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Cryopreservation alters the Ca<sup>2+</sup> flux of bovine spermatozoa
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1994
Year
BiologyAnimal PhysiologyInfertilityAnimal ReproductionFertilityPhysiologyFresh SpermatozoaGameteBovine SpermatozoaSemen AnalysisIntracellular Ca 2+Reproductive BiologyPublic HealthFertilisationHuman ReproductionReproductive Physiology
Capacitation and the acrosome reaction are Ca 2+ -dependent events that must be properly timed for successful fertilization to occur. To test the hypothesis that the cryopreservation procedures alter the ability of bovine spermatozoa to regulate Ca 2+ , the ability of Percoll-washed fresh and cryopreserved spermatozoa obtained from the same ejaculate (four ejaculates from each of six bulls) to regulate Ca 2+ over time was monitored using the fluorescent Ca 2+ chelator indo-1. The ability of spermatozoa to control Ca 2+ levels varied among ejaculates from a bull, and among bulls; these effects were statistically accounted for in the analysis of the effects of cryopreservation. Initially, cryopreserved spermatozoa had lower viability, motility, and normal acrosome scores and more intra- and extra-cellular Ca 2+ than fresh spermatozoa. Intra- and extra-cellular Ca 2+ was monitored for 150 min, with 1 mM exogenous Ca 2+ or buffer being added at 30 min to the spermatozoa being used to monitor intracellular Ca 2+ . By 30 min, extracellular Ca 2+ was higher for fresh cells and then remained constant. Intracellular Ca 2+ of fresh and cryopreserved spermatozoa in Ca 2+ -free media slowly increased. While both fresh and cryopreserved cells in Ca 2+ -supplemented media accumulated Ca 2+ more rapidly, cryopreserved spermatozoa did so faster than fresh. Post-experimental viability was lower in cryopreserved spermatozoa that had been exposed to exogenous Ca 2+ . In conclusion, cryopreservation affects initial intra- and extra-cellular Ca 2+ levels of bovine spermatozoa, and their ability to control subsequent rates of Ca 2+ accumulation. Key words: Bovine, cryopreservation, calcium, indo–1, spermatozoa