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Cryopreservation of bovine semen using extract of Cinnamomum zeylanicum

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BACKGROUND: Antioxidants minimise oxidative stress and enhance sperm quality in the process of cryopreservation. OBJECTIVE: To assess the impact of Cinnamomum zeylanicum extract as an additive during the post-dilution and post-thaw stages of Murrah buffalo semen cryopreservation. MATERIALS AND METHODS: The semen sample was diluted using Tris-Egg-Yolk-Citric-Acid-Fructose-Glycerol extender and subsequently divided into three groups: Group 1, TEYCAFG without any additives or controls (C); Group 2, TEYCAFG fortified with a 50 μg/mL aqueous extract of cinnamon (T1); and Group 3, TEYCAFG fortified with a 50 μg/mL ethanolic extract of cinnamon (T2). The evaluation included an assessment of progressive motility, live spermatozoa, sperm abnormalities, HOST, CMPT, and enzyme leakage (GOT and GPT) at both the post-dilution and post-thaw stages. RESULTS: The groups that received cinnamon supplementation demonstrated statistically significant improvements (p<0.05) in various parameters, including an increase in the progressive motility, live spermatozoa, and HOS-positive spermatozoa, as well as greater distance traveled by vanguard spermatozoa compared to the control group. Furthermore, the cinnamon-added groups exhibited a significant decrease (p<0.05) in the percentage of sperm abnormalities and lower enzyme leakage (GOT and GPT) in post-thawed semen. CONCLUSION: Aqueous extract of C. zeylanicum at a concentration of 50 μg/mL provides superior protection of sperm structures and functions as compared to both the ethanolic extract of C. zeylanicum at the same concentration and the control group.
Title: Cryopreservation of bovine semen using extract of Cinnamomum zeylanicum
Description:
BACKGROUND: Antioxidants minimise oxidative stress and enhance sperm quality in the process of cryopreservation.
OBJECTIVE: To assess the impact of Cinnamomum zeylanicum extract as an additive during the post-dilution and post-thaw stages of Murrah buffalo semen cryopreservation.
MATERIALS AND METHODS: The semen sample was diluted using Tris-Egg-Yolk-Citric-Acid-Fructose-Glycerol extender and subsequently divided into three groups: Group 1, TEYCAFG without any additives or controls (C); Group 2, TEYCAFG fortified with a 50 μg/mL aqueous extract of cinnamon (T1); and Group 3, TEYCAFG fortified with a 50 μg/mL ethanolic extract of cinnamon (T2).
The evaluation included an assessment of progressive motility, live spermatozoa, sperm abnormalities, HOST, CMPT, and enzyme leakage (GOT and GPT) at both the post-dilution and post-thaw stages.
RESULTS: The groups that received cinnamon supplementation demonstrated statistically significant improvements (p<0.
05) in various parameters, including an increase in the progressive motility, live spermatozoa, and HOS-positive spermatozoa, as well as greater distance traveled by vanguard spermatozoa compared to the control group.
Furthermore, the cinnamon-added groups exhibited a significant decrease (p<0.
05) in the percentage of sperm abnormalities and lower enzyme leakage (GOT and GPT) in post-thawed semen.
CONCLUSION: Aqueous extract of C.
zeylanicum at a concentration of 50 μg/mL provides superior protection of sperm structures and functions as compared to both the ethanolic extract of C.
zeylanicum at the same concentration and the control group.

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