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In vivo and in vitro mutants of FNR the anaerobic transcriptional regulator of E.coli
[摘要]

FNR regulates the expression of target genes in response to anaerobiosis. It resembles the catabolite gene activator or cAMP-receptor protein (CRP) except for the presence of an N-terminal cysteine cluster, which may form a redox-sensing iron-binding site. Site-directed mutagenesis has shown that 3 of the 4 cysteine residues in the N-terminal cluster (Cys-20, -23 and -29, but not Cys-16) and the only other cysteine residue (Cys-122), are essential for the normal activation and repression of PNR-dependent promoters. Deletion of residues Pro-3-Arg-9 (inclusive) had no effect, but FNR was inactivated by a frameshift extending through the C-terminal DNA-binding domain. Four independent in vivo mutants contained identical Gly-96→Asp substitutions, which may inactivate FNR by distorting a sharp turn between β-strands in the predicted structure.

[发布日期]  [发布机构] 
[效力级别]  [学科分类] 生物化学/生物物理
[关键词] FNR;Transcriptional regulation;Anaerobic gene expression;Cysteine residue;fnr mutant;Escherichia coli;CRP;cAMP receptor protein;PCR;polymerase chain reaction;SSB;single-stranded DNA binding protein [时效性] 
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