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通过 RNA-Seq 对通过各种辅助生殖技术生成的附着前猪胚胎进行转录谱分析。

Transcriptional profiling by RNA-Seq of peri-attachment porcine embryos generated by a variety of assisted reproductive technologies.

机构信息

Animal Dairy & Veterinary Sciences Department, Utah State University, Logan, Utah, USA.

出版信息

Physiol Genomics. 2013 Jul 15;45(14):577-89. doi: 10.1152/physiolgenomics.00094.2012. Epub 2013 May 21.

Abstract

Substantial mortality of in vitro manipulated porcine embryos is observed during peri-attachment development. Herein we describe our efforts to characterize the transcriptomes of embryonic disc (ED) and trophectoderm (TE) cells from porcine embryos derived from in vivo fertilization, in vitro fertilization (IVF), parthenogenetic oocyte activation (PA), and somatic cell nuclear transfer (SCNT) on days 10, 12, and 14 of gestation. The IVF, PA, and SCNT embryos were generated with in vitro matured oocytes and were cultured overnight in vitro before being transferred to recipient females. Sequencing of cDNA from the resulting embryonic samples was accomplished with the Genome Analyzer IIx platform from Illumina. Reads were aligned to a custom-built swine transcriptome. A generalized linear model was fit for ED and TE samples separately, accounting for embryo type, gestation day, and their interaction. Those genes with significant differences between embryo types were characterized in terms of gene ontologies and KEGG pathways. Transforming growth factor-β signaling was downregulated in the EDs of IVF embryos. In TE cells from IVF embryos, ubiquitin-mediated proteolysis and ErbB signaling were aberrantly regulated. Expression of genes involved in chromatin modification, gene silencing by RNA, and apoptosis was significantly disrupted in ED cells from SCNT embryos. In summary, we have used high-throughput sequencing technologies to compare gene expression profiles of various embryo types during peri-attachment development. We expect that these data will provide important insight into the root causes of (and possible opportunities for mitigation of) suboptimal development of embryos derived from assisted reproductive technologies.

摘要

在附着前发育过程中,体外操作的猪胚胎的死亡率很高。在此,我们描述了我们的努力,以描绘来自体内受精、体外受精 (IVF)、孤雌激活 (PA) 和体细胞核移植 (SCNT) 的胚胎盘 (ED) 和滋养外胚层 (TE) 细胞的转录组特征来自妊娠第 10、12 和 14 天的猪胚胎。IVF、PA 和 SCNT 胚胎是用体外成熟的卵母细胞产生的,并在体外培养过夜,然后转移到受体雌性体内。从所得胚胎样本的 cDNA 进行测序使用 Illumina 的 Genome Analyzer IIx 平台完成。将 reads 分别对齐到定制的猪转录组。为 ED 和 TE 样本分别拟合广义线性模型,考虑胚胎类型、妊娠天数及其相互作用。对胚胎类型之间存在显著差异的基因进行了基因本体论和 KEGG 途径特征描述。IVF 胚胎的 ED 中转化生长因子-β信号下调。在 IVF 胚胎的 TE 细胞中,泛素介导的蛋白水解和 ErbB 信号异常调节。在 SCNT 胚胎的 ED 细胞中,涉及染色质修饰、RNA 介导的基因沉默和细胞凋亡的基因表达显著中断。总之,我们使用高通量测序技术比较了附着前发育过程中各种胚胎类型的基因表达谱。我们期望这些数据将为辅助生殖技术衍生的胚胎发育不良的根本原因(和可能的缓解机会)提供重要的见解。

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