Literature DB >> 2497778

Transcriptional switching by the MerR protein: activation and repression mutants implicate distinct DNA and mercury(II) binding domains.

L M Shewchuk1, J D Helmann, W Ross, S J Park, A O Summers, C T Walsh.   

Abstract

Bacterial resistance to mercuric compounds is controlled by the MerR metalloregulatory protein. The MerR protein functions as both a transcriptional repressor and a mercuric ion dependent transcriptional activator. Chemical mutagenesis of the cloned merR structural gene has led to the identification of mutant proteins that are specifically deficient in transcriptional repression, activation, or both. Five mutant proteins have been overproduced, purified to homogeneity, and assayed for ability to dimerize, bind mer operator DNA, and bind mercuric ion. A mutation in the recognition helix of a proposed helix-turn-helix DNA binding motif (E22K) yields protein deficient in both activation and repression in vivo (a-r-) and deficient in operator binding in vitro. In contrast, mutations in three of the four MerR cysteine residues are repression competent but activation deficient (a-r+) in vivo. In vitro, the purified cysteine mutant proteins bind to the mer operator site with near wild-type affinity but are variably deficient in binding the in vivo inducer mercury(II) ion. A subset of the isolated proteins also appears compromised in their ability to form dimers at low protein concentrations. These data, taken with the results in the preceding paper (Shewchuk et al., 1989), support a model in which DNA-bound MerR dimer binds one mercuric ion and transmits this occupancy information to a protein region involved in transcriptional activation.

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Year:  1989        PMID: 2497778     DOI: 10.1021/bi00431a053

Source DB:  PubMed          Journal:  Biochemistry        ISSN: 0006-2960            Impact factor:   3.162


  18 in total

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Authors:  A O Summers
Journal:  J Bacteriol       Date:  1992-05       Impact factor: 3.490

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Journal:  Microbiol Rev       Date:  1992-03

3.  Ultrasensitivity and heavy-metal selectivity of the allosterically modulated MerR transcription complex.

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4.  Cd-specific mutants of mercury-sensing regulatory protein MerR, generated by directed evolution.

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5.  BrlR from Pseudomonas aeruginosa is a c-di-GMP-responsive transcription factor.

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6.  Cd(II)-responsive and constitutive mutants implicate a novel domain in MerR.

Authors:  J J Caguiat; A L Watson; A O Summers
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7.  Genetic analysis of transcriptional activation and repression in the Tn21 mer operon.

Authors:  W Ross; S J Park; A O Summers
Journal:  J Bacteriol       Date:  1989-07       Impact factor: 3.490

8.  Characterization of mutations that inactivate the diphtheria toxin repressor gene (dtxR).

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9.  Engineered single-chain, antiparallel, coiled coil mimics the MerR metal binding site.

Authors:  Lingyun Song; Jonathan Caguiat; Zhongrui Li; Jacob Shokes; Robert A Scott; Lynda Olliff; Anne O Summers
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10.  The major facilitator superfamily-type transporter YmfE and the multidrug-efflux activator Mta mediate bacillibactin secretion in Bacillus subtilis.

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Journal:  J Bacteriol       Date:  2008-05-23       Impact factor: 3.490

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