The transcriptional regulator LrpA from the hyperthermophilic archaeon Pyrococcus furiosus is negatively autoregulated

The archaeal transcriptional initiation machinery closely resembles core elements of the eukaryal polymerase II system. However, apart from the established basal archaeal transcription system, little is known about the modulation of gene expression in archaea. At present, no obvious eukaryal-like tr...

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Bibliographic Details
Published in:The Journal of biological chemistry 2000, Vol.275
Main Authors: Brinkman, A.B, Dahlke, I, Tuininga, J.E, Lammers, T, Dumay, V, Heus, E., de, Lebbink, J.H.G, Thomm, M, Vos, W.M., de, Oost, J., van der
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Laboratorium voor Microbiologie
Microbiological Laboratory
Microbiologie
Microbiology
VLAG
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Summary:The archaeal transcriptional initiation machinery closely resembles core elements of the eukaryal polymerase II system. However, apart from the established basal archaeal transcription system, little is known about the modulation of gene expression in archaea. At present, no obvious eukaryal-like transcriptional regulators have been identified in archaea. Instead, we have previously isolated an archaeal gene, the Pyrococcus furiosus lrpA, that potentially encodes a bacterial-like transcriptional regulator. In the present study, we have for the first time addressed the actual involvement of an archaeal Lrp homologue in transcription modulation. For that purpose, we have produced LrpA in Escherichia coli. In a cell-free P. furiosus transcription system we used wild-type and mutated lrpA promoter fragments to demonstrate that the purified LrpA negatively regulates its own transcription. In addition, gel retardation analyses revealed a single protein-DNA complex, in which LrpA appeared to be present in (at least) a tetrameric conformation. The location of the LrpA binding site was further identified by DNaseI and hydroxyl radical footprinting, indicating that LrpA binds to a 46-base pair sequence that overlaps the transcriptional start site of its own promoter. The molecular basis of the transcription inhibition by LrpA is discussed.
ISSN:0021-9258
1083-351X