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两种用于提高人诱导多能干细胞系的产生和分离效率的新方案。

Two new protocols to enhance the production and isolation of human induced pluripotent stem cell lines.

作者信息

Dick Emily, Matsa Elena, Bispham Jayson, Reza Mojgan, Guglieri Michela, Staniforth Andrew, Watson Sue, Kumari Rajendra, Lochmüller Hanns, Young Lorraine, Darling David, Denning Chris

机构信息

Wolfson Centre for Stem Cells, Tissue Engineering & Modelling, Centre for Biomolecular Sciences, University of Nottingham, University Park, Nottingham, NG7 2RD, UK.

出版信息

Stem Cell Res. 2011 Mar;6(2):158-67. doi: 10.1016/j.scr.2010.10.002. Epub 2010 Nov 20.

Abstract

There are two critical stages in the retroviral reprogramming of somatic cells to produce human induced pluripotent stem cell (hiPSC) lines. One is the production of high titer virus required to reprogram somatic cells; the other is identification of true hiPSC colonies from heterogeneous cell populations, and their isolation and expansion to generate a sustainable, pluripotent stem cell line. Here we describe simple, time-saving methods to address the current difficulties at these two critical junctures. First, we have developed a method to increase the number of infectious viral units 600-fold. Second, we have developed a TRA-1-81-based positive selection column method for isolating "true" hiPSCs from the heterogeneous cell populations, which overcomes the labor-intensive and highly subjective method of manual selection of hiPSC colonies. We have used these techniques to produce 8 hiPSC lines from human fibroblasts and we believe that they are of considerable utility to researchers in the hiPSC field.

摘要

将体细胞重编程以产生人诱导多能干细胞(hiPSC)系的逆转录病毒重编程过程中有两个关键阶段。一个是重编程体细胞所需的高滴度病毒的产生;另一个是从异质细胞群体中鉴定真正的hiPSC集落,并对其进行分离和扩增以产生可持续的多能干细胞系。在此,我们描述了简单、省时的方法来解决这两个关键时刻的当前困难。首先,我们开发了一种将感染性病毒单位数量增加600倍的方法。其次,我们开发了一种基于TRA-1-81的阳性选择柱方法,用于从异质细胞群体中分离“真正的”hiPSC,该方法克服了手动选择hiPSC集落的劳动密集型和高度主观的方法。我们已使用这些技术从人成纤维细胞中产生了8个hiPSC系,并且我们认为它们对hiPSC领域的研究人员具有相当大的实用性。

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