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评估靶向基因组无效区域的CRISPR-Cas9 sgRNA的切割效率。

Evaluating the cleavage efficacy of CRISPR-Cas9 sgRNAs targeting ineffective regions of genome.

作者信息

Malik Afsheen, Gul Alvina, Munir Faiza, Amir Rabia, Alipour Hadi, Babar Mustafeez Mujtaba, Bakhtiar Syeda Marriam, Paracha Rehan Zafar, Khalid Zoya, Hayat Muhammad Qasim

机构信息

Department of Plant Biotechnology, Atta-ur-Rahman School of Applied Biosciences, National University of Sciences and Technology, Islamabad, Pakistan.

Department of Plant Production and Genetics, Faculty of Agriculture and Natural Resources, Urmia University, Urmia, Iran.

出版信息

PeerJ. 2021 May 21;9:e11409. doi: 10.7717/peerj.11409. eCollection 2021.

Abstract

The CRISPR-Cas9 system has recently evolved as a powerful mutagenic tool for targeted genome editing. The impeccable functioning of the system depends on the optimal design of single guide RNAs (sgRNAs) that mainly involves sgRNA specificity and on-target cleavage efficacy. Several research groups have designed algorithms and models, trained on mammalian genomes, for predicting sgRNAs cleavage efficacy. These models are also implemented in most plant sgRNA design tools due to the lack of on-target cleavage efficacy studies in plants. However, one of the major drawbacks is that almost all of these models are biased for considering only coding regions of the DNA while excluding ineffective regions, which are of immense importance in functional genomics studies especially for plants, thus making prediction less reliable. In the present study, we evaluate the on-target cleavage efficacy of experimentally validated sgRNAs designed against diverse ineffective regions of genome using various statistical tests. We show that nucleotide preference in protospacer adjacent motif (PAM) proximal region, GC content in the PAM proximal seed region, intact RAR and 3 stem loop structures, and free accessibility of nucleotides in seed and tracrRNA regions of sgRNAs are important determinants associated with their high on-target cleavage efficacy. Thus, our study describes the features important for plant sgRNAs high on-target cleavage efficacy against ineffective genomic regions previously shown to give rise to ineffective sgRNAs. Moreover, it suggests the need of developing an elaborative plant-specific sgRNA design model considering the entire genomic landscape including ineffective regions for enabling highly efficient genome editing without wasting time and experimental resources.

摘要

CRISPR-Cas9系统最近已发展成为一种用于靶向基因组编辑的强大诱变工具。该系统的完美运行取决于主要涉及sgRNA特异性和靶向切割效率的单向导RNA(sgRNA)的优化设计。几个研究小组设计了基于哺乳动物基因组训练的算法和模型,用于预测sgRNA的切割效率。由于缺乏植物中靶向切割效率的研究,这些模型也在大多数植物sgRNA设计工具中得以应用。然而,主要缺点之一是几乎所有这些模型都存在偏差,仅考虑DNA的编码区域而排除无效区域,而这些区域在功能基因组学研究中,尤其是对植物而言非常重要,从而使得预测不太可靠。在本研究中,我们使用各种统计测试评估了针对基因组不同无效区域设计的经实验验证的sgRNA的靶向切割效率。我们表明,原间隔相邻基序(PAM)近端区域的核苷酸偏好、PAM近端种子区域的GC含量完整的RAR和3茎环结构,以及sgRNA种子和反式激活crRNA(tracrRNA)区域中核苷酸的自由可及性是与其高靶向切割效率相关的重要决定因素。因此,我们的研究描述了对于植物sgRNA针对先前显示会产生无效sgRNA的无效基因组区域具有高靶向切割效率而言重要的特征。此外,这表明需要开发一种详尽的植物特异性sgRNA设计模型,该模型考虑包括无效区域在内的整个基因组格局,以便在不浪费时间和实验资源的情况下实现高效的基因组编辑。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/7252/8142926/1f5fa171bf00/peerj-09-11409-g001.jpg

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