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加氏乳杆菌中基于缺失的CRISPR-Cas9靶向逃逸

Deletion-based escape of CRISPR-Cas9 targeting in Lactobacillus gasseri.

作者信息

Stout Emily A, Sanozky-Dawes Rosemary, Goh Yong Jun, Crawley Alexandra B, Klaenhammer Todd R, Barrangou Rodolphe

机构信息

1​Department of Food, Bioprocessing and Nutrition Sciences, North Carolina State University, Raleigh, NC, USA.

2​Functional Genomics Program, North Carolina State University, Raleigh, NC, USA.

出版信息

Microbiology (Reading). 2018 Sep;164(9):1098-1111. doi: 10.1099/mic.0.000689. Epub 2018 Jul 19.

DOI:10.1099/mic.0.000689
PMID:30024364
Abstract

Lactobacillus gasseri is a human commensal which carries CRISPR-Cas, an adaptive immune system that protects the cell from invasive mobile genetic elements (MGEs). However, MGEs occasionally escape CRISPR targeting due to DNA mutations that occur in sequences involved in CRISPR interference. To better understand CRISPR escape processes, a plasmid interference assay was used to screen for mutants that escape CRISPR-Cas targeting. Plasmids containing a target sequence and a protospacer adjacent motif (PAM) were transformed for targeting by the native CRISPR-Cas system. Although the primary outcome of the assay was efficient interference, a small proportion of the transformed population overcame targeting. Mutants containing plasmids that had escaped were recovered to investigate the genetic routes of escape and their relative frequencies. Deletion of the targeting spacer in the native CRISPR array was the dominant pattern of escape, accounting for 52-70 % of the mutants from two L. gasseri strains. We repeatedly observed internal deletions in the chromosomal CRISPR array, characterized by polarized excisions from the leader end that spanned 1-15 spacers, and systematically included the leader-proximal targeting spacer. This study shows that deletions of spacers within CRISPR arrays constitute a key escape mechanism to evade CRISPR targeting, while preserving the functionality of the CRISPR-Cas system. This mechanism enables cells to maintain an active immune system, but allows the uptake of potentially beneficial plasmids. Our study revealed the co-occurrence of other genomic mutations associated with various phenotypes, showing how this selection process uncovers population diversification.

摘要

加氏乳杆菌是一种人体共生菌,携带CRISPR-Cas,这是一种适应性免疫系统,可保护细胞免受侵入性移动遗传元件(MGEs)的侵害。然而,由于CRISPR干扰相关序列中发生的DNA突变,MGEs偶尔会逃脱CRISPR的靶向作用。为了更好地理解CRISPR逃逸过程,采用了质粒干扰试验来筛选逃脱CRISPR-Cas靶向作用的突变体。含有靶序列和原间隔相邻基序(PAM)的质粒被转化,以便由天然CRISPR-Cas系统进行靶向。尽管该试验的主要结果是有效干扰,但一小部分转化群体克服了靶向作用。回收含有逃脱质粒的突变体,以研究逃逸的遗传途径及其相对频率。天然CRISPR阵列中靶向间隔序列的缺失是主要的逃逸模式,占来自两株加氏乳杆菌突变体的52-70%。我们反复观察到染色体CRISPR阵列中的内部缺失,其特征是从先导端开始的极化切除,跨越1-15个间隔序列,并系统地包括靠近先导端的靶向间隔序列。这项研究表明,CRISPR阵列中间隔序列的缺失构成了逃避CRISPR靶向作用的关键逃逸机制,同时保留了CRISPR-Cas系统的功能。这种机制使细胞能够维持活跃的免疫系统,但允许摄取潜在有益的质粒。我们的研究揭示了与各种表型相关的其他基因组突变的共存,展示了这种选择过程如何揭示群体多样性。

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