Lysosomal storage disease proteo/lipidomic profiling using nMOST links ferritinophagy with mitochondrial iron deficiencies in cells lacking NPC2

Author:

Kraus FelixORCID,He YuchenORCID,Swarup SharanORCID,Overmyer Katherine A.ORCID,Jiang Yizhi,Brenner JohannORCID,Capitanio CristinaORCID,Bieber AnnaORCID,Jen AnnieORCID,Nightingale Nicole M.ORCID,Anderson Benton J.ORCID,Lee ChanORCID,Paulo Joao A.ORCID,Smith Ian R.ORCID,Plitzko Jürgen M.,Schulman Brenda A.ORCID,Wilfling FlorianORCID,Coon Joshua J.ORCID,Harper J. WadeORCID

Abstract

SUMMARYLysosomal storage diseases (LSDs) comprised ∼50 monogenic diseases characterized by the accumulation of cellular material in lysosomes and associated defects in lysosomal function, but systematic molecular phenotyping is lacking. Here, we develop a nanoflow-based multi-omic single-shot technology (nMOST) workflow allowing simultaneously quantify HeLa cell proteomes and lipidomes from more than two dozen LSD mutants, revealing diverse molecular phenotypes. Defects in delivery of ferritin and its autophagic receptor NCOA4 to lysosomes (ferritinophagy) were pronounced in NPC2-/-cells, which correlated with increased lyso-phosphatidylcholine species and multi-lamellar membrane structures visualized by cryo-electron-tomography. Ferritinophagy defects correlated with loss of mitochondrial cristae, MICOS-complex components, and electron transport chain complexes rich in iron-sulfur cluster proteins. Strikingly, mitochondrial defects were alleviated when iron was provided through the transferrin system. This resource reveals how defects in lysosomal function can impact mitochondrial homeostasis in trans and highlights nMOST as a discovery tool for illuminating molecular phenotypes across LSDs.

Publisher

Cold Spring Harbor Laboratory

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