Active calcium mobilization from a thapsigargin-sensitive pool by free 32.5n6 in spermatids

Santiago Valtierra, Florencia Ximena; Peñalva, Daniel Alejandro; Luquez, Jessica Mariela; Aveldaño, Marta Isabel; Reyes, Juan Guillermo; Oresti, Gerardo Martin

info:eu-repo/semantics/publishedVersion

Fecha

2020

Registro en:

Active calcium mobilization from a thapsigargin-sensitive pool by free 32.5n6 in spermatids; LVI Annual Meeting Argentine Society for Biochemistry and Molecular Biology (SAIB); XV Annual Meeting Argentinean Society for General Microbiology (SAMIGE) ; Mendoza; Argentina; 2020; 1-7

0327-9545

http://hdl.handle.net/11336/156881

1667-5746

CONICET Digital

CONICET

https://repositorioslatinoamericanos.uchile.cl/handle/2250/4379989

Autor

Santiago Valtierra, Florencia Ximena

Peñalva, Daniel Alejandro

Luquez, Jessica Mariela

Aveldaño, Marta Isabel

Reyes, Juan Guillermo

Oresti, Gerardo Martin

Institución

Consejo Nacional de Investigaciones Científicas y Tecnológicas (Argentina)

Resumen

In their free form, long chain (C18–22) polyunsaturated fatty acids (PUFA), especially 20:4n−6, can modify calcium homeostasis in male germ cells. These cells also contain unusual n-6 very-long-chain (VLC) PUFA (28:4, 30:5, and 32:5), in non-hydroxy (n-V) and 2-hydroxy (h-V) forms, in their membrane sphingolipids. Potential biological roles of VLCPUFA, as free fatty acids (FFA), in the physiology of male germ cells are unknown. In this study we explored the ability of n-V FFA, and their h-V counterparts, to modify the intracellular calcium homeostasis in rat spermatids. After obtaining the n-V and h-V FFA from testicular sphingomyelin, their natural source, each group was separately added to spermatids suspensions at an 8 µM concentration. The n-V FFA increased the intracellular calcium concentration ([Ca2+]i) in spermatids several fold more intensely than did the h-V FFA. After isolating the components of n-V and h-V mixtures by HPLC to study the effect of each VLCPUFA, free n-32:5 was found to be the most active in increasing the [Ca2+]i, followed by n-30:5, while h-32:5 augmented it only slightly. In addition to fatty acid-specific, the response was dose-dependent. The rates of [Ca2+]i upsurge were independent of the presence of extracellular calcium. Pretreatment with thapsigargin inhibited the effect of n-32:5, suggesting that this FFA promotes the release of Ca2+ from intracellular calcium stores, mainly the endoplasmic reticulum. The n-V FFA did not seem to exert their effects through the G protein-coupled receptor GPR120, a putative receptor for free PUFA, as they occurred in the presence of a GPR120 inhibitor. Ceramides containing the same fatty acids did not modify [Ca2+]i, thus the observed [Ca2+]i increases may be attributed to the FFA themselves. The possibility that they occur after VLC-FFAs are converted into other bioactive compounds remains to be investigated. Our results revealed a biological activity of VLCPUFA that suggests a physiological role for these fatty acids. As VLCPUFA-mediated Ca2+ rises occurred in spermatids, they may activate Ca2+ signaling pathways with specific functional targets in germ cells differentiation.

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