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CRISPR/Cas9介导的四倍体马铃薯中微小RNA表达的微调

CRISPR/Cas9-mediated fine-tuning of miRNA expression in tetraploid potato.

作者信息

Lukan Tjaša, Veillet Florian, Križnik Maja, Coll Anna, Mahkovec Povalej Tjaša, Pogačar Karmen, Stare Katja, Chauvin Laura, Chauvin Jean-Eric, Gruden Kristina

机构信息

Department of Biotechnology and Systems Biology, National Institute of Biology, Večna pot 111, Ljubljana, 1000 Slovenia.

IGEPP, INRAE, Institut Agro, Universite ´ de Rennes, Ploudaniel 29260, France.

出版信息

Hortic Res. 2022 Jun 30;9:uhac147. doi: 10.1093/hr/uhac147. eCollection 2022.

Abstract

MicroRNAs (miRNAs) are small noncoding RNAs, which modulate the abundance and spatiotemporal accumulation of target mRNAs at transcriptional and post-transcriptional levels and through that play important roles in several biological processes in plants. Here we show that in polyploid species, CRISPR/Cas9 system can be used for fine-tuning of miRNA expression, which can have broader range of applications compared to knock-out mutants. We established the complete pipeline for CRISPR-Cas9-mediated modulation of miRNA expression in potato. It consists of (1) design and assembly of dual sgRNA CRISPR/Cas9 constructs, (2) transient transfection of protoplasts following fast and efficient screening by high resolution melting analysis to select functional sgRNAs, and (3) stable transformation of potato explants with functional sgRNAs and selection of regenerated transgenic lines with desired mutations and desired miRNA abundance based on sequencing and RT-qPCR. We show that miRNA-editing using dual sgRNA approach results in different types of mutations among transgenic lines but also in different alleles of the same plant, which are target site-dependent. The most frequent were short deletions, but we also detected 1-nt insertions (T or G), deletions between two sgRNAs and larger deletions. miRNA abundance correlates with the frequency and type of introduced mutations, as more extensive mutations in more alleles result in lower miRNA abundance. Interestingly, some mutated loci can generate alternative miRNAs, now novel targets were however predicted for those. In all transgenic lines with expression, we detected mutations, suggesting high efficiency of Cas9-editing. We confirmed the miRNA-editing efficiency of our optimised approach in two different potato genotypes and three different loci.

摘要

微小RNA(miRNA)是一类小的非编码RNA,它们在转录和转录后水平调节靶标mRNA的丰度和时空积累,从而在植物的多个生物学过程中发挥重要作用。在此我们表明,在多倍体物种中,CRISPR/Cas9系统可用于微调miRNA表达,与敲除突变体相比,其应用范围更广。我们建立了CRISPR-Cas9介导的马铃薯miRNA表达调控的完整流程。它包括:(1)双sgRNA CRISPR/Cas9构建体的设计与组装;(2)原生质体的瞬时转染,随后通过高分辨率熔解分析进行快速高效筛选以选择功能性sgRNA;(3)用功能性sgRNA稳定转化马铃薯外植体,并基于测序和RT-qPCR选择具有所需突变和所需miRNA丰度的再生转基因株系。我们表明,使用双sgRNA方法进行miRNA编辑会导致转基因株系间出现不同类型的突变,同一植株的不同等位基因中也会出现不同类型的突变,这些突变取决于靶位点。最常见的是短缺失,但我们也检测到1个核苷酸的插入(T或G)、两个sgRNA之间的缺失以及更大的缺失。miRNA丰度与引入突变的频率和类型相关,因为更多等位基因中更广泛的突变会导致更低的miRNA丰度。有趣的是,一些突变位点可产生替代性miRNA,但尚未预测到这些miRNA的新靶标。在所有具有[此处原文缺失相关内容]表达的转基因株系中,我们都检测到了突变,这表明Cas9编辑效率很高。我们在两种不同的马铃薯基因型和三个不同位点上证实了我们优化方法的miRNA编辑效率。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/5a76/9437727/36099788d76b/uhac147f1.jpg

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