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携带X和Y染色体的哺乳动物精子的流式分选:分选后的公牛、公猪和公羊精子显微注射到仓鼠卵母细胞后的激活及原核发育

Flow sorting of X and Y chromosome-bearing mammalian sperm: activation and pronuclear development of sorted bull, boar, and ram sperm microinjected into hamster oocytes.

作者信息

Johnson L A, Clarke R N

机构信息

U.S. Department of Agriculture, Beltsville Agricultural Research Center, Maryland 20705.

出版信息

Gamete Res. 1988 Dec;21(4):335-43. doi: 10.1002/mrd.1120210402.

Abstract

Flow cytometric techniques were used to measure relative DNA content of X and Y chromosome-bearing bull, boar, and ram sperm populations and to separate the two sex-determining populations. Neat semen was prepared for flow cytometric analysis by washing, light sonication, and staining with 9 microM Hoechst 33342. Computer analysis of the bimodal histograms showed mean X-Y DNA differences of 3.9, 3.7, and 4.2% for bull, boar, and ram, respectively. Flow cytometric reanalysis of sorted bull, boar, and ram sperm showed purities greater than 90%. Bull, boar, and ram sperm nuclei were microinjected into hamster oocytes. Microinjected sperm were either unsorted, sorted, unsorted plus dithiothreitol (DTT) exposure, or sorted plus DTT exposure. Following microinjection, eggs were incubated 3 hr, fixed, and stained. A total of 579 eggs was observed for sperm activation (decondensation or formation of a male pronucleus). A lower percentage of sorted than unsorted (3 vs. 23%) boar sperm was activated (P less than .05). However, sorted and unsorted DTT-exposed boar sperm or sorted and unsorted bull or ram sperm, regardless of DTT treatment, did not differ significantly. Sorted sperm nuclei of both rams and bulls exhibited higher activation rates than sorted boar sperm (P less than .05). Treatment of sperm with DTT increased the activation rate (P less than .05) for sorted boar sperm but not for bull or ram sperm.(ABSTRACT TRUNCATED AT 250 WORDS)

摘要

采用流式细胞术技术来测量携带X和Y染色体的公牛、公猪和公羊精子群体的相对DNA含量,并分离这两个决定性别的群体。通过洗涤、轻度超声处理并用9微摩尔的Hoechst 33342染色,将纯精液制备用于流式细胞术分析。对双峰直方图的计算机分析显示,公牛、公猪和公羊的平均X - Y DNA差异分别为3.9%、3.7%和4.2%。对分选后的公牛、公猪和公羊精子进行流式细胞术重新分析,结果显示纯度大于90%。将公牛、公猪和公羊的精子细胞核显微注射到仓鼠卵母细胞中。显微注射的精子要么未分选、已分选,要么未分选加二硫苏糖醇(DTT)处理,或者已分选加DTT处理。显微注射后,将卵孵育3小时,固定并染色。共观察了579个卵以检测精子激活情况(去浓缩或雄性原核形成)。已分选的公猪精子激活率低于未分选的公猪精子(3%对23%,P < 0.05)。然而,无论是否进行DTT处理,已分选和未分选的经DTT处理的公猪精子或已分选和未分选的公牛或公羊精子之间没有显著差异。公羊和公牛的已分选精子细胞核的激活率均高于已分选的公猪精子(P < 0.05)。用DTT处理精子可提高已分选公猪精子的激活率(P < 0.05),但对公牛或公羊精子无效。(摘要截短于250字)

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