Effects of chelating calcium in cryopreservation extender on frozen-thawed dog semen

Author:

Deco-Souza T.1ORCID,Paula T.A.R.1ORCID,Araujo G.R.1ORCID,Bergo L.C.F.1ORCID,Carazo L.R.B.1ORCID,Vasconcelos G.S.C.1ORCID,Silva M.C.C.2ORCID

Affiliation:

1. Universidade Federal de Viçosa, Brazil

2. UFMS, Brazil

Abstract

ABSTRACT We evaluated the effect of reducing free calcium in the cryopreservation medium, using the calcium chelator ethylene diamine tetracetic acid (EDTA) at 0.3% and 0.5% concentrations. Three male mixed breed dogs were subjected to semen collection by digital manipulation (n=16). Each ejaculate was divided in three aliquots, and each one was diluted in TRIS-glucose-egg yolk extender with 6% glycerol and 0.5% Equex STM Paste® (TGE, control); and added with 0.3% EDTA (EDTA 0.3) or 0.5% EDTA (EDTA 0.5). Calcium concentration reduced in EDTA 0.3 and all the calcium ions were chelated in EDTA 0.5. The EDTA addition did not affect sperm morphology or plasma membrane integrity; however, by removing all free calcium (EDTA 0.5), the sperm motility reduced (64.7% in TGE and 45% in EDTA 0.5; p<0.05). Acrosome integrity and sperm binding ability were not improved by calcium chelation. The failure to prevent the premature AR may explain why sperm longevity was not affected by calcium removal. Thus, the partial or complete calcium removal, through EDTA addition, is not able to prevent acrosomal damage or premature acrosomal reaction, and therefore does not improve the dog sperm binding ability.

Publisher

FapUNIFESP (SciELO)

Subject

General Veterinary

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