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Integrated Analysis of miRNA and mRNA Expression Profiles Reveals Functional miRNA-Targets in Development Testes of Small Tail Han Sheep

机译:miRNA和mRNA表达谱的综合分析揭示了小尾寒羊发育睾丸中的功能性miRNA目标。

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摘要

Small Tail Han Sheep is a highly valued local breed in China because of their precocity, perennial estrus, and high fecundity. The average annual lambing rate of ewes is as high as 180–270%, the semen of ram has characteristics of high yield, high density, and good motility. To reveal the key miRNAs and miRNA-targets underlying testis development and spermatogenesis in male Small Tail Han Sheep, integrated analysis of miRNA and mRNA expression profiles in 2-, 6-, and 12-month-old testes was performed by RNA-seq technology and bioinformatics methods. The results showed that total of 153 known sheep miRNAs and 2712 novel miRNAs were obtained in 2-,6 - and 12-month-old Small Tail Han Sheep testes; 5, 1, and 4 differentially expressed (DE) known sheep miRNAs, and 132, 105, and 24 DE novel miRNAs were identified in 2- vs. 6-, 6- vs. 12-, and 2- vs. 12-month-old testes, respectively. We combined miRNA results of this study and the mRNA results obtained in our previous study to predict the target mRNAs of DE known sheep miRNAs; 131, 10, and 15 target mRNAs of DE known sheep miRNAs and 76, 1, and 11 DE miRNA–targets were identified in the three groups, respectively. GO and KEGG analyses showed that: in 2- vs. 6-month-olds, the target genes of DE known sheep miRNAs were involved in 100 biological processes and 11 signaling pathways; in 6- vs. 12-month-olds, the target genes of DE known sheep miRNAs were involved in 4 biological processes; and in 2- vs. 12-month-olds, the target genes of DE known sheep miRNAs were involved in 17 biological processes and 4 signaling pathways. Three miR–target regulatory networks were constructed based on these DE miRNA–targets. The key miRNA-Targets involved in testis development and spermatogenesis were screened. 6 known sheep miRNAs and 6 novel miRNAs were selected to validate the accuracy of miRNA sequencing data by qRT-PCR. The binding sites of oar-miR-379-5p with WNT8A was validated by a dual luciferase reporter gene detection system.
机译:小尾寒羊由于其早熟,多年生发情和高繁殖力而在中国是极有价值的地方品种。母羊的年平均产羔率高达180-270%,公羊的精液具有高产量,高密度和良好的运动性的特点。为了揭示雄性小尾寒羊睾丸发育和精子形成的关键miRNA和miRNA靶标,通过RNA-seq技术对2个月,6个月和12个月大睾丸中的miRNA和mRNA表达谱进行了综合分析。和生物信息学方法。结果表明,在2、6和12个月大的小尾寒羊绵羊睾丸中共获得了153种已知的绵羊miRNA和2712种新颖的miRNA;在2个月,6个月,6个月,12个月和2个月和12个月的时间内鉴定出5、1、4个差异表达(DE)的已知绵羊miRNA,以及132、105和24个DE新型miRNA。老睾丸。我们将本研究的miRNA结果与先前研究中获得的mRNA结果结合起来,以预测DE已知绵羊miRNA的靶标mRNA。在这三组中分别鉴定出DE已知绵羊miRNA的131、10和15个靶mRNA和76、1和11个DE miRNA –靶。 GO和KEGG分析表明:在2个月和6个月大的婴儿中,DE已知绵羊miRNA的靶基因参与了100个生物过程和11个信号通路。在6个月和12个月大的婴儿中,DE已知绵羊miRNA的靶基因参与了4个生物学过程。在2个月和12个月大的婴儿中,DE已知绵羊miRNA的靶基因参与了17个生物学过程和4条信号通路。基于这些DE miRNA靶标构建了三个miR靶标调控网络。筛选了涉及睾丸发育和精子发生的关键miRNA-Targets。选择了6种已知的绵羊miRNA和6种新颖的miRNA,以通过qRT-PCR验证miRNA测序数据的准确性。通过双重荧光素酶报告基因检测系统验证了oar-miR-379-5p与WNT8A的结合位点。

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