<b>Isolation and characterization of insertional mutations in flagellin genes in the archaeon <i>Methanococcus voltae</i></b>

Jarrell, Ken F.; Bayley, Douglas P.; Florian, Volker; Klein, Albrecht

doi:10.1046/j.1365-2958.1996.5371058.x

Cited by 54 publications

(67 citation statements)

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“…In this approach, recombination between a truncated version of the gene and its chromosomal copy leads to an insertion/disruption mutation ( Figure 2B). A targeted version of insertional mutagenesis has been used in M. voltae, to characterise genes encoding flagellins and hydrogenases [95][96][97] . For random mutagenesis, a genomic library of small fragments (less than a full-length gene) is used to target recombination.…”

Section: Transformationmentioning

confidence: 99%

Archaeal genetics — the third way

2005

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| For decades, archaea were misclassified as bacteria on account of their prokaryotic morphology. Molecular phylogeny eventually revealed that archaea, like bacteria and eukaryotes, are a fundamentally distinct domain of life. Genome analyses have confirmed that archaea share many features with eukaryotes, particularly in information processing, and therefore can serve as streamlined models for understanding eukaryotic biology. Biochemists and structural biologists have embraced the study of archaea but geneticists have been more wary, despite the fact that genetic techniques for archaea are quite sophisticated. It is high time for geneticists to start asking fundamental questions about our distant relatives.

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Section: Transformationmentioning

confidence: 99%

Archaeal genetics — the third way

2005

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“…Most genetic studies of methanoarchaea published to date have involved directed mutagenesis of previously identified genes using gene replacement methods (4,(11)(12)(13). Although such studies are invaluable for examining the roles of specific genes in specific functions, they are of limited use in identifying new roles for these genes, because one must have a specific trait in mind when testing the phenotypic consequences of mutations in a given gene.…”

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In vivo transposon mutagenesis of the methanogenic archaeon Methanosarcina acetivorans C2A using a modified version of the insect mariner -family transposable element Himar1

Zhang

Pritchett

Lampe

et al. 2000

Proc. Natl. Acad. Sci. U.S.A.

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We present here a method for in vivo transposon mutagenesis of a methanogenic archaeon, Methanosarcina acetivorans C2A, which because of its independence from host-specific factors may have broad application among many microorganisms. Because there are no known Methanosarcina transposons we modified the mariner transposable element Himar1, originally found in the insect Hematobia irritans, to allow its use in this organism. This element was chosen because, like other mariner elements, its transposition is independent of host factors, requiring only its cognate transposase. Modified mini-Himar1 elements were constructed that carry selectable markers that are functional in Methanosarcina species and that express the Himar1 transposase from known Methanosarcina promoters. These mini-mariner elements transpose at high frequency in M. acetivorans to random sites in the genome. The presence of an Escherichia coli selectable marker and plasmid origin of replication within the mini-mariner elements allows facile cloning of these transposon insertions to identify the mutated gene. In preliminary experiments, we have isolated numerous mini-mariner-induced M. acetivorans mutants, including ones with insertions that confer resistance to toxic analogs and in genes that encode proteins involved in heat shock, nitrogen fixation, and cell-wall structures.

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“…One transcriptional unit contains only flaA; the other, polycistronic transcriptional unit (at least 5.4 kb in length), containing flaB1, flaB2, flaB3, and a number of presumed flagellum accessory genes, initiates at flaB1 and extends to at least the end of flaG (13; D. P. Bayley, J. D. Correia, and K. F. Jarrell, unpublished data). N-terminal (14), transcriptional (13), and mutational (9) analyses have provided evidence that flaB1 and flaB2 encode the major flagellins in M. voltae. Comparison of the N-terminal sequence of one purified flagellin with the amino acid sequence predicted from the gene sequence (13) confirmed the presence of a 12-amino-acid leader peptide.…”

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“…A nonflagellated M. voltae mutant (M. voltae P-2 [9]) was also examined for preflagellin peptidase activity under the standard reaction conditions. This mutant has an insertional vector located in flaB2, which also results in a polar effect on the cotranscribed downstream genes.…”

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Posttranslational Processing ofMethanococcus voltaePreflagellin by Preflagellin Peptidases ofM. voltaeand Other Methanogens

Correia

Jarrell

2000

J Bacteriol

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Methanococcus voltae is a mesophilic archaeon with flagella composed of flagellins that are initially made with 11-or 12-amino-acid leader peptides that are cleaved prior to incorporation of the flagellin into the growing filament. Preflagellin peptidase activity was demonstrated in immunoblotting experiments with flagellin antibody to detect unprocessed and processed flagellin subunits. Escherichia coli membranes containing the expressed M. voltae preflagellin (as the substrate) were combined in vitro with methanogen membranes (as the enzyme source). Correct processing of the preflagellin to the mature flagellin was also shown directly by comparison of the N-terminal sequences of the two flagellin species. M. voltae preflagellin peptidase activity was optimal at 37°C and pH 8.5 and in the presence of 0.4 M KCl with 0.25% (vol/vol) Triton X-100.All of the major subgroupings of archaea, including methanogens, extreme halophiles, and sulfur-dependent thermophiles and hyperthermophiles, have members that possess flagella that look superficially like bacterial flagella (10). However, recent evidence has indicated that the archaeal flagellum is a unique motility structure, distinct from that of bacteria in composition and likely assembly (4, 10). One major distinction is that the assembly of archaeal flagella requires the posttranslational cleavage of a short (11-or 12-amino-acid) leader peptide (2, 13) from the precursor form of the flagellin monomer (preflagellin) before its incorporation into the growing filament. Bacterial flagellins are not made with leader peptides (12).Previously, in Methanococcus voltae, four flagellin genes (flaA, flaB1, flaB2, and flaB3) carried by two transcriptional units were identified (13). One transcriptional unit contains only flaA; the other, polycistronic transcriptional unit (at least 5.4 kb in length), containing flaB1, flaB2, flaB3, and a number of presumed flagellum accessory genes, initiates at flaB1 and extends to at least the end of flaG (13; D. P. Bayley, J. D. Correia, and K. F. Jarrell, unpublished data). N-terminal (14), transcriptional (13), and mutational (9) analyses have provided evidence that flaB1 and flaB2 encode the major flagellins in M. voltae. Comparison of the N-terminal sequence of one purified flagellin with the amino acid sequence predicted from the gene sequence (13) confirmed the presence of a 12-amino-acid leader peptide. Similarly, in the related methanogen Methanococcus vannielii, comparison of the N-terminal sequences obtained from the two major flagellins of purified flagellar filaments with the deduced amino acid sequence of the cloned genes indicated the presence of 12-amino-acid leader peptides on the FlaB1 and FlaB2 flagellins (2). The presence of leader peptides on archaeal flagellins indicated that enzymatic activity must be present in archaeal cells to process the preflagellins.Two different substrates were used for the determination of preflagellin peptidase activity. One preflagellin substrate was prepared by the expression of M. voltae Fla...

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Isolation and characterization of insertional mutations in flagellin genes in the archaeon Methanococcus voltae

Cited by 54 publications

References 26 publications

Archaeal genetics — the third way

Archaeal genetics — the third way

In vivo transposon mutagenesis of the methanogenic archaeon Methanosarcina acetivorans C2A using a modified version of the insect mariner -family transposable element Himar1

Posttranslational Processing ofMethanococcus voltaePreflagellin by Preflagellin Peptidases ofM. voltaeand Other Methanogens

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