The Yersinia pestis Effector YopM Inhibits Pyrin Inflammasome Activation.

dc.contributor.author

Ratner, Dmitry

dc.contributor.author

Orning, M Pontus A

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Proulx, Megan K

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Wang, Donghai

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Gavrilin, Mikhail A

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Wewers, Mark D

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Alnemri, Emad S

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Johnson, Peter F

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Lee, Bettina

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Mecsas, Joan

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Kayagaki, Nobuhiko

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Goguen, Jon D

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Lien, Egil

dc.date.accessioned

2019-06-01T14:45:40Z

dc.date.available

2019-06-01T14:45:40Z

dc.date.issued

2016-12-02

dc.date.updated

2019-06-01T14:45:38Z

dc.description.abstract

Type III secretion systems (T3SS) are central virulence factors for many pathogenic Gram-negative bacteria, and secreted T3SS effectors can block key aspects of host cell signaling. To counter this, innate immune responses can also sense some T3SS components to initiate anti-bacterial mechanisms. The Yersinia pestis T3SS is particularly effective and sophisticated in manipulating the production of pro-inflammatory cytokines IL-1β and IL-18, which are typically processed into their mature forms by active caspase-1 following inflammasome formation. Some effectors, like Y. pestis YopM, may block inflammasome activation. Here we show that YopM prevents Y. pestis induced activation of the Pyrin inflammasome induced by the RhoA-inhibiting effector YopE, which is a GTPase activating protein. YopM blocks YopE-induced Pyrin-mediated caspase-1 dependent IL-1β/IL-18 production and cell death. We also detected YopM in a complex with Pyrin and kinases RSK1 and PKN1, putative negative regulators of Pyrin. In contrast to wild-type mice, Pyrin deficient mice were also highly susceptible to an attenuated Y. pestis strain lacking YopM, emphasizing the importance of inhibition of Pyrin in vivo. A complex interplay between the Y. pestis T3SS and IL-1β/IL-18 production is evident, involving at least four inflammasome pathways. The secreted effector YopJ triggers caspase-8- dependent IL-1β activation, even when YopM is present. Additionally, the presence of the T3SS needle/translocon activates NLRP3 and NLRC4-dependent IL-1β generation, which is blocked by YopK, but not by YopM. Taken together, the data suggest YopM specificity for obstructing the Pyrin pathway, as the effector does not appear to block Y. pestis-induced NLRP3, NLRC4 or caspase-8 dependent caspase-1 processing. Thus, we identify Y. pestis YopM as a microbial inhibitor of the Pyrin inflammasome. The fact that so many of the Y. pestis T3SS components are participating in regulation of IL-1β/IL-18 release suggests that these effects are essential for maximal control of innate immunity during plague.

dc.identifier

PPATHOGENS-D-16-01946

dc.identifier.issn

1553-7366

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1553-7374

dc.identifier.uri

https://hdl.handle.net/10161/18595

dc.language

eng

dc.publisher

Public Library of Science (PLoS)

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PLoS pathogens

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10.1371/journal.ppat.1006035

dc.subject

Animals

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Mice, Knockout

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Mice

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Yersinia pestis

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Plague

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Disease Models, Animal

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Bacterial Outer Membrane Proteins

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Inflammasomes

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Pyrin

dc.title

The Yersinia pestis Effector YopM Inhibits Pyrin Inflammasome Activation.

dc.type

Journal article

pubs.begin-page

e1006035

pubs.issue

12

pubs.organisational-group

School of Medicine

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Duke

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Duke Cancer Institute

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Institutes and Centers

pubs.organisational-group

Immunology

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Basic Science Departments

pubs.organisational-group

Medicine, Rheumatology and Immunology

pubs.organisational-group

Medicine

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Clinical Science Departments

pubs.publication-status

Published

pubs.volume

12

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