ABSTRACT
The present study investigated the effects of chilled storage and cryopreservation on ide sperm motility and fertilizing capacity alongside the longevity of sperm movement. The parameters of motility (progressive motility-pMOT, curvilinear velocity-VCL and straightness-STR) have been recorded during 48â¯h of chilled storage (4⯰C) at 24-h intervals. The longevity of sperm movement was measured following activation for up to 120â¯s (in a range at 10-120â¯s) in freshly stripped and thawed sperm. A formerly established cryopreservation method was tested on ide sperm where motility parameters, hatching rate and larval malformation (according to 7 category groups) were investigated. Significant decrement of pMOT has already been observed after 24â¯h (6⯱â¯5%) compared to the freshly stripped sperm (49⯱â¯22%). pMOT and STR showed no significant changes for up to 120â¯s following activation in fresh sperm, whereas VCL showed significant difference between 10 (51⯱â¯11⯵m/s), 90 (33⯱â¯3⯵m/s) and 120 (31⯱â¯4⯵m/s) seconds as well as between 20 (48⯱â¯12⯵m/s), and 120â¯s. No negative effect of cryopreservation was recorded on pMOT (fresh: 49⯱â¯19%, cryopreserved: 22⯱â¯22%), VCL (fresh: 45⯱â¯9⯵m/s and cryopreserved: 57⯱â¯5⯵m/s), STR (fresh: 81⯱â¯3% and cryopreserved: 92⯱â¯1%) hatching rate (fresh: 22⯱â¯15%, cryopreserved: 33⯱â¯18%) or larval malformation (fresh: 12⯱â¯4%, cryopreserved: 12⯱â¯4%). No significant correlation was found between the three motility parameters and hatching rate. Cryopreservation had no effect on hatching and the prevalence of larval deformity. Furthermore craniofacial and eye deformities were characteristic in the group originating from fertilization with cryopreserved sperm, while edemas (pericardial, yolk) occurred more frequently in the control. The formerly developed cryopreservation protocol (method for cyprinids) was applicable to ide sperm.
