Literature DB >> 18375196

Cell-free protein synthesis system from Escherichia coli cells cultured at decreased temperatures improves productivity by decreasing DNA template degradation.

Eiko Seki1, Natsuko Matsuda, Shigeyuki Yokoyama, Takanori Kigawa.   

Abstract

Cell-free protein synthesis has become one of the standard methods for protein expression. One of the major advantages of this method is that PCR-amplified linear DNA fragments can be directly used as templates for protein synthesis. The productivity of cell-free protein synthesis using linear DNA templates is generally lower than that from plasmid DNA templates, especially when using an Escherichia coli cell extract. In the present study, we found that a simple modification of the protocol for cell extract preparation from E. coli, just by altering the cultivation temperature (37 degrees C) of the cells to a moderately lower range (20-34 degrees C), dramatically reduced the linear DNA degradation activity in the cell extract. This modification greatly improved the productivity of cell-free protein synthesis from linear DNA templates. The removal of the RecD protein, one of the components of exonuclease V, from the extract had almost the same effect, indicating that the linear DNA degradation activity in the extract was mainly due to the RecD protein and that its expression level was decreased at the lower cultivation temperature.

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Year:  2008        PMID: 18375196     DOI: 10.1016/j.ab.2008.03.001

Source DB:  PubMed          Journal:  Anal Biochem        ISSN: 0003-2697            Impact factor:   3.365


  14 in total

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2.  Stable isotope labeling strategy based on coding theory.

Authors:  Takuma Kasai; Seizo Koshiba; Jun Yokoyama; Takanori Kigawa
Journal:  J Biomol NMR       Date:  2015-08-21       Impact factor: 2.835

3.  Cell-free Protein Expression Using the Rapidly Growing Bacterium Vibrio natriegens.

Authors:  Daniel J Wiegand; Henry H Lee; Nili Ostrov; George M Church
Journal:  J Vis Exp       Date:  2019-03-14       Impact factor: 1.355

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Authors:  Xiao Xiao; Yuan Zhou; Yuqiong Sun; Qing Wang; Jianbo Liu; Jin Huang; Xiaobei Zhu; Xiaohai Yang; Kemin Wang
Journal:  Biomicrofluidics       Date:  2018-09-13       Impact factor: 2.800

5.  An economical method for producing stable-isotope labeled proteins by the E. coli cell-free system.

Authors:  Jun Yokoyama; Takayoshi Matsuda; Seizo Koshiba; Takanori Kigawa
Journal:  J Biomol NMR       Date:  2010-11-04       Impact factor: 2.835

6.  CAMSAP2 organizes a γ-tubulin-independent microtubule nucleation centre through phase separation.

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Journal:  Elife       Date:  2022-06-28       Impact factor: 8.713

7.  Glutarate and N-acetyl-L-glutamate buffers for cell-free synthesis of selectively 15N-labelled proteins.

Authors:  Xinying Jia; Kiyoshi Ozawa; Karin Loscha; Gottfried Otting
Journal:  J Biomol NMR       Date:  2009-04-28       Impact factor: 2.835

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Authors:  Ingrid Babel; Rodrigo Barderas; Alberto Peláez-García; J Ignacio Casal
Journal:  BMC Biotechnol       Date:  2011-06-02       Impact factor: 2.563

Review 9.  Escherichia coli Extract-Based Cell-Free Expression System as an Alternative for Difficult-to-Obtain Protein Biosynthesis.

Authors:  Sviatlana Smolskaya; Yulia A Logashina; Yaroslav A Andreev
Journal:  Int J Mol Sci       Date:  2020-01-31       Impact factor: 5.923

10.  Simplification of the genetic code: restricted diversity of genetically encoded amino acids.

Authors:  Akio Kawahara-Kobayashi; Akiko Masuda; Yuhei Araiso; Yoko Sakai; Atsushi Kohda; Masahiko Uchiyama; Shun Asami; Takayoshi Matsuda; Ryuichiro Ishitani; Naoshi Dohmae; Shigeyuki Yokoyama; Takanori Kigawa; Osamu Nureki; Daisuke Kiga
Journal:  Nucleic Acids Res       Date:  2012-08-21       Impact factor: 16.971

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