变体外,所有突变蛋白均能与LF结合,并且与LF联合使用时对巨噬细胞有毒性。得出的结论是,PA的202、203、205和207位残基对于LF与PA的结合至关重要。

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