Molecular mechanisms of developmentally programmed crinophagy in Drosophila

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Abstract

At the onset of metamorphosis, Drosophila salivary gland cells undergo a burst of glue granule secretion to attach the forming pupa to a solid surface. Here, we show that excess granules evading exocytosis are degraded via direct fusion with lysosomes, a secretory granule-specific autophagic process known as crinophagy. We find that the tethering complex HOPS (homotypic fusion and protein sorting); the small GTPases Rab2, Rab7, and its effector, PLE KHM1; and a SNAP receptor complex consisting of Syntaxin 13, Snap29, and Vamp7 are all required for the fusion of secretory granules with lysosomes. Proper glue degradation within lysosomes also requires the Uvrag-containing Vps34 lipid kinase complex and the v-ATPase proton pump, whereas Atg genes involved in macroautophagy are dispensable for crinophagy. Our work establishes the molecular mechanism of developmentally programmed crinophagy in Drosophila and paves the way for analyzing this process in metazoans.

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CITATION STYLE

APA

Csizmadia, T., Lorincz, P., Hegedus, K., Széplaki, S., Low, P., & Juhász, G. (2018). Molecular mechanisms of developmentally programmed crinophagy in Drosophila. Journal of Cell Biology, 217(1), 361–374. https://doi.org/10.1083/jcb.201702145

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