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首页> 外文期刊>Stem cell reviews and Reports >Human Genome-Specific Real-Time PCR Method for Sensitive Detection and Reproducible Quantitation of Human Cells in Mice
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Human Genome-Specific Real-Time PCR Method for Sensitive Detection and Reproducible Quantitation of Human Cells in Mice

机译:人类基因组特异性实时PCR方法用于小鼠细胞的灵敏检测和可重复定量

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Xenotransplantation of human cells into immunodeficiency mice has been frequently used to study stem cells in tissue repair and regeneration and cancer cell metastasis. However, a sensitive and reproducible method to quantify cell engraftment lacks. Here, we developed a Real-Time PCR-based method which facilitated consistent detection and quantification of small amounts of human cells distributed in mouse organs after infusion. The principle of the method was to directly detect a humans-specific sequence in the human-murine genomic DNA mixture. In a mouse myocardial infarction model, the Real-Time PCR-based method consistently determined the amounts of human mesenchymal stem cells (hMSCs) engrafted into the heart and other organs 7 days after infusion of as little as 2. 5 × 105 cells, indicating a high sensitivity, and the amounts of hMSCs detected in mice highly correlated to the numbers of hMSCs transplanted. Importantly, different from previous PCR-based methods, our method produced highly consistent and reproducible results. The reliability of the method was further proven by parallel analyses of DiI-labeled hMSCs in tissue sections and in single cell suspensions of mice. Our data show that the present human genomic DNA-specific primers-based Real-Time PCR method is sensitive and highly reproducible in determining the amount of xenotransplanted human cells in murine tissues.
机译:人类细胞的异种移植到免疫缺陷小鼠中已经常用于研究干细胞在组织修复和再生以及癌细胞转移中的作用。然而,缺少一种灵敏且可再现的量化细胞植入的方法。在这里,我们开发了一种基于实时PCR的方法,该方法有助于在输注后对小鼠器官中分布的少量人体细胞进行一致的检测和定量。该方法的原理是直接检测人-鼠基因组DNA混合物中的人特异性序列。在小鼠心肌梗塞模型中,基于实时PCR的方法可在输注少至2天后7天一致地确定植入心脏和其他器官的人间充质干细胞(hMSC)的数量。高灵敏度,并且在小鼠中检测到的hMSC的数量与移植的hMSC的数量高度相关。重要的是,与以前的基于PCR的方法不同,我们的方法产生了高度一致且可重复的结果。通过在组织切片和小鼠单细胞悬液中对DiI标记的hMSC进行平行分析,进一步证明了该方法的可靠性。我们的数据表明,目前的基于人类基因组DNA特异性引物的实时PCR方法在确定鼠组织中异种移植的人类细胞的数量方面是灵敏且高度可重复的。

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