Investigating the role of neutral sphingomyelinases in membrane vesicle trafficking
von Dolma Choezom
Datum der mündl. Prüfung:2022-04-26
Erschienen:2022-07-21
Betreuer:Prof. Dr. Julia Groß
Gutachter:Prof. Dr. Michael Meinecke
Gutachter:Prof. Dr. Jörg Enderlein
Dateien
Name:PhD Dissertation+Dolma+Full+Version +Final.pdf
Size:7.36Mb
Format:PDF
Zusammenfassung
Englisch
Evidence collected over the years has established small extracellular vesicle (sEV) or exosome secretion as a novel paradigm for intercellular communication under both physiological and pathological conditions. SEVs are generated as intraluminal vesicles (ILVs) during multivesicular body (MVB) maturation in the endocytic pathway. Upon fusion of MVBs with the plasma membrane, ILVs are released into the extracellular space as sEVs. The molecular mechanisms that underlies ILV generation and the subsequent sorting of these secretory MVBs from the conventional degradative MVBs remain largely unraveled. Neutral sphingomyelinase 2 (nSMase2, encoded by SMPD3) activity drives intraluminal vesicle (ILV) generation for sEV secretion. In addition to its role in producing ceramide required for membrane invagination to form ILVs, here, we report that nSMase2 regulates sEV secretion through modulation of vacuolar H+ -ATPase (V-ATPase) activity. Specifically, we show that nSMase2 inhibition induces V-ATPase complex assembly that drives MVB lumen acidification and consequently reduces sEV secretion. Conversely, we demonstrate that stimulating nSMase2 activity with the inflammatory cytokine TNFα decreases acidification and increases sEV secretion. Thus, we unravel that nSMase2 activity affects MVB membrane lipid composition to counteract V-ATPase-mediated endosome acidification, and thereby shift MVB fate towards sEV secretion. The second part of this thesis focuses on neutral sphingomyelinase 1 (nSMase1, encoded by SMPD2), which also belongs to the sphingomyelinase enzyme family. The molecular characterization and biological function of nSMase1 remain poorly studied. Here, we show that SMPD2 knockdown (KD) reduces LAMP1 at the mRNA levels and is required for initiating a full-potential unfolded protein response under ER stress. Additionally, SMPD2 KD dramatically reduces the global protein translation rate. We further show that SMPD2 KD cells are arrested in the G1 phase of the cell cycle and that two important cell cycle regulating processes - PI3K/Akt pathway and Wnt signaling pathway are altered. Taken together, we propose a role for nSMase1 in buffering ER stress and modulating cellular fitness via cell cycle regulation.
Keywords: SMPD2; SMPD3; lipids; Cell Cycle; Wnt Signaling; Extracellular Vesicles