Analyzing the Interaction of RseA and RseB, the Two Negative Regulators of the σE Envelope Stress Response, Using a Combined Bioinformatic and Experimental Strategy

被引:8
作者
Ahuja, Nidhi [1 ]
Korkin, Dmitry [3 ,4 ]
Chaba, Rachna [1 ]
Cezairliyan, Brent O. [5 ]
Sauer, Robert T. [5 ]
Kim, Kyeong Kyu [6 ]
Gross, Carol A. [1 ,2 ]
机构
[1] Univ Calif San Francisco, Dept Microbiol & Immunol, San Francisco, CA 94158 USA
[2] Univ Calif San Francisco, Dept Cell & Tissue Biol, San Francisco, CA 94158 USA
[3] Univ Missouri, Inst Informat, Columbia, MO 65211 USA
[4] Univ Missouri, Dept Comp Sci, Columbia, MO 65211 USA
[5] MIT, Dept Biol, Cambridge, MA 02139 USA
[6] Sungkyunkwan Univ, Samsung Biomed Res Inst, Dept Mol Cell Biol, Suwon 440746, South Korea
基金
美国国家卫生研究院;
关键词
ESCHERICHIA-COLI SIGMA(E); MULTIPLE SEQUENCE ALIGNMENT; EXTRACYTOPLASMIC STRESS; CRYSTAL-STRUCTURE; PERIPLASMIC STRESS; PDZ DOMAIN; PROTEIN; PROTEOLYSIS; BINDING; RPOE;
D O I
10.1074/jbc.M806012200
中图分类号
Q5 [生物化学]; Q7 [分子生物学];
学科分类号
071010 ; 081704 ;
摘要
The Escherichia coli envelope stress response is controlled by the alternative sigma factor, sigma(E), and is induced when unfolded outer membrane proteins accumulate in the periplasm. The response is initiated by sequential cleavage of the membrane-spanning anti-sigma factor, RseA. RseB is an important negative regulator of envelope stress response that exerts its negative effects on sigma(E) activity through its binding to RseA. In this study, we analyze the interaction between RseA and RseB. We found that tight binding of RseB to RseA required intact RseB. Using programs that performed global and local sequence alignment of RseB and RseA, we found regions of high similarity and performed alanine substitution mutagenesis to test the hypothesis that these regions were functionally important. This protocol is based on the hypothesis that functionally dependent regions of two proteins co-evolve and therefore are likely to be sequentially conserved. This procedure allowed us to identify both an N-terminal and C-terminal region in RseB important for binding to RseA. We extensively analyzed the C-terminal region, which aligns with a region of RseA coincident with the major RseB binding determinant in RseA. Both allele-specific suppression analysis and cysteine-mediated disulfide bond formation indicated that this C-terminal region of similarity of RseA and RseB identifies a contact site between the two proteins. We suggest a similar protocol can be successfully applied to pairs of non-homologous but functionally linked proteins to find specific regions of the protein sequences that are important for establishing functional linkage.
引用
收藏
页码:5403 / 5413
页数:11
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