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Evaluation of Extenders for Cryopreservation of Cirrhinus mrigala Milt

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This study aimed to evaluate the performance of different extenders for the cryopreservation of Cirrhinus mrigala milt. The extenders under investigation included Kurokura-2 + DMSO (KD), Alsever`s solution + DMSO (AD), Kurokura-2 + Methanol (KM), and Alsever`s solution + Methanol (AM). Sperm quality assessments encompassed critical parameters such as sperm motility, motility duration, viability, and DNA integrity. The initial analysis of fresh milt revealed motility rate of 88.33±1.66%, pH of 7.52±0.76, a volume of 7.83±0.44 mL, a sperm count of 3.55±0.40 x 1010/mL. Upon thawing, it became evident that the KD extender yielded significantly higher post-thaw sperm motility (%) at 68±1.67, compared to the KM (40.00±2.89), AD (38±1.67), and AM (41.67±4.40). Additionally, sperm motility duration (seconds) exhibited a notable increase in the KD extender (78.67±10.413) in comparison to the KM (52.00±5.291), AD (46.66±1.66), and AM (41.67±1.667) extenders. The KD extender also contributed to higher sperm viability (%) at 66.00±1.00, whereas KM and AM exhibited similar values at 59.00±3.00 and 55.33±6.38, respectively. Furthermore, DNA integrity (%) remained consistently high for KD, KM, and AM (98.67±0.66, 98.00±1.52%, and 97.33±1.20%), while a lower percentage was observed for AD (88.00±1.15). In conclusion, the modified Kurokura extender, supplemented with 10% DMSO, showcased a pronounced positive impact on the cryopreservation of Cirrhinus mrigala milt.
Title: Evaluation of Extenders for Cryopreservation of Cirrhinus mrigala Milt
Description:
This study aimed to evaluate the performance of different extenders for the cryopreservation of Cirrhinus mrigala milt.
The extenders under investigation included Kurokura-2 + DMSO (KD), Alsever`s solution + DMSO (AD), Kurokura-2 + Methanol (KM), and Alsever`s solution + Methanol (AM).
Sperm quality assessments encompassed critical parameters such as sperm motility, motility duration, viability, and DNA integrity.
The initial analysis of fresh milt revealed motility rate of 88.
33±1.
66%, pH of 7.
52±0.
76, a volume of 7.
83±0.
44 mL, a sperm count of 3.
55±0.
40 x 1010/mL.
Upon thawing, it became evident that the KD extender yielded significantly higher post-thaw sperm motility (%) at 68±1.
67, compared to the KM (40.
00±2.
89), AD (38±1.
67), and AM (41.
67±4.
40).
Additionally, sperm motility duration (seconds) exhibited a notable increase in the KD extender (78.
67±10.
413) in comparison to the KM (52.
00±5.
291), AD (46.
66±1.
66), and AM (41.
67±1.
667) extenders.
The KD extender also contributed to higher sperm viability (%) at 66.
00±1.
00, whereas KM and AM exhibited similar values at 59.
00±3.
00 and 55.
33±6.
38, respectively.
Furthermore, DNA integrity (%) remained consistently high for KD, KM, and AM (98.
67±0.
66, 98.
00±1.
52%, and 97.
33±1.
20%), while a lower percentage was observed for AD (88.
00±1.
15).
In conclusion, the modified Kurokura extender, supplemented with 10% DMSO, showcased a pronounced positive impact on the cryopreservation of Cirrhinus mrigala milt.

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