Development of genetic methods and construction of a chromosomal glnK1 mutant in Methanosarcina mazei strain Gö1

Ehlers, Claudia; Weidenbach, Katrin; Veit, Katharina; Deppenmeier, Uwe; Metcalf, William W.; Schmitz, Ruth A.

doi:10.1007/s00438-005-1128-7

Cited by 44 publications

(68 citation statements)

References 34 publications

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“…To date, and as far as we know, no PII homologue from a halophilic organism has been studied and the only known representatives from the archaeal domain is M. mazei PII proteins [8,15,16].…”

Section: Introductionmentioning

confidence: 99%

In vitroproof of direct regulation of glutamine synthetase by GlnK proteins in the extreme halophilic archaeonHaloferax mediterranei

Pedro-Roig

Camacho

Bonete

2011

Biochemical Society Transactions

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Haloferax mediterranei is an extreme halophilic micro-organism belonging to the Archaea domain that was isolated from the Santa Pola solar salterns (Alicante, Spain) in 1983. The biochemistry of the proteins involved in nitrogen metabolism is being studied, but the knowledge of their regulation is very scarce at present. The PII superfamily is constituted by major regulators of nitrogen metabolism, which are widespread in prokaryotic and eukaryotic organisms. These trimeric proteins (12 kDa per subunit) have in Escherichia coli long been known to regulate GS (glutamine synthetase) activity via its adenylyltransferase/adenylyl-removing enzyme and, more recently, to be able to interact directly with this enzyme in methanogenic archaea. We have tested the possible role of PII proteins in the regulation of ammonium assimilation in our model organism and the results clearly indicate that the direct influence of GS by PII proteins can also take place in halophilic archaea, starting with the comprehension of nitrogen regulation in those organisms.

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Section: Introductionmentioning

confidence: 99%

In vitroproof of direct regulation of glutamine synthetase by GlnK proteins in the extreme halophilic archaeonHaloferax mediterranei

Pedro-Roig

Camacho

Bonete

2011

Biochemical Society Transactions

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“…An experimental genetic system has been established for this mesophilic methanogen, permitting correlative in vivo studies (24). Further, M. mazei (and Methanosarcina barkeri) possess both redundant pathways for synthesis of CystRNA Cys and three distinct tRNA Cys isoacceptors in their genomes (25,26), suggesting that the properties of SepRS from these organisms may be of particular interest.…”

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confidence: 99%

The Homotetrameric Phosphoseryl-tRNA Synthetase from Methanosarcina mazei Exhibits Half-of-the-sites Activity

Hauenstein

Hou

Perona

2008

Journal of Biological Chemistry

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Synthesis of cysteinyl-tRNACys in methanogenic archaea proceeds by a two-step pathway in which tRNA Cys is first aminoacylated with phosphoserine by phosphoseryl-tRNA synthetase (SepRS). Characterization of SepRS from the mesophile Methanosarcina mazei by gel filtration and nondenaturing mass spectrometry shows that the native enzyme exists as an ␣4 tetramer when expressed at high levels in Escherichia coli. However, active site titrations monitored by ATP/PP i burst kinetics, together with analysis of tRNA binding stoichiometry by fluorescence spectroscopy, show that the tetrameric enzyme binds two tRNAs and that only two of the four chemically equivalent subunits catalyze formation of phosphoseryl adenylate. Therefore, the phenomenon of half-of-the-sites activity, previously described for synthesis of 1 mol of tyrosyl adenylate by the dimeric class I tyrosyl-tRNA synthetase, operates as well in this homotetrameric class II tRNA synthetase. Analysis of cognate and noncognate reactions by ATP/PP i and aminoacylation kinetics strongly suggests that SepRS is able to discriminate against the noncognate amino acids glutamate, serine, and phosphothreonine without the need for a separate hydrolytic editing site. tRNA Cys binding to SepRS also enhances the capacity of the enzyme to discriminate among amino acids, indicating the existence of functional connectivity between the tRNA and amino acid binding sites of the enzyme.

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“…Plasmid DNA was transformed into E. coli according to the method of Inoue et al [14] and into M. mazei using liposome-mediated transformation as described recently [8, 15]. …”

Section: Methodsmentioning

confidence: 99%

“…In order to provide the hpt gene of pRS311 with a strong archaeal promoter, the known p mcr promoter of Methanococcus voltae [9] was cloned upstream of the gene. This was achieved by amplifying p mcr with the primers pmcr BamHI and pmcr XhoI using pRS207 [8] as template. The PCR product was cloned into TOPO-TA-cloning vector pDRIVE (Qiagen, Hilden, Germany) yielding plasmid pRS269.…”

Section: Methodsmentioning

confidence: 99%

“…It serves as an archaeal model for investigating nitrogen stress responses, salt adaptation, methane production from different substrates, energy metabolism, as well as analyzing the role of small RNAs as regulatory elements in stress responses [2–7]. Although it only grows under strictly anaerobic conditions, the organism is genetically tractable and single colonies can be obtained on agar plates, a general requirement for genetic studies [8, 9]. However, genetic manipulation is restricted due to the fact that puromycin is the only selectable marker commercially available for methanoarchaea, which complicates generation of multiple mutations or even complementation experiments.…”

Section: Introductionmentioning

confidence: 99%

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Establishing a Markerless Genetic Exchange System forMethanosarcina mazeiStrain Gö1 for Constructing Chromosomal Mutants of Small RNA Genes

Ehlers

Jäger

Schmitz

2011

Archaea

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A markerless genetic exchange system was successfully established in Methanosarcina mazei strain Gö1 using the hpt gene coding for hypoxanthine phosphoribosyltransferase. First, a chromosomal deletion mutant of the hpt gene was generated conferring resistance to the purine analog 8-aza-2,6-diaminopurine (8-ADP). The nonreplicating allelic exchange vector (pRS345) carrying the pac-resistance cassette for direct selection of chromosomal integration, and the hpt gene for counterselection was introduced into this strain. By a pop-in and ultimately pop-out event of the plasmid from the chromosome, allelic exchange is enabled. Using this system, we successfully generated a M. mazei deletion mutant of the gene encoding the regulatory non-coding RNA sRNA154. Characterizing M. mazeiΔsRNA 154 under nitrogen limiting conditions demonstrated differential expression of at least three cytoplasmic proteins and reduced growth strongly arguing for a prominent role of sRNA154 in regulation of nitrogen fixation by posttranscriptional regulation.

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Development of genetic methods and construction of a chromosomal glnK1 mutant in Methanosarcina mazei strain Gö1

Cited by 44 publications

References 34 publications

In vitroproof of direct regulation of glutamine synthetase by GlnK proteins in the extreme halophilic archaeonHaloferax mediterranei

In vitroproof of direct regulation of glutamine synthetase by GlnK proteins in the extreme halophilic archaeonHaloferax mediterranei

The Homotetrameric Phosphoseryl-tRNA Synthetase from Methanosarcina mazei Exhibits Half-of-the-sites Activity

Establishing a Markerless Genetic Exchange System forMethanosarcina mazeiStrain Gö1 for Constructing Chromosomal Mutants of Small RNA Genes

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