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优化标记策略,以揭示斑马鱼中不同丰度基因的表达谱。

Optimal tagging strategies for illuminating expression profiles of genes with different abundance in zebrafish.

机构信息

State Key Laboratory of Cellular Stress Biology, School of Life Sciences, Faculty of Medicine and Life Sciences, Xiamen University, 361102, Xiamen, Fujian, China.

Laboratory Animal Center, Xiamen University, 361102, Xiamen, Fujian, China.

出版信息

Commun Biol. 2023 Dec 21;6(1):1300. doi: 10.1038/s42003-023-05686-1.

Abstract

CRISPR-mediated knock-in (KI) technology opens a new era of fluorescent-protein labeling in zebrafish, a preferred model organism for in vivo imaging. We described here an optimized zebrafish gene-tagging strategy, which enables easy and high-efficiency KI, ensures high odds of obtaining seamless KI germlines and is suitable for wide applications. Plasmid donors for 3'-labeling were optimized by shortening the microhomologous arms and by reducing the number and reversing the sequence of the consensus Cas9/sgRNA binding sites. To allow for scar-less KI across the genome, linearized dsDNA donors with 5'-chemical modifications were generated and successfully incorporated into our method. To refine the germline screen workflow and expedite the screen process, we combined fluorescence enrichment and caudal-fin junction-PCR. Furthermore, to trace proteins expressed at a low abundance, we developed a fluorescent signal amplifier using the transcriptional activation strategy. Together, our strategies enable efficient gene-tagging and sensitive expression detection for almost every gene in zebrafish.

摘要

CRISPR 介导的基因敲入 (KI) 技术为斑马鱼的荧光蛋白标记开辟了一个新时代,斑马鱼是一种用于体内成像的首选模式生物。我们在这里描述了一种优化的斑马鱼基因标记策略,该策略可实现简便高效的 KI,确保高几率获得无缝 KI 生殖系,并适用于广泛的应用。通过缩短微同源臂和减少 Cas9/sgRNA 结合位点的数量并反转其序列,优化了用于 3'标记的质粒供体。为了实现基因组范围内无疤痕的 KI,我们生成了带有 5'化学修饰的线性化 dsDNA 供体,并成功地将其纳入我们的方法中。为了改进生殖系筛选工作流程并加快筛选过程,我们结合了荧光富集和尾部鳍连接-PCR。此外,为了追踪低丰度表达的蛋白质,我们使用转录激活策略开发了一种荧光信号放大器。总之,我们的策略可实现斑马鱼中几乎每个基因的高效基因标记和敏感表达检测。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/e644/10739737/7bad31bd9a6e/42003_2023_5686_Fig1_HTML.jpg

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