嗜热嗜酸绿藻(Crenarchaeon Sulfolobus acidocalarius)一步PCR多基因敲除系统的建立

IF 4.6 Q2 MATERIALS SCIENCE, BIOMATERIALS
ACS Applied Bio Materials Pub Date : 2017-10-31 eCollection Date: 2017-01-01 DOI:10.1155/2017/7459310
Shoji Suzuki, Norio Kurosawa
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引用次数: 13

摘要

嗜热嗜酸的绿古菌(Sulfolobus acidocalarius)的多基因敲除系统是一种强大的遗传工具。然而,质粒的构建通常需要几个步骤。另外,在S. acidocalarius中也开发了用于高通量基因破坏的PCR尾链,但由于缺乏遗传标记系统,基于PCR尾链的重复基因敲除受到限制。本研究通过优化转化条件,获得了高效的同源重组频率(2.8 × 104±6.9 × 103菌落/μg DNA)。优化后的方案可通过短同源臂双交叉进行可靠的基因敲除,并建立一步PCR多基因敲除系统(MONSTER)。在MONSTER中,无需构建质粒,通过一步PCR简单快速地构建了多基因敲除盒,PCR产物可立即用于靶基因的缺失。作为该策略应用的一个例子,我们成功地培育了一株缺乏DNA光解酶- (phr-)和精氨酸脱羧酶- (argD-)的酸藻菌株。此外,还建立了由agmatine-auxotrophic菌株和argD标记组成的agmatine选择系统。MONSTER提供了一种替代策略,可以非常简单地构建用于酸性藻遗传研究的多基因敲除盒。
本文章由计算机程序翻译,如有差异,请以英文原文为准。

Development of the Multiple Gene Knockout System with One-Step PCR in Thermoacidophilic Crenarchaeon <i>Sulfolobus acidocaldarius</i>.

Development of the Multiple Gene Knockout System with One-Step PCR in Thermoacidophilic Crenarchaeon <i>Sulfolobus acidocaldarius</i>.

Development of the Multiple Gene Knockout System with One-Step PCR in Thermoacidophilic Crenarchaeon <i>Sulfolobus acidocaldarius</i>.

Development of the Multiple Gene Knockout System with One-Step PCR in Thermoacidophilic Crenarchaeon Sulfolobus acidocaldarius.

Multiple gene knockout systems developed in the thermoacidophilic crenarchaeon Sulfolobus acidocaldarius are powerful genetic tools. However, plasmid construction typically requires several steps. Alternatively, PCR tailing for high-throughput gene disruption was also developed in S. acidocaldarius, but repeated gene knockout based on PCR tailing has been limited due to lack of a genetic marker system. In this study, we demonstrated efficient homologous recombination frequency (2.8 × 104 ± 6.9 × 103 colonies/μg DNA) by optimizing the transformation conditions. This optimized protocol allowed to develop reliable gene knockout via double crossover using short homologous arms and to establish the multiple gene knockout system with one-step PCR (MONSTER). In the MONSTER, a multiple gene knockout cassette was simply and rapidly constructed by one-step PCR without plasmid construction, and the PCR product can be immediately used for target gene deletion. As an example of the applications of this strategy, we successfully made a DNA photolyase- (phr-) and arginine decarboxylase- (argD-) deficient strain of S. acidocaldarius. In addition, an agmatine selection system consisting of an agmatine-auxotrophic strain and argD marker was also established. The MONSTER provides an alternative strategy that enables the very simple construction of multiple gene knockout cassettes for genetic studies in S. acidocaldarius.

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来源期刊
ACS Applied Bio Materials
ACS Applied Bio Materials Chemistry-Chemistry (all)
CiteScore
9.40
自引率
2.10%
发文量
464
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