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利用人工转录因子对基因表达进行优化调控。

Optimized regulation of gene expression using artificial transcription factors.

作者信息

Yaghmai Reza, Cutting Garry R

机构信息

McKusick-Nathans Institute of Genetic Medicine, Johns Hopkins Hospital, 600 North Wolfe St., Blalock 1008, Baltimore, Maryland 21287-4922, USA.

出版信息

Mol Ther. 2002 Jun;5(6):685-94. doi: 10.1006/mthe.2002.0610.

DOI:10.1006/mthe.2002.0610
PMID:12027552
Abstract

A major focus in the basic science of gene therapy is the study of factors involved in target-specific regulation of gene expression. Optimization of artificial or "designer" transcription factors capable of specific regulation of target genes is a prerequisite to developing practical applications in human subjects. In this paper, we present a systematic and combinatorial approach to optimize engineered transcription factors using designed zinc-finger proteins fused to transcriptional effector domains derived from the naturally occurring activators (VP16 or P65) or repressor (KRAB) proteins. We also demonstrate effective targeting of artificial transcription factors to regulate gene expression from three different constitutive viral promoters (SV40, CMV, RSV). Achieving a desired level of gene expression from a targeted region depended on several variables, including target site affinities for various DNA-binding domains, the nature of the activator domain, the particular cell type used, and the position of the target site with respect to the core promoter. Hence, several aspects of the artificial transcription factors should be simultaneously evaluated to ensure the optimum level of gene expression from a given target site in a given cell type. Our observations and our optimization approach have substantial implications for designing safe and effective artificial transcription factors for cell-based and therapeutic uses.

摘要

基因治疗基础科学的一个主要重点是研究参与基因表达靶向特异性调控的因素。优化能够特异性调控靶基因的人工或“设计型”转录因子是在人类受试者中开发实际应用的先决条件。在本文中,我们提出了一种系统的组合方法,利用与源自天然存在的激活剂(VP16或P65)或阻遏物(KRAB)蛋白的转录效应结构域融合的设计锌指蛋白来优化工程转录因子。我们还展示了人工转录因子对来自三种不同组成型病毒启动子(SV40、CMV、RSV)的基因表达进行有效靶向调控。从靶向区域实现所需水平的基因表达取决于几个变量,包括各种DNA结合结构域对靶位点的亲和力、激活结构域的性质、所使用的特定细胞类型以及靶位点相对于核心启动子的位置。因此,应该同时评估人工转录因子各个方面,以确保在给定细胞类型中从给定靶位点获得最佳水平的基因表达。我们的观察结果和优化方法对于设计用于基于细胞和治疗用途的安全有效的人工转录因子具有重要意义。

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