4.8 Article

PI(3,5)P2 controls membrane trafficking by direct activation of mucolipin Ca2+ release channels in the endolysosome

Journal

NATURE COMMUNICATIONS
Volume 1, Issue -, Pages -

Publisher

NATURE PUBLISHING GROUP
DOI: 10.1038/ncomms1037

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Funding

  1. Department of MCDB
  2. Biological Science Scholar Program
  3. University of Michigan
  4. NIH [NS062792, R01 GM50403]
  5. UM Initiative on Rare Disease Research
  6. Michigan Alzheimer's Disease Research Center
  7. National Multiple Sclerosis Society

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Membrane fusion and fission events in intracellular trafficking are controlled by both intraluminal Ca2+ release and phosphoinositide (PIP) signalling. However, the molecular identities of the Ca2+ release channels and the target proteins of PIPs are elusive. In this paper, by direct patch-clamping of the endolysosomal membrane, we report that PI(3,5)P-2, an endolysosome-specific PIP, binds and activates endolysosome-localized mucolipin transient receptor potential (TRPML) channels with specificity and potency. Both PI(3,5)P-2-deficient cells and cells that lack TRPML1 exhibited enlarged endolysosomes/vacuoles and trafficking defects in the late endocytic pathway. We find that the enlarged vacuole phenotype observed in PI(3,5)P-2-deficient mouse fibroblasts is suppressed by overexpression of TRPML1. Notably, this PI(3,5)P-2-dependent regulation of TRPML1 is evolutionarily conserved. In budding yeast, hyperosmotic stress induces Ca2+ release from the vacuole. In this study, we show that this release requires both PI(3,5)P-2 production and a yeast functional TRPML homologue. We propose that TRPMLs regulate membrane trafficking by transducing information regarding PI(3,5)P-2 levels into changes in juxtaorganellar Ca2+, thereby triggering membrane fusion/fission events.

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