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Post-thaw viability of bull AI-doses with low-sperm numbers

机译:具有低精子数量的公牛AI剂量解冻后的生存力

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Use of AI-doses containing low-sperm numbers are increasingly been used to optimise use of elite bulls as well as to accommodate an eventual wider application of sex-sorted semen. Since spermatozoa might, however, suffer from high extension rates, thus compromising fertility, this study evaluated the post-thaw sperm quality of semen from commercial progeny-tested, high-ranked AI-sires whose semen was within acceptable limits of normality, frozen in a split-design to 15 (control, 15M) or 2 x 10(6) total spermatozoa (treatment, 2M) per straw. Assessment post-thaw included computer-evaluated sperm motility (CASA), membrane integrity (SYBR-14/PI), membrane stability (Annexin-V/PI), acrosome integrity (Carboxy-SNARF-1/PI/FITC-PSA), and chromatin integrity (AO of in situ acid-induced DNA denaturation). High extension did not affect the proportions of linearly motile spermatozoa, of membrane integrity or stability nor chromatin integrity, immediately post-thaw. However, high extension clearly affected linear sperm motility following incubation at 38 degrees C for 30 min, sperm viability when assessed by SNARF and, particularly, acrosome integrity of the otherwise viable spermatozoa. Individual sire variation was evident. Fertility was preliminarily evaluated for one of the less affected bulls in a blind field trial. A total of 109 dairy cows were randomly inseminated with 15M or 2M-straws without differences in pregnancy rate between them (47% versus 43%). This similarity in fertility rates, confirmed the in vitro methods used were appropriate for identifying cryosurvival and further suggested the site of sperm deposition was not crucial for the fertility of low-sperm AI-numbers for this particular sire. However, the inter-bull variation seen calls for caution when cryopreserving low concentrations of bull spermatozoa with conventional freezing protocols.
机译:越来越多地使用含有低精子数量的AI剂量来优化公牛的使用,并最终适应更广泛的按性别分类的精液。但是,由于精子可能具有较高的延伸率,从而损害了生育能力,因此本研究评估了经商业后代测试的高级AI父级精液的精液解冻后精子质量,其精液在正常范围内,并冷冻。每个稻草的拆分设计为15个(对照,15M)或2 x 10(6)个总精子(处理,2M)。解冻后的评估包括计算机评估的精子活力(CASA),膜完整性(SYBR-14 / PI),膜稳定性(Annexin-V / PI),顶体完整性(Carboxy-SNARF-1 / PI / FITC-PSA),和染色质完整性(原位酸诱导的DNA变性的AO)。融化后立即延伸,高延伸率不会影响线性运动精子的比例,膜完整性或稳定性或染色质完整性。但是,高延伸率明显影响了38℃下孵育30分钟后的线性精子活力,通过SNARF评估的精子生存力,尤其是原本可以存活的精子的顶体完整性。父本个体差异明显。在一项盲区试验中,初步评估了受影响较小的公牛的生育力。共有109头奶牛随机受精15M或2M吸管,它们之间的妊娠率没有差异(47%比43%)。生育率的这种相似性,证实了所用的体外方法适用于鉴定冷冻存活,并且进一步表明,对于这个特定的父亲,精子沉积的部位对于低精子AI值的生育能力不是至关重要的。然而,当使用常规冷冻方案冷冻保存低浓度的公牛精子时,看到的公牛间变异需要谨慎。

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