The Influence of Three Commercial Soy Lecithin-Based Semen Extenders and Two Spermatozoa Concentrations on the Quality of Pre-Freeze and Post-Thaw Ram Epididymal Spermatozoa

Author:

Mujitaba Malam Abulbashar12ORCID,Kútvölgyi Gabriella3,Radnai Szentpáli Judit4,Debnár Viktória Johanna3,Tokár Alexandra5,Vass Nóra1,Bodó Szilárd3

Affiliation:

1. Department of Animal Nutrition and Physiology, Faculty of Agriculture and Food Sciences and Environmental Management, University of Debrecen, Böszörményi Street 138, H-4032 Debrecen, Hungary

2. Doctoral School of Animal Science, University of Debrecen, H-4032 Debrecen, Hungary

3. Department of Precision Livestock Farming and Animal Biotechnics, Institute of Animal Sciences, Hungarian University of Agriculture and Life Sciences, Kaposvár Campus, Guba Sándor Street 40, H-7400 Kaposvár, Hungary

4. Institute of Horticultural Science, Hungarian University of Agriculture and Life Sciences, Buda Campus, Villányi Street 29-43, H-1118 Budapest, Hungary

5. Festetics György Doctoral School, Hungarian University of Agriculture and Life Sciences, Deák Ferenc Street 16, H-8360 Keszthely, Hungary

Abstract

There are limited studies on the factors affecting the success of ram epididymal spermatozoa (REPS) cryopreservation. On this note, the current study assessed the influence of three commercial soy lecithin-based semen extenders, AndroMed® (AND), BioXcell® (BIO), and OviXcell® (OVI), and two concentrations (400 × 106 vs. 200 × 106 spermatozoa/mL) on the pre-freeze and post-thaw quality of REPS. The REPS were retrieved from nine adult rams’ testes and diluted with each of the three extenders to both concentrations. Straws were frozen manually. Standard motility (SMP) and kinematic parameters (KPs) were assessed via a CASA, while spermatozoa viability, morphology, and acrosomal integrity were assessed via the Kovács–Foote staining technique. The concentration did not significantly affect the pre-freeze and post-thaw SMP and KPs of REPS. BIO and OVI had significantly higher pre-freeze and post-thaw BCFs, post-thaw VAP, and the percentage of all intact heads than AND. In contrast, AND had a significantly lower percentage of REPS with tail defects than BIO and OVI. The 400 × 106 spermatozoa/mL concentration resulted in a significantly higher percentage of all intact heads than the 200 × 106 spermatozoa/mL concentration. Freezing significantly increased tail defects and decreased the percentage of REPS with distal cytoplasmic droplets. The cryopreservation of REPS at the 400 × 106 spermatozoa/mL concentration is recommended. All three extenders must be optimized to preserve the viability, membrane integrity, and better normal morphology of REPS; the reason for increased tail abnormality after the freezing/thawing process needs to be studied.

Funder

Stipendium Hungaricum Scholarship Program

Publisher

MDPI AG

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