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Abstract 4146709: TMEM65 regulates NCLX-dependent mitochondrial calcium efflux to limit pathogenic mitochondrial calcium overload

医学 线粒体 细胞生物学 生物 内科学
作者
Joanne F. Garbincius,Oniel Salik,H Cohen,Carmen Choya-Foces,Adam Mangold,Angelina D Makhoul,Anna Schmidt,Dima Y. Khalil,Joshua J. Doolittle,Anya S. Wilkinson,Emma K. Murray,Michael P. Lazaropoulos,Alycia N. Hildebrand,Dhanendra Tomar,John W. Elrod
出处
期刊:Circulation [Ovid Technologies (Wolters Kluwer)]
卷期号:150 (Suppl_1)
标识
DOI:10.1161/circ.150.suppl_1.4146709
摘要

Introduction: Mitochondrial calcium ( m Ca 2+ ) exchange regulates energy metabolism, but if perturbed causes m Ca 2+ depletion and energy starvation or m Ca 2+ overload and cell death. The mitochondrial sodium (Na + )-calcium exchanger, NCLX, is critical for m Ca 2+ efflux in the heart, and animal models support NCLX as a therapeutic target to limit pathogenic m Ca 2+ overload. However, the mechanisms that regulate NCLX activity are largely unknown, representing a key barrier to translation. Goal: We used proximity biotinylation screening to identify the NCLX interactome and define novel regulators of NCLX function. Hypothesis: Our screen identified the mitochondrial inner membrane protein, TMEM65, as an NCLX-proximal protein that potently enhances Na + -dependent m Ca 2+ efflux. Therefore, we hypothesized that TMEM65 promotes m Ca 2+ efflux through NCLX. Approach: We measured m Ca 2+ exchange in AC16 cardiomyocytes with TMEM65 overexpression (OE) or CRISPR/Cas9 genetic disruption of TMEM65 to test its effect on m Ca 2+ efflux, and used pharmacologic inhibition and genetic knockout to determine TMEM65’s functional dependence on NCLX. We evaluated TMEM65’s impact on murine cardiac function in vivo using an AAV9-shRNA knockdown strategy. Results: Deletion of TMEM65 attenuated Na + -dependent m Ca 2+ efflux, while inhibition or deletion of NCLX ablated the increase in m Ca 2+ efflux observed with TMEM65 OE. Proximity ligation assay revealed co-localization of TMEM65 and NCLX in intact cells. In silico molecular modeling and co-fractionation of NCLX and TMEM65 via size-exclusion chromatography support their existence in a common macromolecular complex. Mutagenesis studies identified residues N163/D167 as critical to TMEM65 function, suggesting their importance to its cooperation with NCLX. TMEM65 expression decreased in human and murine heart failure, and Tmem65 KD in mice promoted myocardial m Ca 2+ overload and impaired cardiac function. Notably, TMEM65 OE mitigated necrotic cell death during cellular Ca 2+ -overload in vitro . Conclusions: Loss of TMEM65 function disrupts NCLX-dependent m Ca 2+ efflux, causing pathogenic m Ca 2+ overload, cell death and organ-level dysfunction, whereas gain of TMEM65 function can attenuate these effects. Our findings demonstrate the essential role of TMEM65 in maintaining m Ca 2+ efflux and suggest modulation of TMEM65 as a novel therapeutic strategy to control m Ca 2+ homeostasis in heart failure and other pathologies featuring dysregulated m Ca 2+ exchange.

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