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Validation of reference genes for quantitative RT-PCR studies in porcine oocytes and preimplantation embryos

机译:在猪卵母细胞和植入前胚胎中进行定量RT-PCR研究的参考基因的验证

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Background In the developing embryo, total RNA abundance fluctuates caused by functional RNA degradation and zygotic genome activation. These variations in the transcriptome in early development complicate the choice of good reference genes for gene expression studies by quantitative real time polymerase chain reaction. Results In order to identify stably expressed genes for normalisation of quantitative data, within early stages of development, transcription levels were examined of 7 frequently used reference genes (B2M, BACT, GAPDH, H2A, PGK1, SI8, and UBC) at different stages of early porcine embryonic development (germinal vesicle, metaphase-2, 2-cell, 4-cell, early blastocyst, expanded blastocyst). Analysis of transcription profiling by geNorm software revealed that GAPDH, PGK1, S18, and UBC showed high stability in early porcine embryonic development, while transcription levels of B2M, BACT, and H2A were highly regulated. Conclusion Good reference genes that reflect total RNA content were identified in early embryonic development from oocyte to blastocyst. A selection of either GAPDH or PGK1, together with ribosomal protein S18 (S18), and UBC is proposed as reference genes, but the use of B2M, BACT, or H2A is discouraged.
机译:背景技术在发育中的胚胎中,总RNA丰度因功能性RNA降解和合子基因组激活而波动。早期转录组中的这些变异使通过定量实时聚合酶链反应进行基因表达研究的良好参考基因的选择复杂化。结果为了鉴定稳定表达的基因以用于定量数据的标准化,在开发的早期阶段,检查了不同阶段的7种常用参考基因​​(B2M,BACT,GAPDH,H2A,PGK1,SI8和UBC)的转录水平。猪早期胚胎发育(胚泡,中期2、2细胞,4细胞,早期胚泡,膨胀胚泡)。通过geNorm软件进行的转录谱分析表明,GAPDH,PGK1,S18和UBC在早期猪胚胎发育中显示出高稳定性,而B2M,BACT和H2A的转录水平受到高度调节。结论在从卵母细胞到胚泡的早期胚胎发育中,鉴定出了反映总RNA含量的良好参考基因。建议选择GAPDH或PGK1以及核糖体蛋白S18(S18)和UBC作为参考基因,但不建议使用B2M,BACT或H2A。

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