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在机制毒理学中的功能基因组筛选方法和 CRISPR-Cas9 的潜在未来应用。

Functional genomic screening approaches in mechanistic toxicology and potential future applications of CRISPR-Cas9.

机构信息

Superfund Research Program, Division of Environmental Health Sciences, School of Public Health, University of California, Berkeley, CA 94720, USA.

Superfund Research Program, Division of Environmental Health Sciences, School of Public Health, University of California, Berkeley, CA 94720, USA.

出版信息

Mutat Res Rev Mutat Res. 2015 Apr-Jun;764:31-42. doi: 10.1016/j.mrrev.2015.01.002. Epub 2015 Jan 25.

Abstract

Characterizing variability in the extent and nature of responses to environmental exposures is a critical aspect of human health risk assessment. Chemical toxicants act by many different mechanisms, however, and the genes involved in adverse outcome pathways (AOPs) and AOP networks are not yet characterized. Functional genomic approaches can reveal both toxicity pathways and susceptibility genes, through knockdown or knockout of all non-essential genes in a cell of interest, and identification of genes associated with a toxicity phenotype following toxicant exposure. Screening approaches in yeast and human near-haploid leukemic KBM7 cells have identified roles for genes and pathways involved in response to many toxicants but are limited by partial homology among yeast and human genes and limited relevance to normal diploid cells. RNA interference (RNAi) suppresses mRNA expression level but is limited by off-target effects (OTEs) and incomplete knockdown. The recently developed gene editing approach called clustered regularly interspaced short palindrome repeats-associated nuclease (CRISPR)-Cas9, can precisely knock-out most regions of the genome at the DNA level with fewer OTEs than RNAi, in multiple human cell types, thus overcoming the limitations of the other approaches. It has been used to identify genes involved in the response to chemical and microbial toxicants in several human cell types and could readily be extended to the systematic screening of large numbers of environmental chemicals. CRISPR-Cas9 can also repress and activate gene expression, including that of non-coding RNA, with near-saturation, thus offering the potential to more fully characterize AOPs and AOP networks. Finally, CRISPR-Cas9 can generate complex animal models in which to conduct preclinical toxicity testing at the level of individual genotypes or haplotypes. Therefore, CRISPR-Cas9 is a powerful and flexible functional genomic screening approach that can be harnessed to provide unprecedented mechanistic insight in the field of modern toxicology.

摘要

描述环境暴露反应的程度和性质的可变性是人类健康风险评估的一个关键方面。然而,化学毒物通过许多不同的机制起作用,而且参与不良反应途径 (AOP) 和 AOP 网络的基因尚未得到描述。功能基因组方法可以通过敲低或敲除感兴趣的细胞中的所有非必需基因,以及在毒物暴露后识别与毒性表型相关的基因,揭示毒性途径和易感性基因。酵母和人类近单倍体白血病 KBM7 细胞中的筛选方法已经确定了许多毒物反应中涉及的基因和途径的作用,但受到酵母和人类基因之间部分同源性的限制,以及与正常二倍体细胞的相关性有限。RNA 干扰 (RNAi) 抑制 mRNA 表达水平,但受到脱靶效应 (OTE) 和不完全敲低的限制。最近开发的基因编辑方法称为成簇规律间隔短回文重复相关核酸酶 (CRISPR)-Cas9,可以在 DNA 水平上精确敲除基因组的大多数区域,与 RNAi 相比,OTEs 更少,在多种人类细胞类型中,从而克服了其他方法的局限性。它已被用于鉴定几种人类细胞类型中对化学和微生物毒物反应的基因,并且可以很容易地扩展到对大量环境化学物质的系统筛选。CRISPR-Cas9 还可以抑制和激活基因表达,包括非编码 RNA 的表达,接近饱和,从而有可能更全面地描述 AOP 和 AOP 网络。最后,CRISPR-Cas9 可以生成复杂的动物模型,以便在个体基因型或单倍型水平上进行临床前毒性测试。因此,CRISPR-Cas9 是一种强大而灵活的功能基因组筛选方法,可以用于在现代毒理学领域提供前所未有的机制见解。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/b539/4456615/fa094577f784/nihms658655f1.jpg

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