Literature DB >> 23684308

The Shigella OspC3 effector inhibits caspase-4, antagonizes inflammatory cell death, and promotes epithelial infection.

Taira Kobayashi1, Michinaga Ogawa2, Takahito Sanada1, Hitomi Mimuro3, Minsoo Kim4, Hiroshi Ashida4, Reiko Akakura2, Mitsutaka Yoshida5, Magdalena Kawalec6, Jean-Marc Reichhart6, Tsunehiro Mizushima7, Chihiro Sasakawa8.   

Abstract

Caspase-mediated inflammatory cell death acts as an intrinsic defense mechanism against infection. Bacterial pathogens deploy countermeasures against inflammatory cell death, but the mechanisms by which they do this remain largely unclear. In a screen for Shigella flexneri effectors that regulate cell death during infection, we discovered that Shigella infection induced acute inflammatory, caspase-4-dependent epithelial cell death, which is counteracted by the bacterial OspC3 effector. OspC3 interacts with the caspase-4-p19 subunit and inhibits its activation by preventing caspase-4-p19 and caspase-4-p10 heterodimerization by depositing the conserved OspC3 X1-Y-X₂-D-X₃ motif at the putative catalytic pocket of caspase-4. Infection of guinea pigs with a Shigella ospC3-deficient mutant resulted in enhanced inflammatory cell death and associated symptoms, correlating with decreased bacterial burdens. Salmonella Typhimurium and enteropathogenic Escherichia coli infection also induced caspase-4-dependent epithelial death. These findings highlight the importance of caspase-4-dependent innate immune responses and demonstrate that Shigella delivers a caspase-4-specific inhibitor to delay epithelial cell death and promote infection.
Copyright © 2013 Elsevier Inc. All rights reserved.

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Year:  2013        PMID: 23684308     DOI: 10.1016/j.chom.2013.04.012

Source DB:  PubMed          Journal:  Cell Host Microbe        ISSN: 1931-3128            Impact factor:   21.023


  76 in total

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Journal:  Curr Opin Microbiol       Date:  2013-12-22       Impact factor: 7.934

9.  Salmonella enterica Infection of Murine and Human Enteroid-Derived Monolayers Elicits Differential Activation of Epithelium-Intrinsic Inflammasomes.

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