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用于研究细胞死亡释放的DNA的自然转化和环境归宿的诱导性细胞裂解系统。

Inducible cell lysis system for the study of natural transformation and environmental fate of DNA released by cell death.

作者信息

Kloos D U, Strätz M, Güttler A, Steffan R J, Timmis K N

机构信息

Department of Microbiology, National Research Centre for Biotechnology (GBF), Braunschweig, Germany.

出版信息

J Bacteriol. 1994 Dec;176(23):7352-61. doi: 10.1128/jb.176.23.7352-7361.1994.

Abstract

Two novel conditional broad-host-range cell lysis systems have been developed for the study of natural transformation in bacteria and the environmental fate of DNA released by cell death. Plasmid pDKL02 consists of lysis genes S, R, and Rz from bacteriophage lambda under the control of the Ptac promoter. The addition of inducer to Escherichia coli, Acinetobacter calcoaceticus, or Pseudomonas stutzeri containing plasmid pDKL02 resulted in cell lysis coincident with the release of high amounts of nucleic acids into the surrounding medium. The utility of this lysis system for the study of natural transformation with DNA released from lysed cells was assessed with differentially marked but otherwise isogenic donor-recipient pairs of P. stutzeri JM300 and A. calcoaceticus BD4. Transformation frequencies obtained with lysis-released DNA and DNA purified by conventional methods and assessed by the use of antibiotic resistance (P. stutzeri) or amino acid prototrophy (A. calcoaceticus) for markers were comparable. A second cell lysis plasmid, pDKL01, contains the lysis gene E from bacteriophage phi X174 and causes lysis of E. coli and P. stutzeri bacteria by activating cellular autolysins. Whereas DNA released from pDKL02-containing bacteria persists in the culture broth for days, that from induced pDKL01-containing bacteria is degraded immediately after release. The lysis system involving pDKL02 is thus useful for the study of both the fate of DNA released naturally into the environment by dead cells and gene transfer by natural transformation in the environment in that biochemically unmanipulated DNA containing defined sequences and coding for selective phenotypes can be released into a selected environment at a specific time point. This will allow kinetic measurements that will answer some of the current ecological questions about the fate and biological potential of environmental DNA to be made.

摘要

为了研究细菌中的自然转化以及细胞死亡释放的DNA在环境中的归宿,已经开发了两种新型的条件性广宿主范围细胞裂解系统。质粒pDKL02由来自噬菌体λ的裂解基因S、R和Rz组成,受Ptac启动子控制。向含有质粒pDKL02的大肠杆菌、醋酸钙不动杆菌或施氏假单胞菌中添加诱导剂会导致细胞裂解,同时大量核酸释放到周围培养基中。用施氏假单胞菌JM300和醋酸钙不动杆菌BD4的差异标记但其他方面同基因的供体-受体对评估了该裂解系统在研究裂解细胞释放的DNA自然转化中的效用。用裂解释放的DNA和通过常规方法纯化的DNA获得的转化频率相当,并且通过使用抗生素抗性(施氏假单胞菌)或氨基酸原养型(醋酸钙不动杆菌)作为标记进行评估。第二个细胞裂解质粒pDKL01包含来自噬菌体φX174的裂解基因E,并通过激活细胞自溶素导致大肠杆菌和施氏假单胞菌细菌裂解。虽然从含有pDKL02的细菌释放的DNA在培养液中持续存在数天,但从诱导的含有pDKL01的细菌释放的DNA在释放后立即被降解。因此,涉及pDKL02的裂解系统对于研究死细胞自然释放到环境中的DNA的归宿以及环境中自然转化的基因转移都很有用,因为可以在特定时间点将含有确定序列并编码选择性表型的未经生化操作的DNA释放到选定的环境中。这将允许进行动力学测量,以回答一些当前关于环境DNA的归宿和生物学潜力的生态问题。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/7b35/197125/9555868595d8/jbacter00041-0239-a.jpg

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