Glycogen in Methanolobus and Methanococcus

König, Helmut

doi:10.1016/0378-1097(85)90093-x

Cited by 12 publications

(15 citation statements)

References 15 publications

Supporting

Mentioning

Contrasting

Order By: Relevance

“…Sibold et al (27) reported hybridization between eubacterial nifHDK probes and DNA from four different methanogenic species. These discoveries were the first confirmed examples of diazotrophy among members of the archaebacteria and have been followed by other descriptions of nitrogen-fixing methanogenic archaebacteria (1,9,13,18 There have been several recent studies on the physiology of diazotrophy in methanogens (1,3,16,18,25). In our previous study on M. barkeri 227 (16) we found similarities to the process in eubacteria, including significant decreases in growth yields and rates when N2 was the N source, stimulation of diazotrophic growth by Mo, and switch-off of C2H2-reducing activity in response to added NH4+.…”

mentioning

confidence: 68%

“…Sibold et al (27) reported hybridization between eubacterial nifHDK probes and DNA from four different methanogenic species. These discoveries were the first confirmed examples of diazotrophy among members of the archaebacteria and have been followed by other descriptions of nitrogen-fixing methanogenic archaebacteria (1,9,13,18). The existence of archaebacterial diazotrophy raises the following question: in light of the structural and functional homology among eubacterial nitrogenases, would archaebacterial nitrogenases be similar to them, or would they have subtle or major differences?…”

mentioning

confidence: 68%

See 1 more Smart Citation

Nitrogenase in the archaebacterium Methanosarcina barkeri 227

Lobo

Zinder

1990

J Bacteriol

View full text Add to dashboard Cite

The discovery of nitrogen fixation in the archaebacterium Methanosarcina barkeri 227 raises questions concerning the similarity of archaebacterial nitrogenases to Mo and alternative nitrogenases in eubacteria. A scheme for achieving a 20-to 40-fold partial purification of nitrogenase components from strain 227 was developed by using protamine sulfate precipitation, followed by using a fast protein liquid chromatography apparatus operated inside an anaerobic glove box. As in eubacteria, the nitrogenase activity was resolved into two components. by strain 227 cells. Antiserum against component 2 of Rhodospirillum rubrum nitrogenase was found to cross-react with component 2 from strain 227, and Western immunoblots using this antiserum showed no evidence for covalent modification of component 2. Also, extracts of strain 227 cells prepared before and after switch-off had virtually the same level of nitrogenase activity. In conclusion, the nitrogenase from strain 227 is similar in overall structure to the eubacterial nitrogenases and shows greatest similarity to alternative nitrogenases.In 1984 to 1985, the property of diazotrophy (nitrogen fixation) was reported in the methanogenic archaebacteria Methanosarcina barkeri 227 (19), Methanococcus thermolithotrophicus (2), and M. barkeri Fusaro (3). Sibold et al. (27) reported hybridization between eubacterial nifHDK probes and DNA from four different methanogenic species. These discoveries were the first confirmed examples of diazotrophy among members of the archaebacteria and have been followed by other descriptions of nitrogen-fixing methanogenic archaebacteria (1,9,13,18 There have been several recent studies on the physiology of diazotrophy in methanogens (1,3,16,18,25). In our previous study on M. barkeri 227 (16) we found similarities to the process in eubacteria, including significant decreases in growth yields and rates when N2 was the N source, stimulation of diazotrophic growth by Mo, and switch-off of C2H2-reducing activity in response to added NH4+. Scherer (25) has demonstrated stimulation of diazoatrophic growth in two strains of M. barkeri by V as well as Mo. We and others have found anomalously low in vivo and in vitro nitrogenase activity, as measured by rates of C2H2 reduction to C2H4 in all diazotrophic methanogens studied thus far (2, 3, 16, 18). The rates measured for methanogen cells and extracts are typically 100-to 500-fold lower than those of typical eubacterial diazotrophs with similar growth rates. One hypothesis considered (16) was that C2H2 was a poorer substrate than N2 for methanogen nitrogenases; another is that methanogen nitrogenases are switched off when assayed (18).We report here the partial purification of nitrogenase from strain 227, a description of its subunit composition, and measurements of its activity toward C2H2 and N2. We also describe more detailed studies on NH4' switch-off and its mechanism in strain 227. 6789on May 13, 2018 by guest

show abstract

mentioning

confidence: 68%

“…Sibold et al (27) reported hybridization between eubacterial nifHDK probes and DNA from four different methanogenic species. These discoveries were the first confirmed examples of diazotrophy among members of the archaebacteria and have been followed by other descriptions of nitrogen-fixing methanogenic archaebacteria (1,9,13,18). The existence of archaebacterial diazotrophy raises the following question: in light of the structural and functional homology among eubacterial nitrogenases, would archaebacterial nitrogenases be similar to them, or would they have subtle or major differences?…”

mentioning

confidence: 68%

Nitrogenase in the archaebacterium Methanosarcina barkeri 227

Lobo

Zinder

1990

J Bacteriol

View full text Add to dashboard Cite

show abstract

“…This microbial ecosystem was selected to investigate, among other questions, whether, under this approach, a hypothetic microorganism capable of producing methane directly from glucose would be competitive over the experimentally reported volatile fatty acid (VFAs) synthesizers in synergy with methane-producing archaea. Methanogens have been reported to possess the biochemical mechanisms to metabolize carbohydrates (König et al, 1985;Murray and Zinder, 1987); however, there is no experimental evidence of any microorganism producing methane directly from a carbohydrate as substrate (Schink, 1997).…”

Section: Resultsmentioning

confidence: 99%

Microbial catabolic activities are naturally selected by metabolic energy harvest rate

González-Cabaleiro

Ofiţeru²,

Lema

et al. 2015

The ISME Journal

View full text Add to dashboard Cite

The fundamental trade-off between yield and rate of energy harvest per unit of substrate has been largely discussed as a main characteristic for microbial established cooperation or competition. In this study, this point is addressed by developing a generalized model that simulates competition between existing and not experimentally reported microbial catabolic activities defined only based on well-known biochemical pathways. No specific microbial physiological adaptations are considered, growth yield is calculated coupled to catabolism energetics and a common maximum biomassspecific catabolism rate (expressed as electron transfer rate) is assumed for all microbial groups. Under this approach, successful microbial metabolisms are predicted in line with experimental observations under the hypothesis of maximum energy harvest rate. Two microbial ecosystems, typically found in wastewater treatment plants, are simulated, namely: (i) the anaerobic fermentation of glucose and (ii) the oxidation and reduction of nitrogen under aerobic autotrophic (nitrification) and anoxic heterotrophic and autotrophic (denitrification) conditions. The experimentally observed cross feeding in glucose fermentation, through multiple intermediate fermentation pathways, towards ultimately methane and carbon dioxide is predicted. Analogously, two-stage nitrification (by ammonium and nitrite oxidizers) is predicted as prevailing over nitrification in one stage. Conversely, denitrification is predicted in one stage (by denitrifiers) as well as anammox (anaerobic ammonium oxidation). The model results suggest that these observations are a direct consequence of the different energy yields per electron transferred at the different steps of the pathways. Overall, our results theoretically support the hypothesis that successful microbial catabolic activities are selected by an overall maximum energy harvest rate.

show abstract

“…Several of these enzymes, including a glycogen debranching enzyme and predicted alpha-1,6-glucosidase activity, are not present in any other known members of class Halobacteria. However, these enzyme activities are frequently found in archaea from classes Methanococci and Thermoplasmata that utilize starch as an internal storage molecule (Kö nig et al, 1985(Kö nig et al, , 1982. This suggests a possible common ancestral origin, with subsequent gene loss in the Halobacteria lineage.…”

Section: Genome Characteristics Of J07ab43 and J07ab56mentioning

confidence: 99%

De novo metagenomic assembly reveals abundant novel major lineage of Archaea in hypersaline microbial communities

Narasingarao¹,

Podell²,

Ugalde³

et al. 2011

The ISME Journal

338

361

View full text Add to dashboard Cite

This study describes reconstruction of two highly unusual archaeal genomes by de novo metagenomic assembly of multiple, deeply sequenced libraries from surface waters of Lake Tyrrell (LT), a hypersaline lake in NW Victoria, Australia. Lineage-specific probes were designed using the assembled genomes to visualize these novel archaea, which were highly abundant in the 0.1-0.8 lm size fraction of lake water samples. Gene content and inferred metabolic capabilities were highly dissimilar to all previously identified hypersaline microbial species. Distinctive characteristics included unique amino acid composition, absence of Gvp gas vesicle proteins, atypical archaeal metabolic pathways and unusually small cell size (approximately 0.6 lm diameter). Multi-locus phylogenetic analyses demonstrated that these organisms belong to a new major euryarchaeal lineage, distantly related to halophilic archaea of class Halobacteria. Consistent with these findings, we propose creation of a new archaeal class, provisionally named 'Nanohaloarchaea'. In addition to their high abundance in LT surface waters, we report the prevalence of Nanohaloarchaea in other hypersaline environments worldwide. The simultaneous discovery and genome sequencing of a novel yet ubiquitous lineage of uncultivated microorganisms demonstrates that even historically well-characterized environments can reveal unexpected diversity when analyzed by metagenomics, and advances our understanding of the ecology of hypersaline environments and the evolutionary history of the archaea.

show abstract

Glycogen in Methanolobus and Methanococcus

Cited by 12 publications

References 15 publications

Nitrogenase in the archaebacterium Methanosarcina barkeri 227

Nitrogenase in the archaebacterium Methanosarcina barkeri 227

Microbial catabolic activities are naturally selected by metabolic energy harvest rate

De novo metagenomic assembly reveals abundant novel major lineage of Archaea in hypersaline microbial communities

Contact Info

Product

Resources

About