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A simple PCR-based strategy for estimating species-specific contributions in chimeras and xenografts

机译:一种基于PCR的简单策略,用于估计嵌合体和异种移植中物种特异性的贡献

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摘要

Many tissue-engineering approaches for repair and regeneration involve transplants between species. Yet a challenge is distinguishing donor versus host effects on gene expression. This study provides a simple molecular strategy to quantify species-specific contributions in chimeras and xenografts. Species-specific primers for reverse transcription quantitative real-time PCR (RT-qPCR) were designed by identifying silent mutations in quail, duck, chicken, mouse and human ribosomal protein L19 (RPL19). cDNA from different pairs of species was mixed in a dilution series and species-specific RPL19 primers were used to generate standard curves. Then quail cells were transplanted into transgenic-GFP chick and resulting chimeras were analyzed with species-specific primers. Fluorescence-activated cell sorting (FACS) confirmed that donor- and host-specific levels of RPL19 expression represent actual proportions of cells. To apply the RPL19 strategy, we measured Runx2 expression in quail-duck chimeras. Elevated Runx2 levels correlated with higher percentages of donor cells. Finally, RPL19 primers also discriminated mouse from human and chick. Thus, this strategy enables chimeras and/or xenografts to be screened rapidly at the molecular level.
机译:用于修复和再生的许多组织工程方法涉及物种之间的移植。然而,一个挑战是区分供体与宿主对基因表达的影响。这项研究提供了一种简单的分子策略来量化嵌合体和异种移植中物种特异性的贡献。通过鉴定鹌鹑,鸭,鸡,小鼠和人核糖体蛋白L19(RPL19)中的沉默突变,设计了用于逆转录定量实时PCR(RT-qPCR)的物种特异性引物。将来自不同物种对的cDNA以稀释系列混合,并使用物种特异性RPL19引物生成标准曲线。然后将鹌鹑细胞移植到转基因GFP小鸡中,并使用物种特异性引物分析所得嵌合体。荧光激活细胞分选(FACS)证实RPL19表达的供体和宿主特异性水平代表细胞的实际比例。为了应用RPL19策略,我们测量了鹌鹑鸭嵌合体中Runx2的表达。 Runx2水平升高与供体细胞百分比升高相关。最后,RPL19引物也将小鼠与人和小鸡区分开。因此,该策略使得嵌合体和/或异种移植物能够在分子水平上被快速筛选。

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