Laparoscopic Ovum PickUp (LOPU) is the most reliable and efficient technique for collecting high quality oocytes from live animals in certain species or age groups, allowing its use for In Vitro Embryo Production (IVEP) and Somatic Cell Nuclear Transfer (SCNT). In order to maximize the number and quality of oocytes collected by donor, it is necessary to synchronize estrus and stimulate follicular growth using hormonal protocols that vary according to species. There are 2 big categories of applications for the LOPU-IVEP technology in production animals, those in which it acts as an alternative to MOET (competitive applications) and those in which it doesn't compete with MOET as it cannot be done in those categories (non competitive applications). In wild animals, LOPU can play an important role in conservation programs for endangered species when associated with effective IVEP and has been done in several species. It has commercial application in sheep, goats, cattle and buffaloes calves. Repeating LOPU procedures in the same female does not cause sequels with impact on the female's reproductive life, even when performed on prepubertal or wild animals.
We report heart murmur in Jaguars and Cougars found during reproductive procedures for semen and oocyte collection. Two male Cougars (n=2) and three female Jaguars (n=3) were examined. Anesthesia was performed with ketamine and medetomidine in males. Females also received propofol and were maintained with isoflurane. The animals were evaluated during anesthetic monitoring with multiparameter monitor alongside clinical examination, ambulatory electrocardiogram and echocardiogram. All animals presented mitral valve regurgitation under anesthesia, but without morphological changes in the cardiac structure or hemodynamic changes. Medetomidine may cause transitory heart murmur in healthy Jaguars and Cougars.
The cryopreservation of jaguar semen must be improved to produce high-quality biobanking doses. Until now, the rare studies of semen freezing in the species have only evaluated glycerol, always with a significant reduction in sperm quality in thawed semen. The purpose of this study was to assess the efficacy of three cryoprotectants, dimethylsulfoxide (DMSO), glycerol (GLY), and methanol (MET), in the cryopreservation of jaguar semen in an LDL-based extender, as well as the effect of thawing temperature on dosage quality. Five mature males with a history of reproduction were used. On the males, an infrared thermal image (IRT) was captured, the spicules and testes were analyzed, and the CASA system was used to evaluate the quality of fresh and thawed sperm. The superficial IRT was 4.6 ± 1.2 °C cooler than the anal sphincter, and the semen measured between 27.3 and 28.7 °C shortly after exiting the urethra. The total motility of fresh sperm was 55.3 ± 22.6%, and progressive motility was 36.3 ± 18%. The total motility of thawed sperm was 5.28 ± 2.51%, 4.49 ± %2.49, and 0.51 ± 0.62% for DMSO, GLY, and MET, respectively. DMSO and GLY performed better than MET, and there was no difference in thawing temperature (37°C 30 s vs. 50°C 12 s). All animals exhibit a considerable level of morphological changes in sperm. Low amounts of total and progressive motility were found in the thawed sperm. Males with a high level of sperm morphological changes were found to be fertile, but the lone male with normospermia was infertile. Thus, we contest the applicability of the commonly used morphological classification for bovines to felid species.
The aim of this study was to determine the effects of various abiotic factors, such as light, physical stress (pipetting) and thermal shock, on the quality of fresh and cooled equine sperm. In experiment I, four sperm aliquots were subjected to different light exposures: (i) protected control samples (CTRL), (ii) exposed to UV light at 10 cm (UV10), (iii) exposed to UV light at 20 cm (UV20) and (iv) exposed to laboratory lighting (LAB). In experiment II, four semen aliquots were subjected to repeated pipetting for 0, 10, 20 and 30 times (CTRL, P10, P20 and P30, respectively). In experiment III, four semen aliquots at 15°C were subjected to thermal oscillations: (i) cooled control sperm at 15°C (CTRL), (ii) oscillations of 1.9°C/min to a temperature of 30°C (T30), (iii) oscillations of 1.4°C/min, with the temperature rapidly falling until reaching 1.3°C (T0R) and (iv) oscillations of 1.1°C/min, with the temperature slowly falling until reaching 4.2°C (T0S). The results revealed that after 30 min, UV10 and UV20 sperm samples showed significantly (p < .05) lower total and progressive motility values, sperm kinematic parameters and mitochondrial potential. After 45 min of exposure, differences were highly significant (p < .001). No significant differences (p > .05) were found for pipetting or thermal oscillations. The results suggest that, even if equine sperm samples are not handled in the laboratory under optimal conditions, fresh and cooled equine spermatozoa are able to resist the impact of various abiotic stimuli without any reduction in their quality. This study analyses the effect on normospermic samples, but future research could look at the tolerance that asthenozoospermic equine samples have to these abiotic influences.
Brazilian rabbit breeding plays an important social role through family farming. However, one of the challenges faced is the need for new genetic material from genetically improved rabbits. The artificial insemination (AI) technique in Brazil is restricted to the use of fresh or chilled semen. Hence, this is the first report of the use of frozen semen and live kits in Brazil and probably in Latin America. The aims were to evaluate the commercial viability of frozen rabbit semen in Brazil, ranging from cryopreservation to insemination. Three bucks and three rabbit does of Flemish giant rabbits were used. Semen was collected, evaluated and diluted for freezing with CUNIFreeze. Semen was frozen in a 0.5 mL straw, thawed and then filled in a blue curve rabbit AI sheath with the doe in dorsal position with ovulation induced at the same time with buserelin acetate. The ejaculate volume was 0.8 ± 0.8 mL; the mass motility was 3.3 ± 0.6; and the total motility and vigor after dilution were 65% ± 5 points and 3.7 ± 0.6, respectively. Post-thawed, the motility and vigor were 20% ± 10 and 3,0 ± 0,0, respectively. The pregnancy rate was 66.6% with a litter sizes of 5 and 2 kits. Even with a lower result of litter size compared with refrigerated semen, this report brings a new scenario for rabbit breeding in Brazil, showing that frozen semen is a feasible technique for biobanking and mainly bringing the possibility of imported semen from genetically improved bucks solving inbreeding problems.
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