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Chaperone‐mediated reduction of RepA dimerization is associated with RepA conformational change
Author(s) -
Dibbens Justin A.,
Muraiso Kanae,
Chattoraj Dhruba K.
Publication year - 1997
Publication title -
molecular microbiology
Language(s) - English
Resource type - Journals
SCImago Journal Rank - 1.857
H-Index - 247
eISSN - 1365-2958
pISSN - 0950-382X
DOI - 10.1046/j.1365-2958.1997.5691920.x
Subject(s) - repressor , chaperone (clinical) , biology , mutant , plasma protein binding , binding site , psychological repression , plasmid , genetics , biochemistry , dna , gene , transcription factor , gene expression , medicine , pathology
RepA, the initiator protein of plasmid P1, binds to multiple sites (iterons) in the origin. The binding normally requires participation of chaperones, DnaJ, DnaK and GrpE. When purified, RepA appears dimeric and is inactive in iteron binding. On reaction with chaperones, a species active in iteron binding is formed and found to be monomeric. To test whether the chaperones can reduce dimerization, RepA was used to replace the dimerization domain of the λ repressor. The hybrid protein repressed the λ operator efficiently, indicating that RepA can dimerize in vivo . A further increase in repressor activity was seen in dnaJ mutant cells. These results are consistent with a chaperone‐mediated reduction of RepA dimerization. We also found that RepA mutants defective in dimerization still depend on DnaJ for iteron binding. Conversely, RepA mutants that no longer require chaperones for iteron binding remain dimerization proficient. These results indicate that the chaperone dependence of RepA activity is not solely owing to RepA dimerization. Our results are most simply explained by a chaperone‐mediated conformational change in RepA protomer that activates iteron binding. This conformational change also results in reduced RepA dimerization.