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通过流式细胞分选实现绵羊皮肤成纤维细胞在 G2/M 期的高效同步化,并分离绵羊 Y 染色体。

Highly efficient synchronization of sheep skin fibroblasts at G2/M phase and isolation of sheep Y chromosomes by flow cytometric sorting.

机构信息

Key Laboratory of Animal Genetics, Breeding and Reproduction of the Ministry of Agriculture & Beijing Key Laboratory of Animal Genetic Improvement, China Agricultural University, Beijing, 100193, China.

Department of Animal Science, Center for Reproductive Biology and Health, College of Agricultural Sciences, Pennsylvania State University, University Park, Pennsylvania, 16802, USA.

出版信息

Sci Rep. 2020 Jun 18;10(1):9933. doi: 10.1038/s41598-020-66905-x.

Abstract

At present, based on whole genome sequencing, sequences and genes annotation of the sheep (Ovis aries) Y chromosome are still absent. The isolation of Y chromosomes followed by sequencing has been approved as an effective approach to analyze this complex chromosome in other species. In this study, we established a highly efficient synchronization method for G2/M phase of sheep fibroblasts, which was successfully applied to flow-sorting chromosomes of sheep, with a focus on isolation and sequencing of the ovine Y chromosome. The isolated (~80,000) Y chromosomes were verified by fluorescence quantitative real-time polymerase chain reaction, further confirmed by fluorescence in situ hybridization, and amplified by the MALBAC method before next-generation sequencing. The sequence results indicated that 68.90% of reads were Y chromosome-related sequences as they are homologous to the bovine Y chromosome. The remaining 31.1% of reads were aligned to the sheep reference genome, including 13.57% reads to chromosome X and 6.68% to chromosome 17. Importantly, the paired-end reads that are properly aligned to the bovine Y sequence assembly accounted for 46.49%, indicating the success in the ovine Y chromosome isolation and the high quality of the Y chromosome sequences. This study not only set up a foundation for future sequencing, assembly and annotation of the ovine Y chromosome, but also provide a validated approach to overcoming difficulties in sequencing Y chromosome in other mammalian species.

摘要

目前,绵羊(Ovis aries)Y 染色体的全基因组测序、序列和基因注释仍然缺失。已经证实,通过对 Y 染色体进行测序和分离,然后对其进行测序,是分析其他物种中这种复杂染色体的有效方法。在本研究中,我们建立了一种高效的绵羊成纤维细胞 G2/M 期同步化方法,该方法成功地应用于绵羊染色体的流式分选,重点是绵羊 Y 染色体的分离和测序。通过荧光定量实时聚合酶链反应验证了分离得到的(约 80000 条)Y 染色体,通过荧光原位杂交进一步确认,并通过 MALBAC 方法扩增后进行下一代测序。序列结果表明,68.90%的读取序列与牛 Y 染色体同源,与 Y 染色体相关。其余 31.1%的读取序列与绵羊参考基因组相对应,包括 13.57%的读取序列与 X 染色体和 6.68%的与 17 号染色体相对应。重要的是,与牛 Y 序列组装正确比对的配对末端读取序列占 46.49%,这表明绵羊 Y 染色体的成功分离和 Y 染色体序列的高质量。本研究不仅为绵羊 Y 染色体的未来测序、组装和注释奠定了基础,也为克服其他哺乳动物 Y 染色体测序困难提供了一种经过验证的方法。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/7c6c/7303189/4753f266b8d5/41598_2020_66905_Fig1_HTML.jpg

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