Development of improved versatile broad-host-range vectors for use in methylotrophs and other Gram-negative bacteria The GenBank accession numbers for the sequences reported in this paper are AF327711, AF327712, AF327713, AF327714, AF327715, AF327716, AF327717, AF327718, AF327719 and AF327720.

Marx, Christopher J.; Lidstrom, Mary E.

doi:10.1099/00221287-147-8-2065

Cited by 314 publications

(236 citation statements)

References 37 publications

(44 reference statements)

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“…Genome sequence data obtained as described above were used to design PCR primers for the amplification of the wild-type gene. Products of the expected sizes were obtained and isolated, cloned directly into pCR2.1 and subcloned downstream of the P mxaF promoter in the M. extorquens AM1 expression vector pCM80 (Marx & Lidstrom, 2001) as either EcoRI-EcoRI or XbaI-KpnI fragments.…”

Section: Methodsmentioning

confidence: 99%

“…The recent availability of the M. extorquens AM1 genome sequence along with the advent of genetic tools for the construction of insertion mutants (Chistoserdov et al, 1994) and the overexpression of genes (Marx & Lidstrom, 2001) now enable the application of genomic approaches to the understanding of metabolic pathways in this organism. In a previous study, five genes predicted to be involved in growth on succinate or pyruvate encoding citrate synthase, succinate dehydrogenase, malic enzyme, phosphoenolpyruvate synthase and phosphoenolpyruvate carboxykinase were identified in the genome sequence.…”

Section: Introductionmentioning

confidence: 99%

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Reconstruction of C3 and C4 metabolism in Methylobacterium extorquens AM1 using transposon mutagenesis

et al. 2003

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The growth of Methylobacterium extorquens AM1 on C 1 compounds has been well-studied, but little is known about how this methylotroph grows on multicarbon compounds. A Tn5 transposon mutagenesis procedure was performed to identify genes involved in the growth of M. extorquens AM1 on succinate and pyruvate. Of the 15 000 insertion colonies screened, 71 mutants were found that grew on methanol but either grew slowly or were unable to grow on one or both of the multicarbon substrates. For each of these mutants, the chromosomal region adjacent to the insertion site was sequenced, and 55 different genes were identified and assigned putative functions. These genes fell into a number of predicted categories, including central carbon metabolism, carbohydrate metabolism, regulation, transport and non-essential housekeeping functions. This study focused on genes predicted to encode enzymes of central heterotrophic metabolism: 2-oxoglutarate dehydrogenase, pyruvate dehydrogenase and NADH : ubiquinone oxidoreductase. In each case, the mutants showed normal growth on methanol and impaired growth on pyruvate and succinate, consistent with a role specific to heterotrophic metabolism. For the first two cases, no detectable activity of the corresponding enzyme was found in the mutant, verifying the predictions. The results of this study were used to reconstruct multicarbon metabolism of M. extorquens AM1 during growth on methanol, succinate and pyruvate.

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Section: Methodsmentioning

confidence: 99%

Section: Introductionmentioning

confidence: 99%

Reconstruction of C3 and C4 metabolism in Methylobacterium extorquens AM1 using transposon mutagenesis

et al. 2003

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“…The spectinomycin-resistance gene was amplified with pSJS985Q (Sandler & Clark, 1994) as a template and primers 59-TCGAATTCACAGGATGACGCCTAAC-39 and 59-TC-CTCGAGTCTAACGCTTGAGTTAA-39 (EcoRI and XhoI sites are underlined). The HindIII-EcoRI fragment of the rpoH gene and the EcoRI-XhoI fragment of the spectinomycin-resistance gene were cloned into the XhoI-HindIII fragment from pCM66 (Marx & Lidstrom, 2001). The resultant plasmid was introduced into the rpoH mutant by electroporation (Coppi et al, 2001).…”

Section: Methodsmentioning

confidence: 99%

Heat-shock sigma factor RpoH from Geobacter sulfurreducens

Ueki

Lovley

2007

Microbiology

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Recent studies with Myxococcus xanthus have suggested that homologues of the Escherichia coli heat-shock sigma factor, RpoH, may not be involved in the heat-shock response in this d-proteobacterium. The genome of another d-proteobacterium, Geobacter sulfurreducens, which is considered to be a representative of the Fe(III)-reducing Geobacteraceae that predominate in a diversity of subsurface environments, contains an rpoH homologue. Characterization of the G. sulfurreducens rpoH homologue revealed that it was induced by a temperature shift from 30 6C to 42 6C and that an rpoH-deficient mutant was unable to grow at 42 6C. The predicted heat-shock genes, hrcA, grpE, dnaK, groES and htpG, were heat-shock inducible in an rpoH-dependent manner, and comparison of promoter regions of these genes identified the consensus sequences for the "10 and "35 promoter elements. In addition, DNA elements identical to the CIRCE consensus sequence were found in promoters of rpoH, hrcA and groES, suggesting that these genes are regulated by a homologue of the repressor HrcA, which is known to bind the CIRCE element. These results suggest that the G. sulfurreducens RpoH homologue is the heat-shock sigma factor and that heat-shock response in G. sulfurreducens is regulated positively by RpoH as well as negatively by the HrcA/CIRCE system. INTRODUCTIONThe Gram-negative d-proteobacterium Geobacter sulfurreducens is considered to be a representative of the Fe(III)-reducing Geobacteraceae that predominate in a diversity of subsurface environments where Fe(III) reduction is important . Geobacter species also play critical roles in bioremediation of groundwater contaminated with organic compounds or metals (Lloyd & Lovley, 2001;Lovley, 1997Lovley, , 2003Lovley & Coates, 1997, 2000 and in electricity production from waste organic matter (Bond et al., 2002;Bond & Lovley, 2003; Lovley, 2006a, b). However, the mechanisms they use to deal with the multiple stresses they encounter in these environments are poorly understood.Geobacter species face various environmental changes and growth conditions in the subsurface. Heat shock is a common stress to which all organisms adapt by inducing heat-shock proteins. Many heat-shock proteins are well conserved among organisms (Arrigo & Iandry, 1994;Lindquist & Craig, 1998). In bacteria, the expression of heat-shock genes is regulated in various fashions (Gross, 1996;Hecker et al., 1996;Narberhaus, 1999;Rosen & Ron, 2002;Schumann, 2000Schumann, , 2003Servant & Mazodier, 2001;Yura et al., 2000). The Gram-negative bacterium Escherichia coli uses two sigma factors, RpoH and RpoE, to activate transcription of heat-shock genes (Gross, 1996;Yura et al., 2000). The sigma factor, which is a subunit of RNA polymerase (RNAP), recognizes specific promoter elements and is essential for initiation of transcription. RpoHdependent transcription is also found in other Gramnegative bacteria (Gross, 1996;Yura et al., 2000;Rosen & Ron, 2002). The regulation of heat-shock gene expression in the Gram-positive bacterium Bacillus s...

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“…In order to test this hypothesis, the mxaF A-tract sequence, AAGAAA, was inserted 17 bp upstream of the E. coli lac promoter in the promoter-probe vector pCM130. The lac promoter had been previously shown to be a weak promoter in M. extorquens AM1 (Marx & Lidstrom, 2001). The cloned tac promoter had an activity of 56-60 mU, while the construct containing the AAGAAA showed an increase to 128-180 mU.…”

Section: Use Of the A-tract Sequence As An Enhancer Elementmentioning

confidence: 99%

Identification of an upstream regulatory sequence that mediates the transcription of mox genes in Methylobacterium extorquens AM1

2005

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A multiple A-tract sequence has been identified in the promoter regions for the mxaF, pqqA, mxaW, mxbD and mxcQ genes involved in methanol oxidation in Methylobacterium extorquens AM1, a facultative methylotroph. Site-directed mutagenesis was exploited to delete or change this conserved sequence. Promoter-xylE transcriptional fusions were used to assess promoter activity in these mutants. A fiftyfold drop in the XylE activity was observed for the mxaF and pqqA promoters without this sequence, and a five-to sixfold drop in the XylE activity was observed for the mxbD and mxcQ promoters without this sequence. Mutants were generated in the chromosomal copies in which this sequence was either deleted or altered, and these mutants were unable to grow on methanol. When one of these sequences was added to Plac of Escherichia coli, which is a weak constitutive promoter in M. extorquens AM1, the activity increased two-to threefold. These results suggest that this sequence is essential for normal expression of these genes in M. extorquens AM1, and may serve as a general enhancer element for genetic constructs in this bacterium. INTRODUCTIONMethylobacterium extorquens AM1 (Peel & Quayle, 1961) is a facultative methylotroph that is able to use C 1 compounds as its sole carbon and energy source (Anthony, 1982(Anthony, , 2000Lidstrom, 1991). It can also grow on multi-carbon compounds such as pyruvate and succinate. M. extorquens AM1 is one of the most intensively studied methylotrophs (Chistoserdova et al., 2003) and recently a gapped genome sequence has been made available for this organism (http:// www.integratedgenomics.com/genomereleases.html#list6). Methylotrophic metabolism in M. extorquens AM1 begins with the oxidation of methanol or methylamine to formaldehyde in the periplasm (Anthony, 1982). Further assimilation and dissimilation of formaldehyde occur in the cytoplasm (Marx et al., 2003). Methanol oxidation is carried out by the enzyme methanol dehydrogenase, which is a quinoprotein using pyrroloquinoline quinone (PQQ) as a prosthetic group, and is an a 2 b 2 heterotetramer coupled to a specific cytochrome c accepter (Anthony, 1982). Methanol dehydrogenase activity and proteins have been shown to be regulated by carbon source in M. extorquens AM1, with three-to sixfold higher levels in the presence of methanol than during growth on multicarbon substrates in the absence of C 1 compounds (Nunn & Lidstrom, 1986a, b).At least 25 genes have been identified to be involved in the methanol oxidation reaction in M. extorquens AM1 (Lidstrom, 1991;Zhang & Lidstrom, 2003). These Mox genes are distributed between three different loci: mxa, mxb and mxc. Fourteen genes (mxaFJGIRSACKLDEHB) transcribed in the same direction, together with an additional gene (mxaW) transcribed in the opposite direction, are located on the mxa gene cluster (Anderson et al., 1990;Morris et al., 1995;Springer et al., 1998Springer et al., , 1995. The large and small subunits of methanol dehydrogenase are encoded by mxaF and mxaI, respectively (Anderson & ...

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Development of improved versatile broad-host-range vectors for use in methylotrophs and other Gram-negative bacteria The GenBank accession numbers for the sequences reported in this paper are AF327711, AF327712, AF327713, AF327714, AF327715, AF327716, AF327717, AF327718, AF327719 and AF327720.

Cited by 314 publications

References 37 publications

Reconstruction of C3 and C4 metabolism in Methylobacterium extorquens AM1 using transposon mutagenesis

Reconstruction of C3 and C4 metabolism in Methylobacterium extorquens AM1 using transposon mutagenesis

Heat-shock sigma factor RpoH from Geobacter sulfurreducens

Identification of an upstream regulatory sequence that mediates the transcription of mox genes in Methylobacterium extorquens AM1

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