Correlation between cytotoxicity induced by Pseudomonas aeruginosa clinical isolates from acute infections and IL-1ß secretion in a model of human THP-1 monocytes

Ahalieyah Anantharajah, Julien M. Buyck, Emmanuel Faure, Youri Glupczynski, Hector Rodriguez-Villalobos, Daniel De Vos, Jean Paul Pirnay, Florence Bilocq, Benǒit Guery, Paul M. Tulkens, Marie Paule Mingeot-Leclercq, Françoise Van Bambeke

    Résultats de recherche: Contribution à un journalArticleRevue par des pairs

    Résumé

    Type III secretion system (T3SS) in Pseudomonas aeruginosa is associated with poor clinical outcome in acute infections. T3SS allows for injection of bacterial exotoxins (e.g. ExoU or ExoS) into the host cell, causing cytotoxicity. It also activates the cytosolic NLRC4 inflammasome, activating caspase-1, inducing cytotoxicity and release of mature IL-1ß, which impairs bacterial clearance. In addition, flagellum-mediated motility has been suggested to also modulate inflammasome response and IL-1ß release. Yet the capacity of clinical isolates to induce IL-1ß release and its relation with cytotoxicity have never been investigated. Using 20 clinical isolates from acute infections with variable T3SS expression levels and human monocytes, our aim was to correlate IL-1ß release with toxin expression, flagellar motility and cytotoxicity. ExoU-producing isolates caused massive cell death but minimal release of IL-1ß, while those expressing T3SS but not ExoU (i.e. expressing ExoS or no toxins) induced caspase-1 activation and IL-1ß release, the level of which was correlated with cytotoxicity. Both effects were prevented by a specific caspase-1 inhibitor. Flagellar motility was not correlated with cytotoxicity or IL-1ß release. No apoptosis was detected. Thus, T3SS cytotoxicity is accompanied by a modification in cytokine balance for P. aeruginosa clinical isolates that do not express ExoU.

    langue originaleAnglais
    Numéro d'articleftv049
    journalPathogens and Disease
    Volume73
    Numéro de publication7
    Les DOIs
    étatPublié - oct. 2015

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