CRISPR-Cas9、CRISPR-Cas12f1和CRISPR-Cas3在根除耐药基因KPC-2和IMP-4方面的比较。

Comparison of CRISPR-Cas9, CRISPR-Cas12f1, and CRISPR-Cas3 in eradicating resistance genes KPC-2 and IMP-4.

作者信息

Huang Jun, Ding Kanghui, Chen Jiahui, Fan Jiao, Huang Luyao, Qiu Shaofu, Wang Ligui, Du Xinying, Wang Chao, Pan Haifeng, Yuan Zhengquan, Liu Hongbo, Song Hongbin

机构信息

Department of Infectious Disease Prevention and Control, Chinese People's Liberation Army Center for Disease Control and Prevention, Beijing, China.

Department of Human Anatomy and Histology, School of Basic Medicine, Capital Medical University, Beijing, China.

出版信息

Microbiol Spectr. 2025 Jun 3;13(6):e0257224. doi: 10.1128/spectrum.02572-24. Epub 2025 Apr 28.

DOI:10.1128/spectrum.02572-24

PMID:40293254

原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC12131857/

Abstract

UNLABELLED

Bacterial plasmid encoding antibiotic resistance could be eradicated by various CRISPR systems, such as CRISPR-Cas9, Cas12f1, and Cas3. However, the efficacy of these gene editing tools against bacterial resistance has not been systematically assessed and compared. This study eliminates carbapenem resistance genes KPC-2 and IMP-4 via CRISPR-Cas9, Cas12f1, and Cas3 systems, respectively. The eradication efficiency of the three CRISPR systems was evaluated. First, the target sites for the three CRISPR systems were designed within the regions 542-576 bp of the KPC-2 gene and 213-248 bp of the IMP-4 gene, respectively. The recombinant CRISPR plasmids were transformed into carrying KPC-2 or IMP-4-encoding plasmid. Colony PCR of transformants showed that KPC-2 and IMP-4 were eradicated by the three different CRISPR systems, and the elimination efficacy was both 100.00%. The drug sensitivity test results showed that the resistant strain was resensitized to ampicillin. In addition, the three CRISPR plasmids could block the horizontal transfer of drug-resistant plasmids, with a blocking rate as high as 99%. Importantly, a qPCR assay was performed to analyze the copy number changes of drug-resistant plasmids in cells. The results indicated that CRISPR-Cas3 showed higher eradication efficiency than CRISPR-Cas9 and Cas12f1 systems.

IMPORTANCE

With the continuous development and application of CRISPR-based resistance removal technologies, CRISPR-Cas9, Cas12f1, and Cas3 have gradually come into focus. However, it remains uncertain which system exhibits more potent efficacy in the removal of bacterial resistance. This study verifies that CRISPR-Cas9, Cas12f1, and Cas3 can eradicate the carbapenem-resistant genes KPC-2 and IMP-4 and restore the sensitivity of drug-resistant model bacteria to antibiotics. Among the three CRISPR systems, the CRISPR-Cas3 system showed the highest eradication efficiency. Although each system has its advantages and characteristics, our results provide guidance on the selection of the CRISPR system from the perspective of resistance gene removal efficiency, contributing to the further application of CRISPR-based bacterial resistance removal technologies.

摘要

未标记

编码抗生素抗性的细菌质粒可被多种CRISPR系统消除，如CRISPR-Cas9、Cas12f1和Cas3。然而，这些基因编辑工具对抗细菌抗性的效果尚未得到系统评估和比较。本研究分别通过CRISPR-Cas9、Cas12f1和Cas3系统消除碳青霉烯抗性基因KPC-2和IMP-4。评估了三种CRISPR系统的消除效率。首先，分别在KPC-2基因的542-576 bp区域和IMP-4基因的213-248 bp区域内设计三种CRISPR系统的靶位点。将重组CRISPR质粒转化到携带KPC-2或IMP-4编码质粒的[具体细菌名称未给出]中。转化子的菌落PCR显示，三种不同的CRISPR系统均消除了KPC-2和IMP-4，消除效率均为100.00%。药敏试验结果表明，耐药[具体细菌名称未给出]菌株对氨苄青霉素重新敏感。此外，三种CRISPR质粒可阻断耐药质粒的水平转移，阻断率高达99%。重要的是，进行了qPCR分析以检测[具体细菌名称未给出]细胞中耐药质粒的拷贝数变化。结果表明，CRISPR-Cas3的消除效率高于CRISPR-Cas9和Cas12f1系统。

重要性

随着基于CRISPR的抗性去除技术的不断发展和应用，CRISPR-Cas9、Cas12f1和Cas3逐渐受到关注。然而，哪种系统在去除细菌抗性方面表现出更强的效果仍不确定。本研究证实，CRISPR-Cas9、Cas12f1和Cas3可消除碳青霉烯抗性基因KPC-2和IMP-4，并恢复耐药模型细菌对抗生素的敏感性。在三种CRISPR系统中，CRISPR-Cas3系统的消除效率最高。尽管每个系统都有其优点和特点，但我们的结果从抗性基因去除效率的角度为CRISPR系统的选择提供了指导，有助于基于CRISPR的细菌抗性去除技术的进一步应用。