Trpml controls actomyosin contractility and couples migration to phagocytosis in fly macrophages
Author
dc.contributor.author
Edwards Jorquera, Sandra
Author
dc.contributor.author
Bosveld, Floris
Author
dc.contributor.author
Bellaiche, Yohanns
Author
dc.contributor.author
Lennon Dumenil, Ana María
Author
dc.contributor.author
Glavic Maurer, Álvaro
Admission date
dc.date.accessioned
2020-05-27T13:46:23Z
Available date
dc.date.available
2020-05-27T13:46:23Z
Publication date
dc.date.issued
2020
Cita de ítem
dc.identifier.citation
J. Cell Biol. 2020 e201905228
es_ES
Identifier
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10.1083/jcb.201905228
Identifier
dc.identifier.uri
https://repositorio.uchile.cl/handle/2250/175004
Abstract
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Phagocytes use their actomyosin cytoskeleton to migrate as well as to probe their environment by phagocytosis or macropinocytosis. Although migration and extracellular material uptake have been shown to be coupled in some immune cells, the mechanisms involved in such coupling are largely unknown. By combining time-lapse imaging with genetics, we here identify the lysosomal Ca2+ channel Trpml as an essential player in the coupling of cell locomotion and phagocytosis in hemocytes, the Drosophila macrophage-like immune cells. Trpml is needed for both hemocyte migration and phagocytic processing at distinct subcellular localizations: Trpml regulates hemocyte migration by controlling actomyosin contractility at the cell rear, whereas its role in phagocytic processing lies near the phagocytic cup in a myosin-independent fashion. We further highlight that Vamp7 also regulates phagocytic processing and locomotion but uses pathways distinct from those of Trpml. Our results suggest that multiple mechanisms may have emerged during evolution to couple phagocytic processing to cell migration and facilitate space exploration by immune cells.
es_ES
Patrocinador
dc.description.sponsorship
Chilean grants
Fondap 15090007
Conicyt Act
1401
Conicyt PCI REDES
14004
Comision Nacional de Investigacion Cientifica y Tecnologica (CONICYT)
140289
French funding Labex DCBIOL