Novel and Engineered Type II CRISPR Systems from Uncultivated Microbes with Broad Genome Editing Capability.

IF 3.7 4区生物学 Q2 GENETICS & HEREDITY

CRISPR Journal Pub Date : 2023-06-01 DOI:10.1089/crispr.2022.0090

Lisa M Alexander, Daniela S Aliaga Goltsman, Jason Liu, Jyun-Liang Lin, Morayma M Temoche-Diaz, Sarah M Laperriere, Andreas Neerincx, Christien Bednarski, Philipp Knyphausen, Andre Cohnen, Justine Albers, Liliana Gonzalez-Osorio, Rodrigo Fregoso Ocampo, Jennifer Oki, Audra E Devoto, Cindy J Castelle, Rebecca C Lamothe, Gregory J Cost, Cristina N Butterfield, Brian C Thomas, Christopher T Brown

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引用次数: 1

Abstract

Type II Clustered Regularly Interspaced Short Palindromic Repeats (CRISPR)-Cas9 nucleases have been extensively used in biotechnology and therapeutics. However, many applications are not possible owing to the size, targetability, and potential off-target effects associated with currently known systems. In this study, we identified thousands of CRISPR type II effectors by mining an extensive, genome-resolved metagenomics database encompassing hundreds of thousands of microbial genomes. We developed a high-throughput pipeline that enabled us to predict tracrRNA sequences, to design single guide RNAs, and to demonstrate nuclease activity in vitro for 41 newly described subgroups. Active systems represent an extensive diversity of protein sequences and guide RNA structures and require diverse protospacer adjacent motifs (PAMs) that collectively expand the known targeting capability of current systems. Several nucleases showed activity levels comparable to or significantly higher than SpCas9, despite being smaller in size. In addition, top systems exhibited low levels of off-target editing in mammalian cells, and PAM-interacting domain engineered chimeras further expanded their targetability. These newly discovered nucleases are attractive enzymes for translation into many applications, including therapeutics.

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来自具有广泛基因组编辑能力的未培养微生物的新型和工程化II型CRISPR系统。

II型集群规则间隔短回文重复(CRISPR)-Cas9核酸酶已广泛应用于生物技术和治疗学。然而，由于当前已知系统的大小、可靶向性和潜在的脱靶效应，许多应用程序都不可能实现。在这项研究中，我们通过挖掘包含数十万个微生物基因组的广泛的基因组解析元基因组数据库，鉴定了数千个CRISPR II型效应物。我们开发了一个高通量管道，使我们能够预测tracrRNA序列，设计单个引导rna，并在体外证明41个新描述的亚群的核酸酶活性。活性系统代表了蛋白质序列和引导RNA结构的广泛多样性，并且需要不同的原间隔邻近基序(PAMs)，这些基序共同扩展了当前系统的已知靶向能力。几种核酸酶显示出与SpCas9相当或显著高于SpCas9的活性水平，尽管它们的大小更小。此外，顶级系统在哺乳动物细胞中表现出低水平的脱靶编辑，pam相互作用结构域工程嵌合体进一步扩大了它们的靶向性。这些新发现的核酸酶是有吸引力的酶，可以翻译成许多应用，包括治疗。

本文章由计算机程序翻译，如有差异，请以英文原文为准。

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来源期刊

CRISPR Journal Biochemistry, Genetics and Molecular Biology-Biotechnology

CiteScore

6.30

自引率

2.70%

发文量

期刊介绍： In recognition of this extraordinary scientific and technological era, Mary Ann Liebert, Inc., publishers recently announced the creation of The CRISPR Journal -- an international, multidisciplinary peer-reviewed journal publishing outstanding research on the myriad applications and underlying technology of CRISPR. Debuting in 2018, The CRISPR Journal will be published online and in print with flexible open access options, providing a high-profile venue for groundbreaking research, as well as lively and provocative commentary, analysis, and debate. The CRISPR Journal adds an exciting and dynamic component to the Mary Ann Liebert, Inc. portfolio, which includes GEN (Genetic Engineering & Biotechnology News) and more than 80 leading peer-reviewed journals.