Effect of centrifugation on in vitro survival of fresh diluted canine spermatozoa
2002; Elsevier BV; Volume: 57; Issue: 6 Linguagem: Inglês
10.1016/s0093-691x(02)00663-5
ISSN1879-3231
AutoresTom Rijsselaere, Ann Van Soom, Dominiek Maes, Aart de Kruif,
Tópico(s)Male Reproductive Health Studies
ResumoProstatic fluid is unsuitable for preserving dog semen at 4 °C and exerts harmful effects upon the spermatozoa during the freezing process. Centrifugation immediately after sperm collection is a common method to remove prostatic admixture. In the present study, dog semen, diluted to 25×106/ml, was exposed for 5 min to four different centrifugation speeds (180×g, 720×g, 1620×g and 2880×g) to determine subsequent sperm losses in the supernatant and to assess sperm survival over time. Using 180×g as centrifugation speed, 8.9% of the sperm cells was lost upon supernatant removal. Using 720×g, 1620×g or 2880×g, sperm losses were lower, 2.3, 0.4 and 0.006%, respectively. After centrifugation, the sperm pellet was rediluted in egg–yolk–Tris extender, cooled and stored for 3 days at 4 °C. Motility, progressive motility, membrane integrity and sperm morphology were assessed daily. Acrosomal status was assessed after 3 days of storage. The only functional parameter which was influenced by centrifugation speed was membrane integrity as evaluated by means of SYBR14-PI staining: significantly more dead and moribund sperm cells were found after centrifugation at 1620×g and 2880×g after 48 and 72 h of storage at 4 °C. When higher initial sperm concentrations (50×106, 75×106 or 100×106/ml) were evaluated for sperm losses, less than 2.3% of the initial total sperm cells was lost at lower centrifugation speeds. We conclude that centrifuging dog sperm for 5 min at 720×g is the best strategy to remove prostatic fluid because the loss of sperm cells is acceptable and the functional parameters of the spermatozoa are well preserved, even after 3 days of storage.
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