Targeted gene engineering in Clostridium cellulolyticum H10 without methylation

doi:10.1016/j.mimet.2012.02.015

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	Targeted gene engineering in Clostridium cellulolyticum H10 without methylation
	Cui, Gu-zhen 1; Hong, Wei 1; Zhang, Jie 1; Li, Wen-li 2; Feng, Yingang 1; Liu, Ya-jun 1; Cui, Qiu 1
	2012-06-01
发表期刊	JOURNAL OF MICROBIOLOGICAL METHODS
卷号	89 期号:3 页码:201-208
摘要	Genetic engineering of Clostridium cellulolyticum has been developed slowly compared with that of other clostridial species, and one of the major reasons might be the restriction and modification (RM) system which degrades foreign DNA. Here, a putative MspI endonuclease gene, ccel2866, was inactivated by a ClosTron-based gene disruption method. The resulting C. cellulolyticum mutant H10ΔmspI lost the MspI endonuclease activity and can accept unmethylated DNA efficiently. Following that, an oxygen-independent green fluorescence protein gene was introduced into H10ΔmspI without methylation, generating a convenient reporter system to evaluate the expression of heterologous protein in C. cellulolyticum by green fluorescence. To further demonstrate the efficiency of the H10ΔmspI, double mutants H10ΔmspIΔldh and H10ΔmspIΔack were constructed by disrupting lactate dehydrogenase gene ccel2485 and acetate kinase gene ccel2136 in H10ΔmspI, respectively, without DNA methylation, and the stability of the double mutation was confirmed after the 100th generation. The mutant H10ΔmspI constructed here can be used as a platform for further targeted gene manipulation conveniently and efficiently. It will greatly facilitate the metabolic engineering of C. cellulolyticum aiming at faster cellulose degradation and higher biofuel production at the molecular level.; Genetic engineering of Clostridium cellulolyticum has been developed slowly compared with that of other clostridial species, and one of the major reasons might be the restriction and modification (RM) system which degrades foreign DNA. Here, a putative Mspl endonuclease gene, ccel2866, was inactivated by a ClosTron-based gene disruption method. The resulting C cellulolyticum mutant H10 Delta mspl lost the Mspl endonuclease activity and can accept unmethylated DNA efficiently. Following that, an oxygen-independent green fluorescence protein gene was introduced into H10 Delta mspl without methylation, generating a convenient reporter system to evaluate the expression of heterologous protein in C. cellulolyticum by green fluorescence. To further demonstrate the efficiency of the H10 Delta mspl, double mutants H10 Delta mspl Delta ldh and H10 Delta mspl Delta ack were constructed by disrupting lactate dehydrogenase gene ccel2485 and acetate kinase gene ccel2136 in H10 Delta mspl, respectively, without DNA methylation, and the stability of the double mutation was confirmed after the 100th generation. The mutant H10 Delta mspl constructed here can be used as a platform for further targeted gene manipulation conveniently and efficiently. It will greatly facilitate the metabolic engineering of C. cellulolyticum aiming at faster cellulose degradation and higher biofuel production at the molecular level. (c) 2012 Elsevier B.V. All rights reserved.
文章类型	Article
关键词	Methylation-free Clostron Mspl Oxygen-independent Green Fluorescence Protein Lactate Dehydrogenase Acetate Kinase
学科领域	代谢物组学
WOS标题词	Science & Technology ; Life Sciences & Biomedicine
DOI	10.1016/j.mimet.2012.02.015
关键词[WOS]	GROUP-II INTRONS ; ESCHERICHIA-COLI ; BIOFUEL PRODUCTION ; ACETOBUTYLICUM ; TRANSFORMATION ; RESTRICTION ; DNA ; PROTEIN ; THERMOCELLUM ; EXPRESSION
收录类别	SCI
语种	英语
WOS研究方向	Biochemistry & Molecular Biology ; Microbiology
WOS类目	Biochemical Research Methods ; Microbiology
WOS记录号	WOS:000304506700009
引用统计
文献类型	期刊论文
条目标识符	http://ir.qibebt.ac.cn/handle/337004/1225
专题	代谢物组学研究组
作者单位	1.Chinese Acad Sci, Qingdao Inst Bioenergy & Bioproc Technol, Shandong Prov Key Lab Energy Genet, Key Lab Biofuels, Qingdao 266101, Shandong, Peoples R China 2.Ocean Univ China, Key Lab Marine Drugs, Minist Educ, Sch Med & Pharm, Qingdao, Shandong, Peoples R China
推荐引用方式 GB/T 7714	Cui, Gu-zhen,Hong, Wei,Zhang, Jie,et al. Targeted gene engineering in Clostridium cellulolyticum H10 without methylation[J]. JOURNAL OF MICROBIOLOGICAL METHODS,2012,89(3):201-208.
APA	Cui, Gu-zhen.,Hong, Wei.,Zhang, Jie.,Li, Wen-li.,Feng, Yingang.,...&Cui, Qiu.(2012).Targeted gene engineering in Clostridium cellulolyticum H10 without methylation.JOURNAL OF MICROBIOLOGICAL METHODS,89(3),201-208.
MLA	Cui, Gu-zhen,et al."Targeted gene engineering in Clostridium cellulolyticum H10 without methylation".JOURNAL OF MICROBIOLOGICAL METHODS 89.3(2012):201-208.

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