Transcriptional Profiling by Deep Sequencing Identifies Differences in mRNA Transcript Abundance in In Vivo-Derived Versus In Vitro-Cultured Porcine Blastocyst Stage Embryos1

生物 胚泡 转录组 内细胞团 胚胎 胚胎培养 男科 输卵管 体内 Illumina染料测序 分子生物学 深度测序 体外 合子 生殖技术 遗传学 胚胎发生 基因表达 基因 DNA测序 基因组 内分泌学 医学
作者
B. K. Bauer,S. Clay Isom,Lee D. Spate,Kristin M. Whitworth,William G. Spollen,Sean Blake,Gordon K. Springer,Clifton N. Murphy,Randall S. Prather
出处
期刊:Biology of Reproduction [Oxford University Press]
卷期号:83 (5): 791-798 被引量:80
标识
DOI:10.1095/biolreprod.110.085936
摘要

In vitro embryo culture systems promote development at rates lower than in vivo systems. The goal of this project was to discover transcripts that may be responsible for a decrease of embryo competency in blastocyst-stage embryos cultured in vitro. Gilts were artificially inseminated on the first day of estrus, and on Day 2, one oviduct and the tip of a uterine horn were flushed and the recovered embryos were cultured in porcine zygote medium 3 for 4 days. On Day 6, the gilts were euthanized and the contralateral horn was flushed to obtain in vivo derived embryos. Total RNA was extracted from three pools of 10 blastocysts from each treatment. First and second strand cDNA was synthesized and sequenced using Illumina sequencing. The reads generated were aligned to a custom-built database designed to represent the known porcine transcriptome. A total of 1170 database members were different between the two groups (P < 0.05), and 588 of those had at least a 2-fold difference. Eleven transcripts were subjected to real-time PCR that validated the sequencing. There was an overall decrease in inner cell mass (ICM) and trophectodermal (TE) cell numbers in embryos cultured in vitro; however, no difference in the ICM:TE ratio was found. Interestingly, the transcript SLC7A1 was higher in the in vitro cultured group. This difference disappeared after addition of arginine to the 4-day culture. Illumina sequencing and alignment to a custom transcriptome identified a large number of genes that yield clues on ways to manipulate the culture media to mimic the in vivo environment.
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