Effects of Hypoxia and Reoxygenation on Metabolic Profiles of Cardiomyocytes

Luis Daniel Montañez Condori; Cristofher Victor Vivas; Yan Borges Barreto; Ligia Ferreira Gomes; Adriano Mesquita Alencar; Antonio Carlos Bloise

doi:10.1007/s12013-024-01249-1

Effects of Hypoxia and Reoxygenation on Metabolic Profiles of Cardiomyocytes

Cell Biochem Biophys. 2024 Mar 18. doi: 10.1007/s12013-024-01249-1. Online ahead of print.

Authors

Luis Daniel Montañez Condori¹, Cristofher Victor Vivas¹, Yan Borges Barreto¹, Ligia Ferreira Gomes², Adriano Mesquita Alencar¹, Antonio Carlos Bloise³

Affiliations

¹ Universidade de Sao Paulo, Instituto de Fisica, Rua do Matao 1371, Sao Paulo, Brazil.
² Universidade de Sao Paulo, Instituto de Fisica, Rua do Matao 1371, Sao Paulo, Brazil. lfgomes@usp.br.
³ Universidade de Sao Paulo, Instituto de Fisica, Rua do Matao 1371, Sao Paulo, Brazil. acbloise@usp.br.

PMID: 38498099
DOI: 10.1007/s12013-024-01249-1

Abstract

In vitro cellular models provide valuable insights into the adaptive biochemical mechanisms triggered by cells to cope with the stress situation induced by hypoxia and reoxygenation cycles. The first biological data generated in studies based on this micrometric life-scale has the potential to provide us a global overview about the main biochemical phenomena presented in some reported preconditioning therapies in life-scale of higher dimensions. Thus, in this study, a cell incubator was designed and manufactured to produce a cellular model of heart hypoxia followed by reoxygenation (HfR) through consecutive repetitions of hypoxia-normoxia gas exchange. Samples of cellular extracts and culture media were obtained from non-proliferative cardiomyocytes (CMs) cultivated under challenging HfR (stressed CMs) and regular cultivation (unstressed CMs) in rounds of four days for each case. Metabolomic based on proton magnetic resonance spectroscopy (¹H-MRS) was used as an analytical approach to identify and quantify the metabolomes of these samples, the endo- and exo-metabolome. Despite the stressed CMs presented over 90% higher cellular death rate compared to the unstressed CMs, the metabolic profiles indicates that the surviving cells up-regulate their amino acid metabolism either by active protein degradation or by the consumption of culture media components to increase coenzyme A-dependent metabolic pathways. This cell auto-regulation mechanism could be well characterized in the first two days when the difference smears off under once the metabolomes become similar. The metabolic adaptations of stressed CMs identified the relevance of the cyclic oxidation/reduction reactions of nicotinamide adenine dinucleotide phosphate molecules, NADP⁺/NADPH, and the increased tricarboxylic acid cycle activity in an environment overloaded with such a powerful antioxidant agent to survive an extreme HfR challenge. Thus, the combination of cellular models based on CMs, investigative methods, such as metabolomic and ¹H-MRS, and the instrumental development of hypoxia incubator shown in this work were able to provide the first biochemical evidences behind therapies of gaseous exchanges paving the way to future assays.

Keywords: Cardiomyocytes; Hypoxia; Hypoxia followed by reoxygenation; Metabolomics; Normoxia; Proton magnetic resonance spectroscopy.