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Sperm motility in turbot,Scophthalmus marimus: initiation of movement and changes with time of swimming characteristics
Authors:Laurent Chauvaud  Jacky Cosson  Marc Suquet  Roland Billard
Institution:(1) laboratoire de Recherche Aquacole, IFREMER, BP 70, 29280 Plouzané, France;(2) Station Marine, CNRS, URA 671, 06230 Villefranche sur Mer, France;(3) Laboratoire d'Ichtyologie Générale et Appliquée, Muséum National d'Histoire Naturelle, 43 rue Cuvier, 75231 Paris, France
Abstract:Synopsis Turbot sperm motility is observed using dark field microscopy and stroboscopic illumination combined with video recording. Sperm motility is triggered by dilution of spermatozoa in sea water or in non ionic media (glucose or saccharose), presenting osmotic pressure ranging from 300 to 2100 mOsmol. The percentage of motile spermatozoa reaches 100% under conditions of osmotic pressure of 300 to 1100 mOsmol and pH close to 8.0. In full sea water, glucose or saccharose solutions an agglutination of spermatozoa is observed; this is prevented by addition of bovine serum albumin (5 mg ml–1). Immediately after transfer in activation solutions, 100% spermatozoa are motile in most samples freshly stripped. This percentage drops suddenly between 15 and 30% after 70 to 100 sec. The beat frequency remains at a constant value of 50 Hz during 40 s post activation and then drops suddenly between 15 and 30 Hz. The spermatozoa velocity is about 200 micrometers s–1 during 30 to 40 s and then declines to a stable value of 100 micrometers s–1 at 50 s post activation. After 1.20 mn, more and more spermatozoa become motionless. The minimum calculated and averaged distance covered during 1.20 min, is about 12 mm. The high performances of turbot spermatozoa motility are interpreted as a compensatory mechanism for the low sperm production.
Keywords:Sperm biology  Sperm movement  Sperm diluent  Marine fish
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