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一种用于检测RAG-1基因敲除小鼠体内移植的人肝细胞的“实时”聚合酶链反应检测法。

A "real time" PCR assay to detect transplanted human liver cells in RAG-1-/- mice.

作者信息

Funkhouser A W, Vahed S, Soriano H E

机构信息

University of Chicago, Department of Pediatrics, University of Chicago Children's Hospital, IL 60637, USA.

出版信息

Cell Transplant. 2001 Jan-Feb;10(1):91-9.

Abstract

Xenotransplantation of human liver cells is an expanding field in need of new and precise quantitative techniques. "Real time" PCR is a sensitive and accurate method of quantifying picogram quantities of DNA. We used "real time" PCR with primers complementary to the human alpha-1-antitrypsin gene to assess the efficiency of engraftment of human liver cells transplanted into immunotolerant RAG-1-/- mice. Standard curves were created by mixing known proportions of human and mouse cells. There was a linear relationship between the PCR cycle at which DNA was amplified [threshold cycle (C(T)] and the percent human cells (linear regression, p < 0.00009). Results were reliable, with a maximum 1.27-fold variation in the slopes of repeated standard curves. Linearity was maintained from 100% to as low as 0.01%. Therefore, 1 in 10,000 mouse cells could be detected in a 100 ng DNA sample. We measured the percent engraftment of human liver cells transplanted into the spleen of RAG-1-/- mice. By "real time" PCR assay, 0.23% human cells could be detected at 1 day after human cell transplantation. These results show that "real time" PCR assay is highly sensitive, reproducible, and accurate for detecting human cells in xenotransplanted mice.

摘要

人肝细胞异种移植是一个不断发展的领域,需要新的精确量化技术。“实时”PCR是一种灵敏且准确的定量皮克级DNA的方法。我们使用与人类α-1-抗胰蛋白酶基因互补的引物进行“实时”PCR,以评估移植到免疫耐受的RAG-1-/-小鼠体内的人肝细胞的植入效率。通过混合已知比例的人细胞和小鼠细胞来创建标准曲线。DNA扩增时的PCR循环数[阈值循环(C(T))]与人类细胞百分比之间存在线性关系(线性回归,p < 0.00009)。结果可靠,重复标准曲线的斜率最大变化为1.27倍。线性关系在100%至低至0.01%之间保持。因此,在100 ng DNA样本中可以检测到万分之一的小鼠细胞。我们测量了移植到RAG-1-/-小鼠脾脏中的人肝细胞的植入百分比。通过“实时”PCR检测,在人细胞移植后1天可检测到0.23%的人类细胞。这些结果表明,“实时”PCR检测对于检测异种移植小鼠中的人类细胞具有高度敏感性、可重复性和准确性。

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