Please use this identifier to cite or link to this item: http://hdl.handle.net/20.500.11889/4095
Title: Analysis of HmsH and its role in plague biofilm formation
Authors: Abu Khweek, Arwa
Fetherston, Jacqueline D.
Perry, Robert D.
Keywords: Membrane proteins - Analysis
Yersinia pestis
Issue Date: 2010
Abstract: The Yersinia pestis Hms+ phenotype is a manifestation of biofilm formation that causes adsorption of Congo red and haemin at 26 °C but not at 37 °C. This phenotype is required for blockage of the proventricular valve of the oriental rat flea and plays a role in transmission of bubonic plague from fleas to mammals. Genes responsible for this phenotype are located in three separate operons, hmsHFRS, hmsT and hmsP. HmsH and HmsF are outer membrane (OM) proteins, while the other four Hms proteins are located in the inner membrane. According to the Hidden Markov Method-based predictor, HmsH has a large N terminus in the periplasm, a β-barrel structure with 16 β-strands that traverse the OM, eight surface-exposed loops, and seven short turns connecting the β-strands on the periplasmic side. Here, we demonstrate that HmsH is a heat-modifiable protein, a characteristic of other β-barrel proteins, thereby supporting the bioinformatics analysis. Alanine scanning mutagenesis was used to identify conserved amino acids in the HmsH-like family that are critical for the function of HmsH in biofilm formation. Of 23 conserved amino acids mutated, four residues affected HmsH function and three likely caused protein instability. We used formaldehyde cross-linking to demonstrate that HmsH interacts with HmsF but not with HmsR, HmsS, HmsT or HmsP. Loss-of-function HmsH variants with single alanine substitutions retained their β-structure and interaction with HmsF. Finally, using a polar hmsH : : mini-kan mutant, we demonstrated that biofilm development is not important for the pathogenesis of bubonic or pneumonic plague in mice.
URI: http://hdl.handle.net/20.500.11889/4095
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