Please use this identifier to cite or link to this item: https://hdl.handle.net/11499/7690
Title: Esterified glucomannan improves aflatoxin-induced damage of sperm parameters during liquid storage of ram semen at 5°C
Authors: Ataman, M.B.
Bucak, M.N.
Çoyan, K.
Keywords: Aflatoxin
Glucomannan
Liquid storage
Ram semen
aflatoxin
mannan
(1-6)-alpha-glucomannan
protective agent
animal cell
animal experiment
animal food
article
cell viability
cold acclimatization
controlled study
ejaculation
evolutionary adaptation
food composition
male
nonhuman
priority journal
semen analysis
sperm preservation
spermatozoon
spermatozoon motility
temperature sensitivity
animal
cold
cytology
domestic sheep
drug effects
physiology
procedures
sperm
veterinary
Animalia
Aflatoxins
Animal Feed
Animals
Cold Temperature
Male
Mannans
Protective Agents
Semen
Semen Preservation
Sheep, Domestic
Sperm Motility
Spermatozoa
Publisher: Academic Press Inc.
Abstract: The aim of the present work was to study the effects of aflatoxin (AF) on sperm parameters in rams, and to determine the protective efficiency of esterified glucomannan (EG) co-administered with AF up to 96. h of the liquid storage of ram semen at 5. °C. Thirty-two Merino rams (12-14. months old) were used. The animals were examined for their general health status. To ensure their adaptation to the environment and the new feeding regimen, a 15-day acclimatization programme was applied to the animals, prior to the start of the study. Experimental feeding was continued for ninety-two days. The experimental design consisted of four dietary treatments. The control group (C) was fed with commercial feed. The AF group was fed with commercial feed plus 250. µg/day of total AF. The EG group received commercial feed plus 2. g/day of EG. The AF + EG group was given commercial feed plus 250. µg/day of total AF and 2. g/day of EG. In the study, ejaculates were obtained from rams twice a week for 12. weeks, using an electro-ejaculator. After collected, the ejaculates were diluted with a skimmed milk extender, and stored at 5. °C. Sperm motility and rates of abnormal and nonviable spermatozoa were determined for the different treatment groups at 5. °C at 0, 24, 48, 72 and 96. h of liquid storage.During the first two weeks of the trial, the groups did not statistically differ from each other for sperm motility or rates of abnormal and nonviable spermatozoa at 0, 24, 48 and 96. h of storage. As from the third week, the short-term storage of semen produced statistically significant differences between the AF group and the other treatment groups for sperm parameters (p<. 0.05). The administration of aflatoxin was observed to have reduced sperm motility and to have increased the rates of abnormal and nonviable spermatozoa in comparison to the control group (p<. 0.05), while EG co-administered with AF was determined to have ameliorated the adverse effects of AF on sperm parameters, and this ameliorative effect continued throughout the short-term storage of semen. On the other hand, aflatoxin administration resulted in the deterioration of the sperm parameters in the following weeks, and the combined administration of EG + AF reversed this adverse effect, thus, bringing the sperm parameters closer to the values of the control group. This study demonstrated that, in rams, AF adversely affected sperm, biochemical and testis parameters, and that the combined administration of EG and AF reversibly improved these adverse effects. © 2014 Elsevier Inc.
URI: https://hdl.handle.net/11499/7690
https://doi.org/10.1016/j.cryobiol.2014.03.007
ISSN: 0011-2240
Appears in Collections:PubMed İndeksli Yayınlar Koleksiyonu / PubMed Indexed Publications Collection
Scopus İndeksli Yayınlar Koleksiyonu / Scopus Indexed Publications Collection
Tıp Fakültesi Koleksiyonu
WoS İndeksli Yayınlar Koleksiyonu / WoS Indexed Publications Collection

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