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Specific maternal transcripts in bovine oocytes and cleavaged embryos: identification with novel DDRT-PCR methods

机译:牛卵母细胞和裂解胚胎中的特定母体转录本:用新型DDRT-PCR方法鉴定

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摘要

We used annealing control primer (ACP)-based differential display reverse transcription polymerase chain reaction (DDRT-PCR) to isolate differentially expressed amplicons in bovine germinal vesicle (GV) stage oocytes, 8-cell stage embryos produced in vitro, and blastocyst stage embryos produced in vitro. Four expressed sequence tags (ESTs) of genes that were specifically and predominantly expressed in GV oocytes were cloned and sequenced. We have used a fluorescence monitored real-time quantitative PCR (qPCR) to quantify and analyzed the temporal expression of the target differentially expressed transcripts throughout the preimplantation stages from oocytes to blastocysts. The cloned genes or ESTs all exhibited significant sequence similarity with known bovine genes (98%-100%; DNCL1 and ZP2) or ESTs (81%-97%; FANK1 and GTL3) of other species. As revealed by real-time qRT-PCR, DNCL1, FANK1, GTL3, and ZP2 transcripts were observed in the GV stage oocytes and expression gradually decreased up to the 8-cell stage embryo and the transcripts were not detected in later stages. Similarly, upregulation was observed in GV stage mouse oocytes and metaphase II, suggesting that these four differentially expressed orthologous genes play important roles in early preimplantation, as maternally-derived transcripts.
机译:我们使用了基于退火控制引物(ACP)的差异显示逆转录聚合酶链反应(DDRT-PCR)来分离牛生小泡(GV)阶段卵母细胞,体外产生的8细胞阶段胚胎和囊胚阶段胚胎中差异表达的扩增子。体外产生的。克隆并测序了在GV卵母细胞中特异性和主要表达的四个基因表达序列标签(EST)。我们已经使用了荧光监测的实时定量PCR(qPCR)来量化和分析从卵母细胞到胚泡的整个植入前阶段靶标差异表达转录本的时间表达。克隆的基因或EST与其他物种的已知牛基因(98%-100%; DNCL1和ZP2)或EST(81%-97%; FANK1和GTL3)均显示出显着的序列相似性。如实时qRT-PCR所揭示,在GV期卵母细胞中观察到DNCL1,FANK1,GTL3和ZP2转录物,直到8细胞期胚胎的表达逐渐降低,而在后期则未检测到转录物。同样,在GV期小鼠卵母细胞和中期II中观察到上调,提示这四个差异表达的直系同源基因在早期植入前作为母体来源的转录本起着重要作用。

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