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Establishment of a modified CRISPR/Cas9 system with increased mutagenesis frequency using the translational enhancer dMac3 and multiple guide RNAs in potato

机译:使用翻译增强剂DMAC3和马铃薯的多个指导RNA具有增加的诱变频率和多个指导RNA的改进的CRAP / CAS9系统

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CRISPR/Cas9 is a programmable nuclease composed of the Cas9 protein and a guide RNA (gRNA) molecule. To create a mutant potato, a powerful genome-editing system was required because potato has a tetraploid genome. The translational enhancer dMac3, consisting of a portion of the OsMac3 mRNA 5′-untranslated region, greatly enhanced the production of the protein encoded in the downstream ORF. To enrich the amount of Cas9, we applied the dMac3 translational enhancer to the Cas9 expression system with multiple gRNA genes. CRISPR/Cas9 systems targeting the potato granule-bound starch synthase I ( GBSSI ) gene examined the frequency of mutant alleles in transgenic potato plants. The efficiency of the targeted mutagenesis strongly increased when the dMac3-installed Cas9 was used. In this case, the ratio of transformants containing four mutant alleles reached approximately 25% when estimated by CAPS analysis. The mutants that exhibited targeted mutagenesis in the GBSSI gene showed characteristics of low amylose starch in their tubers. This result suggests that our system may facilitate genome-editing events in polyploid plants.
机译:CRISPR / CAS9是由Cas9蛋白和引导RNA(GRNA)分子组成的可编程核酸酶。为了产生突变体马铃薯,需要一种强大的基因组编辑系统,因为马铃薯具有四倍体基因组。由Osmac3 mRNA 5'-未翻译区域的一部分组成的平移增强剂DMAC3大大提高了在下游ORF中编码的蛋白质的产生。为了丰富CAS9的量,我们将DMAC3平移增强剂应用于具有多个GRNA基因的CAS9表达系统。靶向马铃薯颗粒结合淀粉合酶I(GBSSI)基因的CRISPR / CAS9系统检测了转基因马铃薯植物中突变等位基因的频率。当使用DMAC3安装的CAS9时,靶向诱变的效率强烈增加。在这种情况下,当通过帽分析估计时,含有四个突变等位基因的转化体的比例达到约25%。在GBSSI基因中表现出靶向诱变的突变体在其块茎中显示出低硫化淀粉的特征。该结果表明,我们的系统可以促进多倍体植物中的基因组编辑事件。

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