A simple and reliable method to conduct and monitor expression cassette integration into the <i>Escherichia coli</i> chromosome

Albermann, Christoph; Trachtmann, Natalie; Sprenger, Georg A.

doi:10.1002/biot.200900193

Cited by 42 publications

(34 citation statements)

References 23 publications

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“…For the intracellular synthesis of fucosylated LNTs, the previously described E. coli strain LJ-AY (E. coli LJ110, lacZYA::lgtA-FRT fucIK::lacY-FRT), capable of synthesizing lacto-N-triose II (LNT II), was used as parent strain. 27 By using chromosomal integration technique, 33,34 the Bacteroides fragilis fkp gene (encoding for an L-fucose kinase and L-fucose-1-phosphate guanylyltransferase) 38 was inserted into E. coli LJ-AY, resulting in strain LJ-AYF-cat and strain LJ-AYF (after removal of an antibiotic resistance cassette). In subsequent analysis of intracellular GDP-L-fucose formation by these strains in a manner described before, 13 we found an intracellular level of GDP-L-fucose of about 5 mg per g cellular dry weight, ensuring sufficient substrate supply for the recombinant fucosyltransferase reactions.…”

Section: Strain Constructionmentioning

confidence: 99%

“…antibiotics, the stable, chromosomal integration of recombinant gene expression cassettes can be favorable in terms of process efficiency and product safety. 34 Thus, the gene futC was chromosomally integrated under control of a tac-promoter, which has the advantage that only a single inductor was necessary during synthesis. The resulting strain, E. coli LJ-AYFOC-cat, was cultivated in the same manner as the plasmid carrying strain E. coli LJ-AYFO pCAW55, but without the addition of ampicillin and L-rhamnose.…”

Section: In Vivo Synthesis Of Lnf Imentioning

confidence: 99%

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Synthesis of fucosylated lacto-N-tetraose using whole-cell biotransformation

Baumgärtner

Jurzitza

Conrad

et al. 2015

Bioorganic & Medicinal Chemistry

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Section: Strain Constructionmentioning

confidence: 99%

Section: In Vivo Synthesis Of Lnf Imentioning

confidence: 99%

Synthesis of fucosylated lacto-N-tetraose using whole-cell biotransformation

Baumgärtner

Jurzitza

Conrad

et al. 2015

Bioorganic & Medicinal Chemistry

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“…The expression of each gene is controlled by an IPTG- inducible tac-promoter. The chromosomal insertion of the heterologous expression cassettes were conducted by a method described recently (Albermann et al 2010). This method is based on the k-Redrecombineering technique (Datsenko and Wanner 2000;Zhang et al 1998).…”

Section: Resultsmentioning

confidence: 99%

“…Takara PrimeStar DNA polymerase (Lonza, Belgium) was used for amplification. The chromosomal integration of recombinant crt-gene expression cassettes and elimination of antibiotic resistants gene cassettes using plasmid pCP20 (Cherepanov and Wackernagel 1995) were conduct as described by Albermann et al (2010).…”

Section: Cloning Of the Biosynthesis Genes In E Colimentioning

confidence: 99%

High versus low level expression of the lycopene biosynthesis genes from Pantoea ananatis in Escherichia coli

Albermann

2010

Biotechnol Lett

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The heterologous synthesis of lycopene in non-carotenogenic Escherichia coli required the introduction of the biosynthesis genes crtE, crtB, and crtI. Recombinant E. coli strains, expressing each lycopene biosynthesis gene from Pantoea ananatis using multi-copy plasmid or single-copies after stable chromosomal integration, were cultivated and the formation of lycopene was investigated. The different expression conditions significantly influenced the lycopene formation as well as the growth behaviour. High plasmid expression levels of crtI with a single copy background of crtE and crtB in E. coli led to a predominate synthesis of tetradehydrolycopene at 253 microg g(-1) (cdw).

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“…In addition, we also developed a rapid and efficient method to integrate heterologous genes in the chromosome of E. coli by combining the Red recombination system (Sharan et al 2009;Albermann et al 2010;De Mey et al 2010) and the blue-white screen. Heterologous genes are usually expressed in E. coli using plasmids as the vector.…”

Section: Discussionmentioning

confidence: 99%

Construction of an Escherichia coli mutant producing monophosphoryl lipid A

2011

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Lipid A is a major component in the outer membrane of most gram-negative bacteria. Monophosphoryl lipid A contains no phosphate group at 1-position and can be used as an adjuvant. We constructed an Escherichia coli mutant CW001 by integrating a gene lpxE into the chromosome of E. coli W3110. The gene lpxE encodes an enzyme LpxE which removes the 1-phosphate group of lipid A. CW001 predominantly produces 1-dephosphorylated lipid A in vivo, as adjudged by thin layer chromatography and electro-spray ionization mass spectrometry. This study not only is important for the development of lipid A adjuvants but also provides a novel method for integration of heterologous genes into the chromosome of E. coli.

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A simple and reliable method to conduct and monitor expression cassette integration into the Escherichia coli chromosome

Cited by 42 publications

References 23 publications

Synthesis of fucosylated lacto-N-tetraose using whole-cell biotransformation

Synthesis of fucosylated lacto-N-tetraose using whole-cell biotransformation

High versus low level expression of the lycopene biosynthesis genes from Pantoea ananatis in Escherichia coli

Construction of an Escherichia coli mutant producing monophosphoryl lipid A

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