Solution structure of a paradigm ArsR family zinc sensor in the DNA-bound state

Arunkumar, A.I.; Campanello, Gregory C.; Giedroc, David P.

doi:10.1073/pnas.0905558106

Cited by 62 publications

(200 citation statements)

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“…Because all but the N-terminal residues of the TubR recognition helices are buried in the dimer interface, TubR must use a different mode of DNA binding than the ArsR or other HTH containing proteins (23). Examination of surface electrostatics of TubR reveals that one face of the protein is electronegative, whereas the other is strongly electropositive (Fig.…”

Section: Resultsmentioning

confidence: 99%

Plasmid protein TubR uses a distinct mode of HTH-DNA binding and recruits the prokaryotic tubulin homolog TubZ to effect DNA partition

Kumaraswami

et al. 2010

Proc. Natl. Acad. Sci. U.S.A.

101

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The segregation of plasmid DNA typically requires three elements: a DNA centromere site, an NTPase, and a centromere-binding protein. Because of their simplicity, plasmid partition systems represent tractable models to study the molecular basis of DNA segregation. Unlike eukaryotes, which utilize the GTPase tubulin to segregate DNA, the most common plasmid-encoded NTPases contain Walker-box and actin-like folds. Recently, a plasmid stability cassette on Bacillus thuringiensis pBtoxis encoding a putative FtsZ/tubulin-like NTPase called TubZ and DNA-binding protein called TubR has been described. How these proteins collaborate to impart plasmid stability, however, is unknown. Here we show that the TubR structure consists of an intertwined dimer with a winged helix-turn-helix (HTH) motif. Strikingly, however, the TubR recognition helices mediate dimerization, making canonical HTH-DNA interactions impossible. Mutagenesis data indicate that a basic patch, encompassing the two wing regions and the N termini of the recognition helices, mediates DNA binding, which indicates an unusual HTH-DNA interaction mode in which the N termini of the recognition helices insert into a single DNA groove and the wings into adjacent DNA grooves. The TubZ structure shows that it is as similar structurally to eukaryotic tubulin as it is to bacterial FtsZ. TubZ forms polymers with guanine nucleotide-binding characteristics and polymer dynamics similar to tubulin. Finally, we show that the exposed TubZ C-terminal region interacts with TubR-DNA, linking the TubR-bound pBtoxis to TubZ polymerization. The combined data suggest a mechanism for TubZ-polymer powered plasmid movement.

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Section: Resultsmentioning

confidence: 99%

Plasmid protein TubR uses a distinct mode of HTH-DNA binding and recruits the prokaryotic tubulin homolog TubZ to effect DNA partition

Kumaraswami

et al. 2010

Proc. Natl. Acad. Sci. U.S.A.

101

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“…Previous structural studies of ArsR/SmtB proteins largely focused on the role of metal-dependent conformational changes and not protein-DNA interaction, with one exception. NMR and mutagenesis probed residues in CzrA from Staphylococcus aureus for roles in binding to the palindromic 28-bp czr operator (28). This work suggests that CzrA interaction with target DNA increases protein motion in the allosteric sites and showed essential roles for residues analogous to Gln56, Ser57, Ser60, and Gln61 in DNA binding by CzrA, but did not reveal the details of protein-DNA contacts required for phosphate backbone interactions and/or base specificity.…”

Section: Discussionmentioning

confidence: 86%

“…Sequence and structural comparisons identify NolR as a member of the ArsR/SmtB family of transcription factors (26)(27)(28)(29). NolR shares 22-40% amino acid sequence identity with BigR, HlyU, CadC, CzrA, NmtR, and SmtB (Fig.…”

Section: Resultsmentioning

confidence: 99%

“…In the ArsR/SmtB proteins, metal binding triggers conformational changes that result in derepression of gene expression by driving repositioning of the helix-turn-helix DNA interaction motif (26)(27)(28)(29)(31)(32)(33). This movement results in a switch from a "closed" DNA-binding structure to an "open" low-affinity conformation of the homodimer.…”

Section: Discussionmentioning

confidence: 99%

“…S1). Unlike other ArsR/ SmtB transcription factors (26)(27)(28)(29)(31)(32)(33), no global structural Titrations were performed using 22-bp DNA duplexes.…”

Section: Discussionmentioning

confidence: 99%

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Structural basis for regulation of rhizobial nodulation and symbiosis gene expression by the regulatory protein NolR

Lee

Krishnan

Jez

2014

Proc. Natl. Acad. Sci. U.S.A.

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The symbiosis between rhizobial microbes and host plants involves the coordinated expression of multiple genes, which leads to nodule formation and nitrogen fixation. As part of the transcriptional machinery for nodulation and symbiosis across a range of Rhizobium, NolR serves as a global regulatory protein. Here, we present the X-ray crystal structures of NolR in the unliganded form and complexed with two different 22-base pair (bp) double-stranded operator sequences (oligos AT and AA). Structural and biochemical analysis of NolR reveals protein-DNA interactions with an asymmetric operator site and defines a mechanism for conformational switching of a key residue (Gln56) to accommodate variation in target DNA sequences from diverse rhizobial genes for nodulation and symbiosis. This conformational switching alters the energetic contributions to DNA binding without changes in affinity for the target sequence. Two possible models for the role of NolR in the regulation of different nodulation and symbiosis genes are proposed. To our knowledge, these studies provide the first structural insight on the regulation of genes involved in the agriculturally and ecologically important symbiosis of microbes and plants that leads to nodule formation and nitrogen fixation.transcription factor | protein structure T he symbiosis between rhizobial bacteria from the Rhizobium, Sinorhizobium, Mesorhizobium, Azorhizobium, and Bradyrhizobium genera and leguminous plants leads to the formation of root nodules (1, 2). These plant organs are specialized for nitrogen fixation and assimilation and are of major ecological and agricultural importance. For example, nitrogen-fixing nodules account for one quarter of total nitrogen fixed globally each year (3). The development of nitrogen-fixing nodules by rhizobia involves a variety of interactions between the plant and microbe; however, at the center of this process are a set of nod (nodulation) genes required for the synthesis of oligosaccharide-nodulation factors, for determining host-plant specificity, and for optimizing the efficiency of symbiosis (4-6). Successful interaction between the rhizobium and host plant requires expression of both positive and negative transcriptional control of genes related to nodulation and symbiosis (7,8

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Metal Specificity of Metallosensors

Higgins

Giedroc

2004

Encyclopedia of Inorganic and Bioinorganic Chemistry

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Transition metal ions are biologically required yet toxic when in excess. As such, prokaryotes have developed metal homeostasis systems that allow for the acquisition of essential metal ions, the delivery of these metal ions to target proteins, and the export of metal ions from the cell. Specialized metal‐binding proteins termed metallosensors bind to a cognate metal ion(s) in the cell and either transcriptionally repress the expression of importers or de‐repress the expression of exporters or sequestration systems and therefore govern cellular metal homeostasis. Metallosensors must be selective and appropriately sensitive toward the binding of their cognate metals. Prokaryotic metallosensors have been identified in ten different protein structural families. Each family exploits either one general metal‐binding‐site region, individual members of which have evolved different coordination sites, or alternatively, employs multiple metal‐binding sites to effect coordination of different metal ions. There is now broad support for the hypothesis that metal responsiveness in metallosensors is most closely linked to the coordination number and geometry adopted by cognate metal ion(s), and this is the subject of this article. Since a range of metal ions can be collectively sensed by a single repressor family, a particular protein fold cannot be specific for one particular metal ion. In fact, the converse is true: nature has used convergent evolution to evolve metal‐specific sensors on a variety of structural scaffolds that exploit common principles of coordination chemistry (ligand type, coordination number, and geometry) to effect the same biological outcome.

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Solution structure of a paradigm ArsR family zinc sensor in the DNA-bound state

Cited by 62 publications

References 42 publications

Plasmid protein TubR uses a distinct mode of HTH-DNA binding and recruits the prokaryotic tubulin homolog TubZ to effect DNA partition

Plasmid protein TubR uses a distinct mode of HTH-DNA binding and recruits the prokaryotic tubulin homolog TubZ to effect DNA partition

Structural basis for regulation of rhizobial nodulation and symbiosis gene expression by the regulatory protein NolR

Metal Specificity of Metallosensors

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