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推动基于CRISPR的可编程平台超越哺乳动物细胞中的基因组编辑。

Advancing CRISPR-Based Programmable Platforms beyond Genome Editing in Mammalian Cells.

作者信息

Higashikuni Yasutomi, Lu Timothy K

出版信息

ACS Synth Biol. 2019 Dec 20;8(12):2607-2619. doi: 10.1021/acssynbio.9b00297. Epub 2019 Dec 11.

DOI:10.1021/acssynbio.9b00297
PMID:31751114
Abstract

Human diseases are caused by dysregulation of cellular biological programs that are encoded in DNA. Unveiling the endogenous programs and encoding new programs into the genome are key to creating novel diagnostic and therapeutic strategies. CRISPR/Cas9, originally identified in bacteria, has revolutionized genome editing in mammalian cells. Recent advances in CRISPR technologies have provided new programmable platforms for modifying cell function and behavior. CRISPR-based transcriptional regulators and modified gRNAs have enabled multiplexed regulation and visualization of genome dynamics with spatiotemporal precision. Using these toolkits, genome-scale screening platforms can identify key genetic elements or combinations thereof that modulate phenotypes in mammalian cells. In addition, imaging platforms for multiplexed genomic labeling have been created to study the conformation and dynamics of chromatin in living cells, which are essential for genome function. Furthermore, CRISPR-based computation and memory platforms have been built in living mammalian cells by using DNA as a data processing and storage medium to regulate and monitor cellular behaviors. The conditional regulation of CRISPR-based parts has enabled the design of complex multilayered biological programs. CRISPR-based memory platforms can continuously record biological events as mutations in defined DNA loci. By making use of base editors, CRISPR-based computation and memory platforms have been interconnected to perform logic operations based on past events. These technologies open up new avenues for understanding biological phenomena and designing mammalian cells as living machines for biomedical applications.

摘要

人类疾病是由DNA编码的细胞生物学程序失调引起的。揭示内源性程序并将新程序编码到基因组中是创造新型诊断和治疗策略的关键。CRISPR/Cas9最初在细菌中被发现,它彻底改变了哺乳动物细胞中的基因组编辑。CRISPR技术的最新进展为改变细胞功能和行为提供了新的可编程平台。基于CRISPR的转录调节因子和修饰的引导RNA能够以时空精度对基因组动态进行多重调节和可视化。利用这些工具包,基因组规模的筛选平台可以识别调节哺乳动物细胞表型的关键遗传元件或其组合。此外,还创建了用于多重基因组标记的成像平台,以研究活细胞中染色质的构象和动态,这对基因组功能至关重要。此外,通过将DNA用作数据处理和存储介质来调节和监测细胞行为,在活的哺乳动物细胞中构建了基于CRISPR的计算和记忆平台。基于CRISPR的组件的条件调节使得能够设计复杂的多层生物程序。基于CRISPR的记忆平台可以将生物事件作为定义的DNA位点中的突变持续记录下来。通过利用碱基编辑器,基于CRISPR的计算和记忆平台已经相互连接,以根据过去的事件执行逻辑操作。这些技术为理解生物现象以及将哺乳动物细胞设计为用于生物医学应用的活体机器开辟了新途径。

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引用本文的文献

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JACKIE: Fast Enumeration of Genome-Wide Single- and Multicopy CRISPR Target Sites and Their Off-Target Numbers.JACKIE:基因组中单拷贝和多拷贝 CRISPR 靶位点及其脱靶数量的快速计数。
CRISPR J. 2022 Aug;5(4):618-628. doi: 10.1089/crispr.2022.0042. Epub 2022 Jul 12.
2
Regulating CRISPR/Cas9 Function through Conditional Guide RNA Control.通过条件性向导 RNA 控制来调节 CRISPR/Cas9 功能。
Chembiochem. 2021 Jan 5;22(1):63-72. doi: 10.1002/cbic.202000423. Epub 2020 Nov 17.