A review of bacterial methyl halide degradation: biochemistry, genetics and molecular ecology

McDonald, Ian R.; Warner, Karen L.; McAnulla, Craig; Woodall, Claire A.; Oremland, Ronald S.; Murrell, J. Colin

doi:10.1046/j.1462-2920.2002.00290.x

Cited by 66 publications

(63 citation statements)

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“…Methyl halides are known to be produced in seawater by marine microorganisms (32)(33)(34)(35). Some methyl halides are known to be chemically removed from seawater by nucleophilic attack (36), hydrolysis (37), and bacteria (38)(39)(40). The observed decrease in CH 3 I was negatively correlated with CO 2 uptake and O 2 ( Table 1).…”

Section: Resultsmentioning

confidence: 99%

Changing concentrations of CO, CH ₄ , C ₅ H ₈ , CH ₃ Br, CH ₃ I, and dimethyl sulfide during the Southern Ocean Iron Enrichment Experiments

Wingenter

Haase

Strutton

et al. 2004

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

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Oceanic iron (Fe) fertilization experiments have advanced the understanding of how Fe regulates biological productivity and air-sea carbon dioxide (CO2) exchange. However, little is known about the production and consumption of halocarbons and other gases as a result of Fe addition. Besides metabolizing inorganic carbon, marine microorganisms produce and consume many other trace gases. Several of these gases, which individually impact global climate, stratospheric ozone concentration, or local photochemistry, have not been previously quantified during an Feenrichment experiment. We describe results for selected dissolved trace gases including methane (CH4), isoprene (C5H8), methyl bromide (CH 3Br), dimethyl sulfide, and oxygen (O2), which increased subsequent to Fe fertilization, and the associated decreases in concentrations of carbon monoxide (CO), methyl iodide (CH 3I), and CO 2 observed during the Southern Ocean Iron Enrichment Experiments. P revious iron (Fe) fertilization experiments have been conducted in the North (1) and equatorial Pacific (2, 3) and in the Southern Ocean (4, 5). The Southern Ocean, the largest of the high-nutrient low-chlorophyll regions, represents 6% of the global ocean and has the potential to enhance carbon sequestration by Fe fertilization (6-9), which could slow carbon dioxide (CO 2 ) accumulation in the atmosphere and potentially help alleviate global warming. Experimental MethodsThe experimental design and other results of the Southern Ocean Iron Enrichment Experiment (SOFeX) are presented in an overview paper (8). Of the two regions fertilized with Fe during SOFeX, we focus here on the region north of the Antarctic Polar Front. An area Ϸ15 ϫ 15 km at 56.2°S, 172.0°W (southeast of New Zealand in the southwest Pacific sector of the Southern Ocean) was fertilized with a solution of acidified iron sulfate (FeSO 4 ) over 48 h to a concentration of Ϸ1.2 ϫ 10 Ϫ9 mol⅐liter Ϫ1 (1.2 nM) beginning on January 12, 2002. The background Fe concentration ([Fe]) was Ϸ0.1 nM. A second (36 h) application of FeSO 4 (Ϸ1.2 nM) ended on January 17. These Fe additions were intended to simulate glacial era concentrations of iron in the Southern Ocean (8, 10). The region, or patch, was allowed time to bloom and then was surveyed over a 50-h period, between February 8 and 10, 4 weeks after the first Fe application. By this time the patch had reached a surface area that was a factor of 10 larger than during the initial Fe addition with iron concentrations in the patch of Ϸ0.3 nM (8). During this survey we approached the patch from the South working our way northeast, while crisscrossing the patch. After the shape and orientation of the patch became apparent [elongated and stretching from the southwest to the northeast (11)], more intensive sampling began along the patch. Observations of fluorescence, the partial pressure of CO 2 in seawater (pCO 2 ) (Fig. 1A), dissolved O 2 (Fig. 1B), chlorophyll, and primary productivity indicated a pronounced change in biological activity in the mixed layer (upper 40-5...

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Section: Resultsmentioning

confidence: 99%

Changing concentrations of CO, CH ₄ , C ₅ H ₈ , CH ₃ Br, CH ₃ I, and dimethyl sulfide during the Southern Ocean Iron Enrichment Experiments

Wingenter

Haase

Strutton

et al. 2004

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

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“…A wide range of C 1 compounds are consumed by methylotrophs in the environment, including methane, methanol, methylated amines, methylated glycines, halomethanes, and methylated sulfur species (1,21,24,31,44). Traditional microbial techniques such as enrichment and isolation on defined culture media have revealed that methylotrophic bacteria occur in a variety of environments, such as freshwater, marine, and terrestrial habitats, including habitats characterized by extreme conditions of temperature, salinity, or pH (8,26,44).…”

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confidence: 99%

“…As many methylotrophic bacteria are difficult to isolate, cultivation-independent molecular tools have been developed to characterize natural methylotrophic populations. These tools included oligonucleotide probes and PCR primer sets targeting genes conserved among methylotrophic bacteria, such as 16S RNA genes, or genes encoding specific methylotrophic enzymes, such as particulate and soluble methane monooxygenases, methanol dehydrogenase, corrinoid-linked methyltransferase, or methanesulfonic acid monooxygenase (3,15,21,30,31). However, none of these probes or primers aimed at detection of C 1 -oxidizing populations in a broader sense, encompassing their actual diversity.…”

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Bacterial Populations Active in Metabolism of C ₁ Compounds in the Sediment of Lake Washington, a Freshwater Lake

Nercessian¹,

Noyes

Kalyuzhnaya³

et al. 2005

Appl Environ Microbiol

210

161

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“…strain IMB-1 (41) were shown to be able to oxidize tropospheric concentrations of CH 3 Br (12 pptv), indicating that these and other methyl halide utilizers are responsible for the biological oxidation of tropospheric CH 3 Br and possibly CH 3 Cl in various terrestrial and marine environments (15). This also indicated that ambient concentrations of CH 3 Br and possibly CH 3 Cl were adequate for the induction of methyl halide utilization pathway(s).All four CH 3 Cl-utilizing soil isolates were found to possess the gene cmuA along with other CH 3 Cl-specific genes within their cmu (chloromethane utilization) gene clusters (6,31,32,50,54). The cmuA gene encodes methyltransferase I (CmuA), which catalyzes the initial dehalogenation step of the CH 3 Cl degradation pathway (Fig.…”

mentioning

confidence: 87%

“…All four CH 3 Cl-utilizing soil isolates were found to possess the gene cmuA along with other CH 3 Cl-specific genes within their cmu (chloromethane utilization) gene clusters (6,31,32,50,54). The cmuA gene encodes methyltransferase I (CmuA), which catalyzes the initial dehalogenation step of the CH 3 Cl degradation pathway (Fig.…”

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Chloromethane-Dependent Expression of the cmu Gene Cluster of Hyphomicrobium chloromethanicum

Borodina

McDonald

Murrell

2004

Appl Environ Microbiol

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The methylotrophic bacterium Hyphomicrobium chloromethanicum CM2 can utilize chloromethane (CH 3 Cl) as the sole carbon and energy source. Previously genes cmuB, cmuC, cmuA, and folD were shown to be essential for the growth of Methylobacterium chloromethanicum on CH 3 Cl. These CH 3 Cl-specific genes were subsequently detected in H. chloromethanicum. Transposon and marker exchange mutagenesis studies were carried out to identify the genes essential for CH 3 Cl metabolism in H. chloromethanicum. New developments in genetic manipulation of Hyphomicrobium are presented in this study. An electroporation protocol has been optimized and successfully applied for transformation of mutagenesis plasmids into H. chloromethanicum to generate stable CH 3 Cl-negative mutants. Both transposon and marker exchange mutageneses were highly applicable for genetic analysis of Hyphomicrobium. A reliable and reproducible selection procedure for screening of CH 3 Cl utilization-negative mutants has also been developed. Mutational inactivation of cmuB, cmuC, or hutI resulted in strains that were unable to utilize CH 3 Cl or to express the CH 3 Cl-dependent polypeptide CmuA. Reverse transcription-PCR analysis indicated that cmuB, cmuC, cmuA, fmdB, paaE, hutI, and metF formed a single cmuBCA-metF operon and were coregulated and coexpressed in H. chloromethanicum. This finding led to the conclusion that, in cmuB and cmuC mutants, impaired expression of cmuA was likely to be due to a polar effect of the defective gene (cmuB or cmuC) located upstream (5) of cmuA. The detrimental effect of mutation in hutI on the upstream (5)-located cmuA is not clear but indicated that all the genes located within the cmuBCA-metF operon are coordinately expressed. Expression of the cmuBCA-metF transcript was also shown to be strictly CH 3 Cl inducible and was not repressed by the alternative C 1 substrate methanol. Sequence analysis of a transposon mutant (D20) led to the discovery of the previously undetected hutI and metF genes located 3 of the paaE gene in H. chloromethanicum. MetF, a putative methylene-tetrahydrofolate reductase, had 27% identity to MetF from M. chloromethanicum. Mutational and transcriptional analysis data indicated that, in H. chloromethanicum, CH 3 Cl is metabolized via a corrinoid-specific (cmuA) and tetrahydrofolate-dependent (metF, purU, folD) methyltransfer system. Chloromethane (CH 3 Cl), with an average atmospheric concentration of 500 to 600 pptv (parts per trillion by volume), represents the most abundant halocarbon in the atmosphere (17,49). CH 3 Cl is mainly of natural origin and is responsible for about 17% of chlorine-catalyzed ozone destruction (18,19). Current sources of CH 3 Cl that have been identified include biomass burning, emissions from oceans, salt marshes, wood-rotting fungi, higher plants, coal combustion, and industrial emissions (23,24,27,36,38,52,55). The dominant loss process for CH 3 Cl is via reaction with OH radicals in the atmosphere, but soils have also been identified as a significant sink for CH 3 C...

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A review of bacterial methyl halide degradation: biochemistry, genetics and molecular ecology

Cited by 66 publications

References 67 publications

Changing concentrations of CO, CH ₄ , C ₅ H ₈ , CH ₃ Br, CH ₃ I, and dimethyl sulfide during the Southern Ocean Iron Enrichment Experiments

Changing concentrations of CO, CH ₄ , C ₅ H ₈ , CH ₃ Br, CH ₃ I, and dimethyl sulfide during the Southern Ocean Iron Enrichment Experiments

Bacterial Populations Active in Metabolism of C ₁ Compounds in the Sediment of Lake Washington, a Freshwater Lake

Chloromethane-Dependent Expression of the cmu Gene Cluster of Hyphomicrobium chloromethanicum

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A review of bacterial methyl halide degradation: biochemistry, genetics and molecular ecology

Cited by 66 publications

References 67 publications

Changing concentrations of CO, CH 4 , C 5 H 8 , CH 3 Br, CH 3 I, and dimethyl sulfide during the Southern Ocean Iron Enrichment Experiments

Changing concentrations of CO, CH 4 , C 5 H 8 , CH 3 Br, CH 3 I, and dimethyl sulfide during the Southern Ocean Iron Enrichment Experiments

Bacterial Populations Active in Metabolism of C 1 Compounds in the Sediment of Lake Washington, a Freshwater Lake

Chloromethane-Dependent Expression of the cmu Gene Cluster of Hyphomicrobium chloromethanicum

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Changing concentrations of CO, CH ₄ , C ₅ H ₈ , CH ₃ Br, CH ₃ I, and dimethyl sulfide during the Southern Ocean Iron Enrichment Experiments

Changing concentrations of CO, CH ₄ , C ₅ H ₈ , CH ₃ Br, CH ₃ I, and dimethyl sulfide during the Southern Ocean Iron Enrichment Experiments

Bacterial Populations Active in Metabolism of C ₁ Compounds in the Sediment of Lake Washington, a Freshwater Lake