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MT1-MMP is required for myeloid cell fusion via regulation of Rac1 signaling.

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dc.contributor.authorGonzalo, Pilar
dc.contributor.authorGuadamillas, Marta C
dc.contributor.authorHernández-Riquer, María Victoria
dc.contributor.authorPollán, Angela
dc.contributor.authorGrande-García, Araceli
dc.contributor.authorBartolomé, Rubén A
dc.contributor.authorVasanji, Amit
dc.contributor.authorAmbrogio, Chiara
dc.contributor.authorChiarle, Roberto
dc.contributor.authorTeixidó, Joaquín
dc.contributor.authorRisteli, Juha
dc.contributor.authorApte, Suneel S
dc.contributor.authordel Pozo, Miguel A
dc.contributor.authorArroyo, Alicia G
dc.contributor.funderMinisterio de Ciencia e Innovación (España)
dc.date.accessioned2026-01-26T11:06:19Z
dc.date.available2026-01-26T11:06:19Z
dc.date.issued2010-01-19
dc.description.abstractCell fusion is essential for fertilization, myotube formation, and inflammation. Macrophages fuse under various circumstances, but the molecular signals involved in the distinct steps of their fusion are not fully characterized. Using null mice and derived cells, we show that the protease MT1-MMP is necessary for macrophage fusion during osteoclast and giant-cell formation in vitro and in vivo. Specifically, MT1-MMP is required for lamellipodia formation and for proper cell morphology and motility of bone marrow myeloid progenitors prior to membrane fusion. These functions of MT1-MMP do not depend on MT1-MMP catalytic activity or downstream pro-MMP-2 activation. Instead, MT1-MMP null cells show a decreased Rac1 activity and reduced membrane targeting of Rac1 and the adaptor protein p130Cas. Retroviral rescue experiments and protein binding assays delineate a signaling pathway in which MT1-MMP, via its cytosolic tail, contributes to macrophage migration and fusion by regulating Rac1 activity through an association with p130Cas.
dc.description.peerreviewed
dc.description.tableofcontentsWe thank K. Tryggvason for the generation of MT1-MMP null mice, X. Bustelo for providing the Rac1 retroviral construct, J.C. Ramı´rez for help with retrovirus production, and S. Bartlett for editing. This work was supported by National Institutes of Health grant AR47074 (to S.S.A.), the Fundacio´ n Ramo´ n Areces and Spanish Fondo de Investigacio´ n Sanitaria grant RD06/0014/1016 (to A.G.A.), the Spanish Ministry of Science and Innovation through grants SAF2008-02100 to M.A.d.P. and SAF2008-02104 to A.G.A., and EUROHORCS (European Heads of Research Councils) and the European Science Foundation (ESF) through a EURYI (European Young Investigator) award to M.A.d.P. P.G. was funded by the Juan de la Cierva program and the Fondo de Investigacio´ n Sanitaria. M.C.G. and M.V.H.-R. are supported by fellowships BES-2006-13204 and 12790 from the Spanish Ministry of Science and Innovation, respectively. The CNIC is supported by the Spanish Ministry of Science and Innovation and the Pro-CNIC Foundation. J.R. is one of the inventors of the ICTP assay, but the royalty period has expired.
dc.format.number1
dc.format.page77-89
dc.format.volume18
dc.identifier.citationDev Cell. 2010 Jan 19;18(1):77-89.
dc.identifier.journalDevelopmental Cell
dc.identifier.pubmedID20152179
dc.identifier.urihttps://hdl.handle.net/20.500.12105/27179
dc.language.isoeng
dc.publisherCell Press
dc.relation.isreferencedbyPubMed
dc.relation.projectIDinfo:eu-repo/grantAgreement/ES/SAF2008-02100
dc.relation.projectIDinfo:eu-repo/grantAgreement/ES/SAF2008-02104
dc.relation.projectIDinfo:eu-repo/grantAgreement/ES/BES-2006-13204
dc.relation.publisherversionhttps://doi.org/10.1016/j.devcel.2009.11.012
dc.repisalud.institucionCNIC
dc.rights.accessRightsopen access
dc.rights.licenseAttribution-NonCommercial-NoDerivatives 4.0 Internationalen
dc.rights.urihttp://creativecommons.org/licenses/by-nc-nd/4.0/
dc.titleMT1-MMP is required for myeloid cell fusion via regulation of Rac1 signaling.
dc.typeresearch article
dc.type.hasVersionVoR
dspace.entity.typePublication

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