1887

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Volume 134, Issue 7

Construction of Multicopy Expression Vectors for Regulated Over-production of Proteins in and Other Enteric Bacteria Free

Abstract

A number of expression vectors have been constructed to allow over-production of selected gene products in and other enteric bacteria. The plasmids use the strong hybrid () promoter for gene expression, which is regulated by the allele of the repressor carried on the vector. This provides very tight regulation of gene expression, which is important for over-production of proteins which may be detrimental to cell growth. The vectors carry the standard mpl8 cloning nest in which all the restriction sites are unique to the plasmid (with the exception of RI in pDK7). Derivatives were constructed carrying kanamycin, chloramphenicol or ampillicin resistance as selectable markers, the first two of which are advantageous in due to the high inherent -lactamase activity of this organism.

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© Society for General Microbiology 1988
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1988-07-01
2024-04-27
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References

  1. Amann E., Brosius J., Ptashne M. 1983; Vectors bearing a hybrid trp-lac promoter useful for regulated expression of cloned genes in Escherichia coli. Gene 25:167–178
     [Google Scholar]
  2. Austin S., Henderson N., Dixon R. 1987; Requirements for transcriptional activation in vitro of the nitrogen-regulated glnA and nifLA promoters from Klebsiella pneumoniae: dependence on activator concentration. Molecular Microbiology 1:92–100
     [Google Scholar]
  3. Casadaban M., Cohen S. N. 1980; Analysis of gene control signals by DNA fusion and cloning in Escherichia coli. Journal of Molecular Biology 138:179–207
     [Google Scholar]
  4. Chang A., Cohen S. N. 1978; Construction and characterisation of amplifiable multicopy DNA cloning vehicles derived from the pl5A cryptic miniplasmid. Journal of Bacteriology 134:1141–1156
     [Google Scholar]
  5. Holmes D. S., Quigley M. 1981; A rapid boiling method for the preparation of bacterial plasmids. Analytical Biochemistry 114:193–197
     [Google Scholar]
  6. Hunt T., Magasanik B. 1985; Transcription of glnA by purified Escherichia coli components: core RNA polymerase and the products of glnF, glnG and glnL. Proceedings of the National Academy of Sciences of the United States of America 82:8453–8457
     [Google Scholar]
  7. Maniatis T., Fritsch E. F., Sambrook J. 1982 Molecular Cloning. A Laboratory Manual Cold Spring Harbor, NY: Cold Spring Harbor Laboratory;
     [Google Scholar]
  8. Merrick M. J., Gibbins J. R. 1985; The nucleotide sequence of the nitrogen-regulation gene ntrA of Klebsiella pneumoniae and comparison with conserved features in bacterial RNA polymerase sigma factors. Nucleic Acids Research 13:7607–7620
     [Google Scholar]
  9. Merrick M. J., Gibbins J. R., Postgate J. R. 1987; A rapid and efficient method for plasmid transformation of Klebsiella pneumoniae and Escherichia coli. Journal of General Microbiology 133:2053–2057
     [Google Scholar]
  10. Müller-Hill B., Crapo L., Gilbert W. 1968; Mutants that make more lac repressor. Proceedings of the National Academy of Sciences of the United States of America 59:1259–1264
     [Google Scholar]
  11. Paul W., Merrick M. 1987; The nucleotide sequence of the nifM gene of Klebsiella pneumoniae and identification of a new nif gene - nifZ. European Journal of Biochemistry 170:259–265
     [Google Scholar]
  12. Pouwels PH., Enger-Valk B. E., Brammar W. J. 1985 Cloning Vectors. A Laboratory Manual Amsterdam: Elsevier;
     [Google Scholar]
  13. Remaut E., Stanssens P., Fiers W. 1981; Plasmid vectors for high-efficiency expression controlled by the pL promoter of coliphage lambda. Gene 15:81–93
     [Google Scholar]
  14. Spratt B. G., Hedge P. J., Te Heesen S., Edelman A., Broome-Smith J. K. 1986; Kanamycin- resistant vectors that are analogues of plasmids pUC8, pUC9, pEMBL8 and pEMBL9. Gene 41:337–342
     [Google Scholar]
  15. Stark M. J. R. 1987; Multicopy expression vectors carrying the lac repressor gene for regulated high- level expression of genes in Escherichia coli. Gene 51:255–267
     [Google Scholar]
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Construction of Multicopy Expression Vectors for Regulated Over-production of Proteins in Klebsiella pneumoniae and Other Enteric Bacteria
Microbiology 134, 1779 (1988); https://doi.org/10.1099/00221287-134-7-1779
/content/journal/micro/10.1099/00221287-134-7-1779
/content/journal/micro/10.1099/00221287-134-7-1779
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