Defective lysosome reformation during autophagy causes skeletal muscle disease
Meagan J. McGrath, Matthew J. Eramo, Rajendra Gurung, Absorn Sriratana, Stefan M. Gehrig, Gordon S. Lynch, Sonia Raveena Lourdes, Frank Koentgen, Sandra J. Feeney, Michael Lazarou, Catriona A. McLean, Christina A. Mitchell
Meagan J. McGrath, Matthew J. Eramo, Rajendra Gurung, Absorn Sriratana, Stefan M. Gehrig, Gordon S. Lynch, Sonia Raveena Lourdes, Frank Koentgen, Sandra J. Feeney, Michael Lazarou, Catriona A. McLean, Christina A. Mitchell
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Research Article Cell biology Muscle biology

Defective lysosome reformation during autophagy causes skeletal muscle disease

Abstract

The regulation of autophagy-dependent lysosome homeostasis in vivo is unclear. We showed that the inositol polyphosphate 5-phosphatase INPP5K regulates autophagic lysosome reformation (ALR), a lysosome recycling pathway, in muscle. INPP5K hydrolyzes phosphatidylinositol-4,5-bisphosphate [PI(4,5)P2] to phosphatidylinositol 4-phosphate [PI(4)P], and INPP5K mutations cause muscular dystrophy by unknown mechanisms. We report that loss of INPP5K in muscle caused severe disease, autophagy inhibition, and lysosome depletion. Reduced PI(4,5)P2 turnover on autolysosomes in Inpp5k–/– muscle suppressed autophagy and lysosome repopulation via ALR inhibition. Defective ALR in Inpp5k–/– myoblasts was characterized by enlarged autolysosomes and the persistence of hyperextended reformation tubules, structures that participate in membrane recycling to form lysosomes. Reduced disengagement of the PI(4,5)P2 effector clathrin was observed on reformation tubules, which we propose interfered with ALR completion. Inhibition of PI(4,5)P2 synthesis or expression of WT INPP5K but not INPP5K disease mutants in INPP5K-depleted myoblasts restored lysosomal homeostasis. Therefore, bidirectional interconversion of PI(4)P/PI(4,5)P2 on autolysosomes was integral to lysosome replenishment and autophagy function in muscle. Activation of TFEB-dependent de novo lysosome biogenesis did not compensate for loss of ALR in Inpp5k–/– muscle, revealing a dependence on this lysosome recycling pathway. Therefore, in muscle, ALR is indispensable for lysosome homeostasis during autophagy and when defective is associated with muscular dystrophy.

Authors

Meagan J. McGrath, Matthew J. Eramo, Rajendra Gurung, Absorn Sriratana, Stefan M. Gehrig, Gordon S. Lynch, Sonia Raveena Lourdes, Frank Koentgen, Sandra J. Feeney, Michael Lazarou, Catriona A. McLean, Christina A. Mitchell

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Figure 1

Skeletal muscle–specific Inpp5k deletion leads to early-onset and progressive muscle disease.

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Skeletal muscle–specific Inpp5k deletion leads to early-onset and progre...
(A) H&E-stained muscle (quadriceps). Arrows: black = degenerating fibers; white = centralized nuclei; arrowhead = vacuolated fibers. n = 6 mice/genotype/age. Scale bar: 25 μm. (B) Serum creatine kinase, n = 5 mice/genotype (6 weeks), n = 5–6 mice/genotype (12 weeks), and n = 8 mice/genotype (1 year). ***P = 0.0008, ##P = 0.0065, †††P = 0.0005. (C) Specific (normalized) force: 12-week-old Inpp5kfl/fl (n = 5) and Inpp5kfl/fl MCK-Cre (n = 7) mice. Unpaired 2-tailed Student’s t test, ***P < 0.0001. (D) Transmission electron microscopy images of vacuoles in Inpp5kfl/fl MCK-Cre muscle (white arrows), n = 3 mice/genotype. Scale bar: 0.5 μm. White boxed region shown at high magnification in panels on right. (E) Muscle sections costained for LC3 and LAMP1. Arrows: LC3+/LAMP1+ autolysosomes, n = 3 mice/genotype. Scale bar: 12.5 μm. Yellow boxed region shown at high magnification below. Used for (F) quantification of lysosomes (LC3–/LAMP1+) versus autolysosomes (LC3+/LAMP1+), n = 3 mice/genotype. ***P < 0.0001, ###P < 0.0001. (G) Myoblasts were cultured in nutrient-free EBSS to activate starvation-induced autophagy and immunostained for autolysosomes (LC3+/LAMP1+), which are enlarged in INPP5K-KO (Inpp5kfl/fl Cre) but not control (Inpp5kfl/fl LacZ) cells (arrows). Yellow boxed region shown at high magnification in the panels on right. Scale bars: 20 μm. Unless otherwise stated, data presented in all graphs are the mean ± SEM, with a 2-way ANOVA followed by Bonferroni’s post hoc multiple-comparisons test to determine statistical significance.