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一种在秀丽隐杆线虫中表达遗传工具的融合 PCR 方法。

A Fusion PCR Method for Expressing Genetic Tools in C. elegans.

机构信息

Department of Genetics, Silberman Institute of Life Science, Edmond J. Safra Campus, The Hebrew University of Jerusalem, Jerusalem, Israel.

出版信息

Methods Mol Biol. 2022;2468:205-214. doi: 10.1007/978-1-0716-2181-3_10.

Abstract

C. elegans offer a unique opportunity for understanding computation in neural networks. This is largely due to their relatively compact neural network for which a wiring diagram is available. Recent advances in genetic tools for interrogating neural activity (e.g., optogenetics) make C. elegans particularly compelling as they can be expressed in many different combinations in target individual neurons. Thus, the prospect to decipher principles underlying functionality in neural networks largely depends on the ease by which transgenic animals can be generated. Traditionally, to generate transgenic animals one would inject a plasmid containing the gene of interest under the regulation of the cell- or lineage-specific promoter. This often requires laborious cloning steps of both the gene and the promoter. The Hobert lab has developed a simpler protocol in which linear PCR fragments can be injected to generate transgenic animals. Relying on this PCR fusion-based method, here we provide a detailed protocol that we have optimized for expressing various genetically encoded calcium indicators and optogenetic tools in individual or sets of neurons. We use these simple procedures to generate multiple constructs within a very short time frame (typically 1-2 days).

摘要

秀丽隐杆线虫为理解神经网络中的计算提供了独特的机会。这在很大程度上要归功于其相对紧凑的神经网络,该网络有一个可用的接线图。最近在研究神经活动的遗传工具方面取得了进展(例如光遗传学),这使得秀丽隐杆线虫特别引人注目,因为它们可以在目标单个神经元中以多种不同的组合进行表达。因此,能否阐明神经网络功能背后的原理在很大程度上取决于能否轻松地生成转基因动物。传统上,要生成转基因动物,人们会将含有目的基因的质粒在细胞或谱系特异性启动子的调控下进行注射。这通常需要对基因和启动子进行繁琐的克隆步骤。Hobert 实验室开发了一种更简单的方案,其中可以注射线性 PCR 片段来生成转基因动物。在这里,我们依赖于这种基于 PCR 融合的方法,提供了一种经过优化的详细方案,用于在单个或一组神经元中表达各种遗传编码钙指示剂和光遗传学工具。我们使用这些简单的程序在很短的时间内(通常为 1-2 天)生成多个构建体。

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