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首页> 外文期刊>Reproduction: The official journal of the Society for the Study of Fertility >Evaluation of motility, membrane status and DNA integrity of frozen–thawed bottlenose dolphin (Tursiops truncatus) spermatozoa after sex-sorting and recryopreservation
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Evaluation of motility, membrane status and DNA integrity of frozen–thawed bottlenose dolphin (Tursiops truncatus) spermatozoa after sex-sorting and recryopreservation

机译:进行性别分选和再冷冻保存后,对解冻的宽吻海豚(Tursiops truncatus)精子的活力,膜状态和DNA完整性进行评估

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Artificial insemination (AI) with sex-sorted frozen–thawed spermatozoa has led to enhanced management of ex situ bottlenose dolphin populations. Extended distance of animals from the sorting facility can be overcome by the use of frozen–thawed, sorted and recryopreserved spermatozoa. Although one bottlenose dolphin calf had been born using sexed frozen–thawed spermatozoa derived from frozen semen, a critical evaluation of in vitro sperm quality is needed to justify the routine use of such samples in AI programs. Sperm motility parameters and plasma membrane integrity were influenced by stage of the sex-sorting process, sperm type (non-sorted and sorted) and freezing method (straw and directional) ( P <0.05). After recryopreservation, sorted spermatozoa frozen with the directional freezing method maintained higher ( P <0.05) motility parameters over a 24-h incubation period compared to spermatozoa frozen using straws. Quality of sperm DNA of non-sorted spermatozoa, as assessed by the sperm chromatin structure assay (SCSA), was high and remained unchanged throughout freeze–thawing and incubation processes. Though a possible interaction between Hoechst 33342 and the SCSA-derived acridine orange was observed in stained and sorted samples, the proportion of sex-sorted, recryopreserved spermatozoa exhibiting denatured DNA was low (6.6±4.1%) at 6?h after the second thawing step and remained unchanged ( P >0.05) at 24?h. The viability of sorted spermatozoa was higher ( P <0.05) than that of non-sorted spermatozoa across all time points after recryopreservation. Collective results indicate that bottlenose dolphin spermatozoa undergoing cryopreservation, sorting and recryopreservation are of adequate quality for use in AI.
机译:按性别分类冷冻融化的精子的人工授精(AI)导致对异地宽吻海豚种群的管理得到加强。通过使用冷冻融化,分选和再冷冻保存的精子,可以克服动物离分选设施的距离过大的问题。尽管一只宽吻海豚犊牛出生时使用的是从冷冻精液中提取的经性冻融的精子,但仍需要对体外精子质量进行严格评估,以证明在AI程序中常规使用此类标本是合理的。精子运动参数和质膜完整性受性别分选过程的阶段,精子类型(未分选和分选)和冷冻方法(秸秆和定向)的影响(P <0.05)。冷冻保存后,与使用吸管冷冻的精子相比,定向冷冻法冷冻的精子在24小时的孵育期内保持较高的(P <0.05)活力参数。通过精子染色质结构测定(SCSA)评估,未分选精子的精子DNA质量很高,并且在整个冻融和孵育过程中保持不变。尽管在染色和分选的样品中观察到Hoechst 33342与SCSA衍生的a啶橙之间可能存在相互作用,但在第二次融化后6?h时,经性别分选,再冷冻保存的具有变性DNA的精子的比例较低(6.6±4.1%)。并在24?h保持不变(P> 0.05)。冷冻保存后的所有时间点,分类精子的活力均高于未分类精子的活力(P <0.05)。集体结果表明,进行低温保存,分选和再冷冻保存的宽吻海豚精子具有足够的质量,可用于AI。

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