Development of broad-host-range vectors for expression of cloned genes in Pseudomonas

Jeffrey M. Werneke; Stephen G. Sligar; Mary A. Schuler

doi:10.1016/0378-1119(85)90205-7

Development of broad-host-range vectors for expression of cloned genes in Pseudomonas

Jeffrey M. Werneke, Stephen G. Sligar, Mary A. Schuler

Research output: Contribution to journal › Article › peer-review

Abstract

The cloning and expression of genes in Pseudomonas have been difficult, until now, due to the absence of vector systems that contain multiple restriction sites downstream from promoter sequences that are functional in Pseudomonas. We report here the construction of several broad-host-range vectors that can be utilized in either Pseudomonas or Escherichia coli and that rely on easily selectable antibiotic resistance markers with multiple cloning sites. These vectors were constructed by inserting the entire pUC13 sequence into derivatives of the RSF1010 wide-host-range plasmid. From this construction, other derivatives were obtained, specifically a lacZ:: Km^R fusion gene which provides an easily selectable marker in both E. coli and Pseudomonas. These vectors have been used to express the Pseudomonas putida cytochrome P450 monoxygenase gene in a P450-deficient P. putida strain. Thus, these vectors allow for the cloning, expression and selection of Pseudomonas genes in Pseudomonas by complementation.

Original language	English (US)
Pages (from-to)	73-84
Number of pages	12
Journal	Gene
Volume	38
Issue number	1-3
DOIs	https://doi.org/10.1016/0378-1119(85)90205-7
State	Published - 1985

Keywords

E. coli host
Recombinant DNA
cytochrome P450 monoxygenase
plasmids
selectable antibiotic-resistance markers
shuttle vehicles

ASJC Scopus subject areas

Genetics

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10.1016/0378-1119(85)90205-7

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title = "Development of broad-host-range vectors for expression of cloned genes in Pseudomonas",

abstract = "The cloning and expression of genes in Pseudomonas have been difficult, until now, due to the absence of vector systems that contain multiple restriction sites downstream from promoter sequences that are functional in Pseudomonas. We report here the construction of several broad-host-range vectors that can be utilized in either Pseudomonas or Escherichia coli and that rely on easily selectable antibiotic resistance markers with multiple cloning sites. These vectors were constructed by inserting the entire pUC13 sequence into derivatives of the RSF1010 wide-host-range plasmid. From this construction, other derivatives were obtained, specifically a lacZ:: KmR fusion gene which provides an easily selectable marker in both E. coli and Pseudomonas. These vectors have been used to express the Pseudomonas putida cytochrome P450 monoxygenase gene in a P450-deficient P. putida strain. Thus, these vectors allow for the cloning, expression and selection of Pseudomonas genes in Pseudomonas by complementation.",

keywords = "E. coli host, Recombinant DNA, cytochrome P450 monoxygenase, plasmids, selectable antibiotic-resistance markers, shuttle vehicles",

author = "Werneke, {Jeffrey M.} and Sligar, {Stephen G.} and Schuler, {Mary A.}",

note = "Funding Information: We would like to thank Dr. I.C. Gunsalus for providingt hep KT230 strainsB, . Ungerf or mapping of Pseudomonas P450 gene,K . Brumbaughfo r help in thec onstructiono f pWS4.Kpn andG . Govind for help with the CO differences pectra. This work was supportedb y grantsN SF-PCM-84-0279f2r omt heN ationalS cienceF oundationa nd grant GM-33775 from the National Instituteso f Health.",

year = "1985",

doi = "10.1016/0378-1119(85)90205-7",

language = "English (US)",

volume = "38",

pages = "73--84",

journal = "Gene",

issn = "0378-1119",

publisher = "Elsevier B.V.",

number = "1-3",

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T1 - Development of broad-host-range vectors for expression of cloned genes in Pseudomonas

AU - Werneke, Jeffrey M.

AU - Sligar, Stephen G.

AU - Schuler, Mary A.

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PY - 1985

Y1 - 1985

N2 - The cloning and expression of genes in Pseudomonas have been difficult, until now, due to the absence of vector systems that contain multiple restriction sites downstream from promoter sequences that are functional in Pseudomonas. We report here the construction of several broad-host-range vectors that can be utilized in either Pseudomonas or Escherichia coli and that rely on easily selectable antibiotic resistance markers with multiple cloning sites. These vectors were constructed by inserting the entire pUC13 sequence into derivatives of the RSF1010 wide-host-range plasmid. From this construction, other derivatives were obtained, specifically a lacZ:: KmR fusion gene which provides an easily selectable marker in both E. coli and Pseudomonas. These vectors have been used to express the Pseudomonas putida cytochrome P450 monoxygenase gene in a P450-deficient P. putida strain. Thus, these vectors allow for the cloning, expression and selection of Pseudomonas genes in Pseudomonas by complementation.

AB - The cloning and expression of genes in Pseudomonas have been difficult, until now, due to the absence of vector systems that contain multiple restriction sites downstream from promoter sequences that are functional in Pseudomonas. We report here the construction of several broad-host-range vectors that can be utilized in either Pseudomonas or Escherichia coli and that rely on easily selectable antibiotic resistance markers with multiple cloning sites. These vectors were constructed by inserting the entire pUC13 sequence into derivatives of the RSF1010 wide-host-range plasmid. From this construction, other derivatives were obtained, specifically a lacZ:: KmR fusion gene which provides an easily selectable marker in both E. coli and Pseudomonas. These vectors have been used to express the Pseudomonas putida cytochrome P450 monoxygenase gene in a P450-deficient P. putida strain. Thus, these vectors allow for the cloning, expression and selection of Pseudomonas genes in Pseudomonas by complementation.

KW - E. coli host

KW - Recombinant DNA

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KW - plasmids

KW - selectable antibiotic-resistance markers

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Development of broad-host-range vectors for expression of cloned genes in Pseudomonas

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