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Analysis of gene expression in the preimplantation mouse embryo: use of mRNA differential display.

机译:分析植入前小鼠胚胎中的基因表达:利用mRNA差异显示。

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摘要

The analysis of differential gene expression during preimplantation embryogenesis has been hindered by the paucity of biological material. We report modifications of the recently described mRNA differential display method (Liang, P. & Pardee, A. B. (1992) Science 257, 967-971) to analyze differential gene expression during mouse preimplantation development. The method detects the appropriate changes in the temporal pattern of expression of an amplicon that by DNA sequence analysis is the cytokeratin endo A, a gene whose temporal pattern of expression has been previously determined by S1 nuclease digestion. In addition, this method identifies amplicons that likely represent genes (i) that encode maternal mRNAs, (ii) that are products of early and late zygotic gene activation, (iii) whose expression is greatest during the eight-cell stage (i.e., expressed in a stage-specific manner), and (iv) whose expression is greatest in the blastocyst. In addition to endo A, sequence analysis of these amplicons reveals that an amplicon that displays a temporal pattern of expression consistent with it being a maternal mRNA is the alpha subunit of the mitochondrial F1 ATP synthase.
机译:缺乏生物材料阻碍了植入前胚胎发生过程中差异基因表达的分析。我们报告了最近描述的mRNA差异显示方法(Liang,P.&Pardee,A. B.(1992)Science 257,967-971)的修改,以分析小鼠植入前发育过程中的差异基因表达。该方法检测通过DNA序列分析是细胞角蛋白内膜A的扩增子的时间表达模式的适当变化,所述细胞角蛋白内膜A是先前通过S1核酸酶消化确定了其表达时间模式的基因。此外,该方法还可以鉴定出可能代表以下基因的扩增子:(i)编码母体mRNA;(ii)早期和晚期合子基因激活的产物;(iii)在八细胞阶段的表达最大(即表达) (iv)在胚泡中的表达最大。除了内切子A,对这些扩增子的序列分析还发现,显示与其母体mRNA一致的表达时间模式的扩增子是线粒体F1 ATP合酶的α亚基。

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