Effect of exogenous lactoferrin and phosphoglycerate mutase 2 on the cryopreservation of wild ruminant epididymal/ejaculated sperm and testicular tissue

Julián Santiago-Moreno; Patricia Peris-Frau; Adolfo Toledano-Díaz; Cristina Castaño; Rosario Velázquez; Esther Alba; Félix Gómez-Guillamón; Leonor Camacho; Paloma Prieto; Belén Martínez-Madrid

doi:10.1016/j.cryobiol.2024.105182

Effect of exogenous lactoferrin and phosphoglycerate mutase 2 on the cryopreservation of wild ruminant epididymal/ejaculated sperm and testicular tissue

Cryobiology. 2024 Dec 1:118:105182. doi: 10.1016/j.cryobiol.2024.105182. Online ahead of print.

Affiliations

¹ Department of Animal Reproduction, National Institute for Agricultural and Food Research and Technology, Spanish Scientific Research Council (INIA-CSIC), Avda. Puerta de Hierro km5.9, Madrid, 28040, Spain. Electronic address: moreno@inia.csic.es.
² Department of Animal Reproduction, National Institute for Agricultural and Food Research and Technology, Spanish Scientific Research Council (INIA-CSIC), Avda. Puerta de Hierro km5.9, Madrid, 28040, Spain.
³ Programa de Vigilancia Epidemiológica de la Fauna Silvestre en Andalucía (PVE), Consejería de Sostenibilidad y Medio Ambiente, Junta de Andalucía, Málaga, Spain.
⁴ Consejería de Sostenibilidad y Medio Ambiente, Junta de Andalucía, Jaén, Spain.
⁵ Department of Animal Medicine and Surgery, Faculty of Veterinary Medicine, Complutense University of Madrid, Madrid, Spain.

PMID: 39608558
DOI: 10.1016/j.cryobiol.2024.105182

Abstract

Spermatozoa collected from the cauda epididymis of wild ruminants are more cryoresistant than are ejaculated spermatozoa. This work examines the effects of lactoferrin (LF) and phosphoglycerate mutase 2 (PGAM2), which are abundant in the epididymal sperm of wild ruminants, as additives in Iberian ibex and mouflon sperm extenders. In addition, LF was added to a vitrification medium to determine whether it also provided protection during the cryopreservation of testicular tissue. Epididymal sperm samples and testes were recovered post-mortem from ibexes (n = 13) and mouflons (n = 8) during the breeding season. Ejaculates were collected from both species (n = 10 each) using the transrectal ultrasound-guided massage technique. Four aliquots were taken from each sample, diluted in the appropriate freezing extender for each species, and subjected to the following treatments: control, LF (100 μg/ml), PGAM2 (25 μg/ml), and LF + PGAM2. Testicular tissue was cut into small pieces and cryopreserved by needle-immersed vitrification in a medium with or without LF. In vivo fertilization capacity was assessed using frozen-thawed ejaculated sperm from the ibexes. Supplementation of extenders with LF or PGAM2, and their combination, had no beneficial or harmful effect on any sperm variable after freezing-thawing. Artificial insemination of ibexes showed that the fertility rate in controls was 62.5 %, but this fell to 20 % in females inseminated with sperm treated with LF (p = 0.06), suggesting a putative negative effect of LF on fertility. The viability of elongated spermatids and spermatozoa from mouflon testes was greater (p < 0.05) in samples that were vitrified-warmed with LF. Thus, the hypothesis that supplementing ejaculated sperm with LF and/or PGAM2 improves sperm quality after freeze-thawing was not upheld. However, LF would seem an appropriate additive when vitrifying mouflon testicular tissue.

Keywords: Ibex; Lactoferrin; Mouflon; PGAM2; Sperm freezing; Testes vitrification.