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局部注射人骨髓间充质干细胞的生物分布与滞留:基于定量聚合酶链反应检测小鼠器官中的人DNA

Biodistribution and retention of locally administered human mesenchymal stromal cells: Quantitative polymerase chain reaction-based detection of human DNA in murine organs.

作者信息

Creane Michael, Howard Linda, O'Brien Timothy, Coleman Cynthia M

机构信息

Regenerative Medicine Institute, National University of Ireland, Galway, County Galway, Ireland.

Regenerative Medicine Institute, National University of Ireland, Galway, County Galway, Ireland.

出版信息

Cytotherapy. 2017 Mar;19(3):384-394. doi: 10.1016/j.jcyt.2016.12.003. Epub 2017 Jan 12.

DOI:10.1016/j.jcyt.2016.12.003
PMID:28089755
Abstract

BACKGROUND

Determining the distributive fate and retention of a cell therapy product after administration is an essential part of characterizing it's biosafety profile. Therefore, regulatory guidelines stipulate that biodistribution assays are a requirement prior to advancing a cell therapy to the clinic. Here the development of a highly sensitive quantitative polymerase chain reaction (qPCR)-based method of tracking the biodistribution and retention of human mesenchymal stromal cells (hMSCs) in mice, rats or rabbits is described.

METHODS

A primer-probe-based qPCR assay was developed to detect and quantify human Alu sequences in a heterogeneous sample of human DNA (hDNA) and murine DNA from whole organ genomic DNA extracts. The assay measures the amount of genomic hDNA by amplifying a 31-base pair sequence of the human Alu (hAlu) repeat sequence, thus enabling the detection of 0.1 human cells in 1.5 × 10 heterogeneous cells.

RESULTS

Using this assay we investigated the biodistribution of 3 × 10 intramuscularly injected hMSCs in Balb/c nude mice. Genomic DNA was extracted from murine organs and hAlu sequences were quantified using qPCR analysis. After 3 months, hDNA ranging from 0.07%-0.58% was detected only at the injection sites and not in the distal tissues of the mice.

DISCUSSION

This assay represents a reproducible, sensitive a method of detecting hDNA in rodent and lapine models. This manuscript describes the method employed to generate preclinical biodistribution data that was accepted by regulatory bodies in support of a clinical trial application.

摘要

背景

确定细胞治疗产品给药后的分布命运和滞留情况是表征其生物安全性概况的重要组成部分。因此,监管指南规定,在将细胞治疗推进到临床试验之前,生物分布测定是一项要求。本文描述了一种基于高灵敏度定量聚合酶链反应(qPCR)的方法的开发,用于追踪人骨髓间充质干细胞(hMSCs)在小鼠、大鼠或兔子体内的生物分布和滞留情况。

方法

开发了一种基于引物-探针的qPCR测定法,用于检测和定量来自全器官基因组DNA提取物的人DNA(hDNA)和鼠DNA异质样品中的人Alu序列。该测定法通过扩增人Alu(hAlu)重复序列的31个碱基对序列来测量基因组hDNA的量,从而能够在1.5×10个异质细胞中检测到0.1个人类细胞。

结果

使用该测定法,我们研究了3×10个肌肉注射的hMSCs在Balb/c裸鼠体内的生物分布。从鼠器官中提取基因组DNA,并使用qPCR分析对hAlu序列进行定量。3个月后,仅在注射部位检测到0.07%-0.58%的hDNA,而在小鼠的远端组织中未检测到。

讨论

该测定法代表了一种在啮齿动物和兔模型中检测hDNA的可重复、灵敏的方法。本文描述了用于生成临床前生物分布数据的方法,该数据被监管机构接受以支持临床试验申请。

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