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Use of immobilized cryopreserved bovine semen in a blind artificial insemination trial

机译:固定冷冻保存的牛精液在盲人人工授精试验中的使用

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To make timing of artificial insemination (AI) relative to ovulation less critical, methods for prolonging shelf life of spermatozoa in vivo after AI have been attempted to be developed. Encapsulation of sperm cells is a documented technology, and recently, a technology in which sperm cells are embedded in alginate gel has been introduced and commercialized. In this study, standard processed semen with the Biladyl extender (control) was compared with semen processed by sperm immobilization technology developed by SpermVital AS in a blind field trial. Moreover, in vitro acrosome and plasma membrane integrity was assessed and compared with Al fertility data for possible correlation. Semen from 16 Norwegian Red young bulls with unknown fertility was collected and processed after splitting the semen in two aliquots. These aliquots were processed with the standard Biladyl extender or the SpermVital extender to a final number of 12 x 10(6) and 25 x 10(6) spermatozoa/dose, respectively. In total, 2000 semen doses were produced from each bull, divided equally by treatment. Artificial insemination doses were set up to design a blinded Al regime; 5 + 5 straws from each extender within ejaculates in ten-straw goblets were distributed to Al technicians and veterinarians all over Norway. Outcomes of the inseminations were measured as 56-day nonreturn rate (NRR). Postthaw sperm quality was assessed by flow cytometry using propidium iodide and Alexa 488 conjugated peanut agglutinin to assess the proportion of plasma membrane and acrosome-intact sperm cells, respectively. In total, data from 14,125 first inseminations performed over a 12-month period, 7081 with Biladyl and 7044 with SpermVital semen, were used in the statistical analyses. There was no significant difference in 56-day NRR for the two semen categories, overall NRR being 72.5% and 72.7% for Biladyl and SpermVital, respectively. The flow cytometric results revealed a significant higher level of acrosome-intact live spermatozoa in Biladyl-processed semen compared to SpermVital semen. The results indicate that the level of acrosome-intact live spermatozoa in the Al dose did not affect the 56-day NRR for the two semen processing methods. In conclusion, this study has showed that immobilized spermatozoa provide equal fertility results as standard processed semen when Al is performed in a blinded field trial, although the immobilization procedure caused increased sperm damage evaluated in vitro compared to standard semen processing procedure. (C) 2015 The Authors. Published by Elsevier Inc.
机译:为了使相对于排卵的人工授精(AI)时间更不重要,已尝试开发在AI之后延长体内精子货架期的方法。精子细胞的包囊化是有记载的技术,近来,引入了将精子细胞嵌入藻酸盐凝胶中的技术并使其商业化。在这项研究中,在盲区试验中,将使用Biladyl扩展剂(对照)处理的标准精液与通过SpermVital AS开发的精子固定技术处理的精液进行了比较。此外,评估了体外顶体和质膜的完整性,并与A1生育力数据进行了比较,以寻找可能的相关性。在将精液分成两等份后,收集并加工了来自16头不育的挪威红公牛的精液。将这些等分试样分别用标准Biladyl补充剂或SpermVital补充剂加工成最终数量分别为12 x 10(6)和25 x 10(6)的精子/剂量。每头公牛总共产生2000精液剂量,除以治疗均分。设置人工​​授精剂量以设计盲目的Al方案。在十个稻草杯中,每个射精中的5 + 5根吸管被分配给整个挪威的Al技术人员和兽医。授精的结果以56天的不归巢率(NRR)衡量。通过使用碘化丙啶和Alexa 488缀合的花生凝集素通过流式细胞术评估解冻后的精子质量,分别评估质膜和完整的顶体精子细胞的比例。在统计分析中,总共使用了在12个月内进行的14125次首次授精,使用Biladyl的7081和使用SpermVital精液的7044个数据。两种精液类别的56天NRR没有显着差异,Biladyl和SpermVital的总NRR分别为72.5%和72.7%。流式细胞仪检测结果显示,与精子活精液相比,经二甲丙啶处理的精液中的顶体完整活精子水平显着更高。结果表明,两种精液加工方法中,A1剂量的顶体完整活精子水平均不影响56天的NRR。总之,这项研究表明,在固定的精子中,与常规精液加工相比,固定化精子在体外评估的精子损伤增加,尽管在固定盲法试验中进行Al时,固定精子的繁殖力与标准精液相同。 (C)2015作者。由Elsevier Inc.发布

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