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通过对多个基因进行纯合编辑以加速异种移植猪的培育

Homozygous editing of multiple genes for accelerated generation of xenotransplantation pigs.

作者信息

Duan Xiaoyue, Chen Chaolei, Du Chang, Guo Liang, Liu Jun, Hou Naipeng, Li Pan, Qi Xiaolan, Gao Fei, Du Xuguang, Song Jiangping, Wu Sen

机构信息

Sanya Institute of China Agricultural University, Sanya, 572024, China.

State Key Laboratory of Animal Biotech Breeding, College of Biological Sciences, China Agricultural University, Beijing 100193, China.

出版信息

Genome Res. 2025 May 2;35(5):1167-1178. doi: 10.1101/gr.279709.124.

Abstract

Although CRISPR-Cas-based genome editing has made significant strides over the past decade, achieving simultaneous homozygous gene editing of multiple targets in primary cells remains a significant challenge. In this study, we optimized a coselection strategy to enhance homozygous gene editing rates in the genomes of primary porcine fetal fibroblasts (PFFs). The strategy utilizes the expression of a surrogate reporter () to select for cells with the highest reporter expression, thereby improving editing efficiency. For simultaneous multigene editing, we targeted the most challenging site for selection, whereas other target sites did not require selection. Using this approach, we successfully obtained single-cell PFF clones (three of 10) with seven or more homozygously edited genes, including , , , , , , and Importantly, cells edited using this strategy can be efficiently used for somatic cell nuclear transfer (SCNT) to generate healthy xenotransplantation pigs in <5 months, a process that previously required years of breeding or multiple rounds of SCNT.

摘要

尽管基于CRISPR-Cas的基因组编辑在过去十年中取得了重大进展,但在原代细胞中实现多个靶点的同时纯合基因编辑仍然是一项重大挑战。在本研究中,我们优化了一种共选择策略,以提高原代猪胎儿成纤维细胞(PFFs)基因组中的纯合基因编辑率。该策略利用替代报告基因()的表达来选择报告基因表达最高的细胞,从而提高编辑效率。对于同时进行多基因编辑,我们针对最具挑战性的选择位点,而其他靶位点则不需要选择。使用这种方法,我们成功获得了单细胞PFF克隆(10个中有3个),其中包含7个或更多纯合编辑基因,包括、、、、、、和。重要的是,使用该策略编辑的细胞可有效地用于体细胞核移植(SCNT),在不到5个月的时间内培育出健康的异种移植猪,而此前这一过程需要数年的繁殖或多轮SCNT。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/e5bc/12047534/faf397091537/1167f01.jpg

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