Peptide fraction from B. jararaca snake venom protects against oxidative stress-induced changes in neuronal PC12 cell but not in astrocyte-like C6 cell

Halyne Queiroz Pantaleão; Julio Cezar Araujo da Silva; Brenda Rufino da Silva; Marcela Bermudez Echeverry; Carlos Alberto-Silva

doi:10.1016/j.toxicon.2023.107178

Peptide fraction from B. jararaca snake venom protects against oxidative stress-induced changes in neuronal PC12 cell but not in astrocyte-like C6 cell

Toxicon. 2023 Aug 1:231:107178. doi: 10.1016/j.toxicon.2023.107178. Epub 2023 Jun 9.

Authors

Halyne Queiroz Pantaleão¹, Julio Cezar Araujo da Silva¹, Brenda Rufino da Silva¹, Marcela Bermudez Echeverry², Carlos Alberto-Silva³

Affiliations

¹ Natural and Humanities Sciences Center (CCNH), Experimental Morphophysiology Laboratory Federal University of ABC (UFABC), São Bernardo Do Campo, 09606-070, SP, Brazil.
² Center for Mathematics, Computation and Cognition (CMCC), UFABC, São Bernardo Do Campo, 09606-070, SP, Brazil.
³ Natural and Humanities Sciences Center (CCNH), Experimental Morphophysiology Laboratory Federal University of ABC (UFABC), São Bernardo Do Campo, 09606-070, SP, Brazil. Electronic address: carlos.asilva@ufabc.edu.br.

PMID: 37302421
DOI: 10.1016/j.toxicon.2023.107178

Abstract

Venom-derived proteins and peptides have prevented neuronal cell loss, damage, and death in the study of neurodegenerative disorders. The cytoprotective effects of the peptide fraction (PF) from Bothrops jararaca snake venom were evaluated against oxidative stress changes in neuronal PC12 cells and astrocyte-like C6 cells. PC12 and C6 cells were pre-treated for 4 h with different concentrations of PF, and then H₂O₂ was added (0.5 mM in PC12 cells; 0.4 mM in C6 cells) and incubated for 20 h more. In PC12 cells, PF at 0.78 μg mL^-1 increased viability (113.6 ± 6.3%) and metabolism (96.3 ± 10.3%) cell against H₂O₂-induced neurotoxicity (75.6 ± 5.8%; 66.5 ± 3.3%, respectively), reducing oxidative stress markers such as ROS generation, NO production, and arginase indirect activity through urea synthesis. Despite that, PF showed no cytoprotective effects in C6 cells, but potentiated the H₂O₂-induced damage at a concentration lower than 0.07 μg mL^-1. Furthermore, the role of metabolites derived from L-arginine metabolism was verified in PF-mediated neuroprotection in PC12 cells, using specific inhibitors of two of the key enzymes in the L-arginine metabolic pathway: the α-Methyl-DL-aspartic acid (MDLA) to argininosuccinate synthetase (AsS), responsible for the recycling of L-citrulline to L-arginine; and, L-N^Ω-Nitroarginine methyl ester (L-Name) to nitric oxide synthase (NOS), which catalyzes the synthesis of NO from L-arginine. The inhibition of AsS and NOS suppressed PF-mediated cytoprotection against oxidative stress, indicating that its mechanism is dependent on the production pathway of L-arginine metabolites such as NO and, more importantly, polyamines from ornithine metabolism, which are involved in the neuroprotection mechanism described in the literature. Overall, this work provides novel opportunities for evaluating whether the neuroprotective properties of PF shown in particular neuronal cells are sustained and for exploring potential drug development pathways for the treatment of neurodegenerative diseases.

Keywords: Argininosuccinate synthetase; Bioactive peptide; Bothrops jararaca; L-arginine metabolism; Neuroprotection; Polyamines.

MeSH terms

Animals
Arginine / metabolism
Arginine / pharmacology
Astrocytes / metabolism
Bothrops* / metabolism
Hydrogen Peroxide
Nitric Oxide Synthase / metabolism
Nitric Oxide Synthase / pharmacology
Oxidative Stress
PC12 Cells
Peptides / pharmacology
Rats
Snake Venoms / metabolism

Substances

Arginine
Hydrogen Peroxide
Nitric Oxide Synthase
Peptides
Snake Venoms