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Appl Environ Microbiol, March 1998, p. 1091-1098, Vol. 64, No. 3
Darling Marine Center, University of Maine,
Walpole, Maine 04573
Received 3 September 1997/Accepted 23 December 1997
Two methanotrophic bacteria, Methylobacter albus BG8
and Methylosinus trichosporium OB3b, oxidized atmospheric
methane during batch growth on methanol. Methane consumption was
rapidly and substantially diminished (95% over 9 days) when washed
cell suspensions were incubated without methanol in the presence of
atmospheric methane (1.7 ppm). Methanotrophic activity was stimulated
after methanol (10 mM) but not methane (1,000 ppm) addition. M. albus BG8 grown in continuous culture for 80 days with methanol
retained the ability to oxidize atmospheric methane and oxidized
methane in a chemostat air supply. Methane oxidation during growth on methanol was not affected by methane deprivation. Differences in the
kinetics of methane uptake (apparent Km and
Vmax) were observed between batch- and
chemostat-grown cultures. The Vmax and
apparent Km values (means ± standard
errors) for methanol-limited chemostat cultures were 133 ± 46 nmol of methane 108 cells
0099-2240/98/$04.00+0
Copyright © 1998, American Society for Microbiology. All rights reserved.
Methanol Promotes Atmospheric Methane Oxidation by
Methanotrophic Cultures and Soils
1 h
1
and 916 ± 235 ppm of methane (1.2 µM), respectively. These
values were significantly lower than those determined with batch-grown cultures (Vmax of 648 ± 195 nmol of
methane 108 cells
1 h
1 and
apparent Km of 5,025 ± 1,234 ppm of
methane [6.3 µM]). Methane consumption by soils was stimulated by
the addition of methanol. These results suggest that methanol or other
nonmethane substrates may promote atmospheric methane oxidation in
situ.
*
Corresponding author. Phone: (207) 563-3146, ext. 207. E-mail: gking{at}maine.maine.edu.
Contribution 312 from the Darling Marine Center.
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