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Mitochondrial dysfunction in human immunodeficiency virus‐1 transgenic mouse cardiac myocytes
25
Citations
36
References
2018
Year
The pathophysiology of human immunodeficiency virus (HIV)-associated cardiomyopathy remains uncertain. We used HIV-1 transgenic (Tg26) mice to explore mechanisms by which HIV-related proteins impacted on myocyte function. Compared to adult ventricular myocytes isolated from nontransgenic (wild type [WT]) littermates, Tg26 myocytes had similar mitochondrial membrane potential (ΔΨ <sub>m</sub> ) under normoxic conditions but lower Δ Ψ <sub>m</sub> after hypoxia/reoxygenation (H/R). In addition, Δ Ψ <sub>m</sub> in Tg26 myocytes failed to recover after Ca <sup>2+</sup> challenge. Functionally, mitochondrial Ca <sup>2+</sup> uptake was severely impaired in Tg26 myocytes. Basal and maximal oxygen consumption rates (OCR) were lower in normoxic Tg26 myocytes, and further reduced after H/R. Complex I subunit and ATP levels were lower in Tg26 hearts. Post-H/R, mitochondrial superoxide (O <sub>2</sub><sup>•-</sup> ) levels were higher in Tg26 compared to WT myocytes. Overexpression of B-cell lymphoma 2-associated athanogene 3 (BAG3) reduced O <sub>2</sub><sup>•-</sup> levels in hypoxic WT and Tg26 myocytes back to normal. Under normoxic conditions, single myocyte contraction dynamics were similar between WT and Tg26 myocytes. Post-H/R and in the presence of isoproterenol, myocyte contraction amplitudes were lower in Tg26 myocytes. BAG3 overexpression restored Tg26 myocyte contraction amplitudes to those measured in WT myocytes post-H/R. Coimmunoprecipitation experiments demonstrated physical association of BAG3 and the HIV protein Tat. We conclude: (a) Under basal conditions, mitochondrial Ca <sup>2+</sup> uptake, OCR, and ATP levels were lower in Tg26 myocytes; (b) post-H/R, Δ Ψ <sub>m</sub> was lower, mitochondrial O <sub>2</sub><sup>•-</sup> levels were higher, and contraction amplitudes were reduced in Tg26 myocytes; and (c) BAG3 overexpression decreased O <sub>2</sub><sup>•-</sup> levels and restored contraction amplitudes to normal in Tg26 myocytes post-H/R in the presence of isoproterenol.
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