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CRISPR/Cas9 介导的原生质体无缝基因替换扩展了再生烟草对 TMV-U1 株系的抗性谱。

CRISPR/Cas9-mediated seamless gene replacement in protoplasts expands the resistance spectrum to TMV-U1 strain in regenerated Nicotiana tabacum.

机构信息

National Tobacco Genetic Engineering Research Center, Yunnan Academy of Tobacco Agricultural Sciences, Kunming, Yunnan, China.

BGI-Shenzhen, Shenzhen, Guangdong, China.

出版信息

Plant Biotechnol J. 2023 Dec;21(12):2641-2653. doi: 10.1111/pbi.14159. Epub 2023 Aug 23.

Abstract

CRISPR/Cas-based genome editing is now extensively used in plant breeding and continues to evolve. Most CRISPR/Cas current applications in plants focus on gene knock-outs; however, there is a pressing need for new methods to achieve more efficient delivery of CRISPR components and gene knock-ins to improve agronomic traits of crop cultivars. We report here a genome editing system that combines the advantages of protoplast technologies with recent CRISPR/Cas advances to achieve seamless large fragment insertions in the model Solanaceae plant Nicotiana tabacum. With this system, two resistance-related regions of the N' gene were replaced with homologous fragments from the N'alata gene to confer TMV-U1 resistance in the T0 generation of GMO-free plants. Our study establishes a reliable genome-editing tool for efficient gene modifications and provides a detailed description of the optimization process to assist other researchers adapt this system for their needs.

摘要

基于 CRISPR/Cas 的基因组编辑现在被广泛应用于植物育种,并在不断发展。大多数 CRISPR/Cas 在植物中的当前应用侧重于基因敲除;然而,迫切需要新的方法来更有效地递呈 CRISPR 组件和基因敲入,以提高作物品种的农艺性状。我们在这里报告了一个基因组编辑系统,它结合了原生质体技术的优势和最近的 CRISPR/Cas 进展,以实现模式茄科植物烟草中的无缝大片段插入。利用该系统,将 N'基因的两个与抗性相关的区域用来自 N'alata 基因的同源片段替换,从而在无转基因植物的 T0 代中赋予 TMV-U1 抗性。我们的研究为高效基因修饰建立了一个可靠的基因组编辑工具,并提供了优化过程的详细描述,以帮助其他研究人员根据自己的需要适应该系统。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/e37e/11376799/29419131ed3f/PBI-21-2641-g005.jpg

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