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利用线粒体测序技术检测基因编辑和体细胞核移植介导的马匹基因兴奋剂。

Use of mitochondrial sequencing to detect gene doping in horses via gene editing and somatic cell nuclear transfer.

机构信息

Sport and Specialised Analytical Services, LGC, Fordham, UK.

British Horseracing Authority, London, UK.

出版信息

Drug Test Anal. 2022 Aug;14(8):1429-1437. doi: 10.1002/dta.3267. Epub 2022 Apr 25.

DOI:10.1002/dta.3267
PMID:35362263
Abstract

Gene editing and subsequent cloning techniques offer great potential not only in genetic disease correction in domestic animals but also in livestock production by enhancement of desirable traits. The existence of the technology, however, leaves it open to potential misuse in performance-led sports such as horseracing and other equestrian events. Recent advances in equine gene editing, regarding the generation of gene-edited embryos using CRISPR/Cas9 technology and somatic cell nuclear transfer, have highlighted the need to develop tools to detect potential prohibited use of the technology. One possible method involves the characterisation of the mitochondrial genome (which is not routinely preserved during cloning) and comparing it with the sequence of the registered dam. We present here our approach to whole-mitochondrial sequencing using tiled long-range PCR and next-generation sequencing. To determine whether the background mutation rate in the mitochondrial genome could potentially confound results, we sequenced 10 sets of dam and foal duos. We found variation between duos but none within duos, indicating that this method is feasible for future screening systems. Analysis of WGS data from over 100 Thoroughbred horses revealed wide variation in the mitochondria sequence within the breed, further displaying the utility of this approach.

摘要

基因编辑和随后的克隆技术不仅在纠正家畜的遗传疾病方面具有巨大潜力,而且在通过增强理想性状来提高畜牧业生产方面也具有巨大潜力。然而,这项技术的存在使其有可能被滥用于赛马等以性能为导向的运动和其他马术赛事。最近在马的基因编辑方面的进展,涉及使用 CRISPR/Cas9 技术和体细胞核转移来生成基因编辑胚胎,突出了需要开发工具来检测潜在的禁止使用该技术的情况。一种可能的方法涉及对线粒体基因组(在克隆过程中通常不保存)进行特征描述,并将其与注册母马的序列进行比较。我们在这里介绍了使用平铺长距离 PCR 和下一代测序进行全线粒体测序的方法。为了确定线粒体基因组中的背景突变率是否可能混淆结果,我们对 10 对母马和小马驹进行了测序。我们发现了对子之间的差异,但对子内没有差异,这表明这种方法对于未来的筛选系统是可行的。对来自 100 多匹纯血马的 WGS 数据进行分析显示,该品种内线粒体序列存在广泛差异,进一步显示了这种方法的实用性。

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Front Cell Dev Biol. 2023 May 30;11:1225060. doi: 10.3389/fcell.2023.1225060. eCollection 2023.
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Genes (Basel). 2022 Sep 4;13(9):1589. doi: 10.3390/genes13091589.