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在果蝇中进行靶向基因表达的工具的改进。

Refinement of tools for targeted gene expression in Drosophila.

机构信息

Janelia Farm Research Campus, Howard Hughes Medical Institute, Ashburn, VA 20147, USA.

出版信息

Genetics. 2010 Oct;186(2):735-55. doi: 10.1534/genetics.110.119917. Epub 2010 Aug 9.

Abstract

A wide variety of biological experiments rely on the ability to express an exogenous gene in a transgenic animal at a defined level and in a spatially and temporally controlled pattern. We describe major improvements of the methods available for achieving this objective in Drosophila melanogaster. We have systematically varied core promoters, UTRs, operator sequences, and transcriptional activating domains used to direct gene expression with the GAL4, LexA, and Split GAL4 transcription factors and the GAL80 transcriptional repressor. The use of site-specific integration allowed us to make quantitative comparisons between different constructs inserted at the same genomic location. We also characterized a set of PhiC31 integration sites for their ability to support transgene expression of both drivers and responders in the nervous system. The increased strength and reliability of these optimized reagents overcome many of the previous limitations of these methods and will facilitate genetic manipulations of greater complexity and sophistication.

摘要

各种各样的生物学实验都依赖于在转基因动物中以特定水平和时空控制模式表达外源基因的能力。我们描述了在黑腹果蝇中实现这一目标的可用方法的主要改进。我们系统地改变了核心启动子、UTR、操作序列和转录激活结构域,用于指导 GAL4、LexA 和 Split GAL4 转录因子以及 GAL80 转录抑制剂的基因表达。使用位点特异性整合,我们可以在同一基因组位置插入的不同构建体之间进行定量比较。我们还对一组 PhiC31 整合位点进行了特征分析,以确定它们在神经系统中支持驱动基因和反应基因表达的能力。这些优化试剂的增强的强度和可靠性克服了这些方法以前的许多限制,并将促进更复杂和精细的遗传操作。

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