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CasEMBLR:Cas9促进酿酒酵母体内组装的DNA片段进行多位点基因组整合

CasEMBLR: Cas9-Facilitated Multiloci Genomic Integration of in Vivo Assembled DNA Parts in Saccharomyces cerevisiae.

作者信息

Jakočiūnas Tadas, Rajkumar Arun S, Zhang Jie, Arsovska Dushica, Rodriguez Angelica, Jendresen Christian Bille, Skjødt Mette L, Nielsen Alex T, Borodina Irina, Jensen Michael K, Keasling Jay D

机构信息

The Novo Nordisk Foundation Center for Biosustainability, Technical University of Denmark , 2800 Kongens Lyngby, Denmark.

Joint BioEnergy Institute , Emeryville, California 94608, United States.

出版信息

ACS Synth Biol. 2015 Nov 20;4(11):1226-34. doi: 10.1021/acssynbio.5b00007. Epub 2015 Mar 26.

Abstract

Homologous recombination (HR) in Saccharomyces cerevisiae has been harnessed for both plasmid construction and chromosomal integration of foreign DNA. Still, native HR machinery is not efficient enough for complex and marker-free genome engineering required for modern metabolic engineering. Here, we present a method for marker-free multiloci integration of in vivo assembled DNA parts. By the use of CRISPR/Cas9-mediated one-step double-strand breaks at single, double and triple integration sites we report the successful in vivo assembly and chromosomal integration of DNA parts. We call our method CasEMBLR and validate its applicability for genome engineering and cell factory development in two ways: (i) introduction of the carotenoid pathway from 15 DNA parts into three targeted loci, and (ii) creation of a tyrosine production strain using ten parts into two loci, simultaneously knocking out two genes. This method complements and improves the current set of tools available for genome engineering in S. cerevisiae.

摘要

酿酒酵母中的同源重组(HR)已被用于质粒构建和外源DNA的染色体整合。然而,天然的HR机制对于现代代谢工程所需的复杂且无标记的基因组工程来说效率不够高。在此,我们提出了一种用于体内组装DNA片段的无标记多位点整合方法。通过在单、双和三整合位点使用CRISPR/Cas9介导的一步双链断裂,我们报道了DNA片段在体内的成功组装和染色体整合。我们将我们的方法称为CasEMBLR,并通过两种方式验证了其在基因组工程和细胞工厂开发中的适用性:(i)将来自15个DNA片段的类胡萝卜素途径引入三个靶向位点,以及(ii)使用十个片段在两个位点创建酪氨酸生产菌株,同时敲除两个基因。该方法补充并改进了目前可用于酿酒酵母基因组工程的工具集。

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