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Appl Environ Microbiol, April 1998, p. 1372-1378, Vol. 64, No. 4
Laboratory for Nitrogen Fixation
Research1 and
Departments of
Microbiology and Crop and Soil Sciences,2
Oregon State University, Corvallis, Oregon 97331-2902
Received 28 August 1997/Accepted 31 January 1998
Ammonia monooxygenase (AMO) from Nitrosomonas europaea
catalyzes the oxidation of ammonia to hydroxylamine and has been
shown to oxidize a variety of halogenated and nonhalogenated
hydrocarbons. As part of a program focused upon extending these
observations to natural systems, a study was conducted to examine the
influence of soil upon the cooxidative abilities of N. europaea. Small quantities of Willamette silt loam
(organic carbon content, 1.8%; cation-exchange capacity, 15 cmol/kg of soil) were suspended with N. europaea cells in a
soil-slurry-type reaction mixture. The oxidations of ammonia and three
different hydrocarbons (ethylene, chloroethane, and
1,1,1-trichloroethane) were compared to results for controls in which
no soil was added. The soil significantly inhibited nitrite production
from 10 mM ammonium by N. europaea. Inhibition resulted from a combination of ammonium adsorption onto soil colloids and the
exchangeable acidity of the soil lowering the pH of the reaction mixture. These phenomena resulted in a substantial drop in the concentration of NH4+ in solution (10 to
4.5 mM) and, depending upon the pH, in a reduction in the amount of
available NH3 to concentrations (8 to 80 µM) similar to the Ks value of AMO for
NH3 (~29 µM). At a fixed initial pH (7.8), the presence
of soil also modified the rates of oxidation of ethylene and
chloroethane and changed the concentrations at which their maximal
rates of oxidation occurred. The modifying effects of soil on nitrite
production and on the cooxidation of ethylene and chloroethane could be
circumvented by raising the ammonium concentration in the
reaction mixture from 10 to 50 mM. Soil had virtually no effect on the
oxidation of 1,1,1-trichloroethane.
Ammonia-oxidizing bacteria initiate
the process of nitrification in soils and other matrices. The
chemolithotroph Nitrosomonas europaea is the most
extensively studied of the ammonia-oxidizing bacteria and has provided
much of our current knowledge of ammonia oxidation at the molecular and
cellular levels (16). Ammonia is converted to nitrite by the
sequential action of two enzymes: ammonia monooxygenase (AMO), which
oxidizes ammonia to hydroxylamine in a reductant-dependent reaction,
and hydroxylamine oxidoreductase, which oxidizes hydroxylamine to
nitrite with the release of four electrons. Two electrons are returned
to AMO to provide reductant for subsequent oxidations. The other two
electrons can fulfill the remaining reductant needs of the cell.
Nitrification in soils has received considerable attention, though
historically it has been studied in the context of nitrogen cycling in
terrestrial ecosystems (5, 6, 33). A number of physical and
chemical factors affecting nitrification rates in soils have been
identified as a result. Nitrification typically requires
O2 and is inhibited by soil conditions which limit
O2 availability (e.g., water-saturated soils)
(1). Ammonia oxidation is most rapid in neutral to alkaline
soils (11, 12). Nitrification rates are inhibited under
acidic conditions where the
NH4+-NH3 equilibrium is driven
toward NH4+ and the availability of
NH3 becomes limiting. The substrate for AMO is
NH3 and not NH4+ (35).
There have been a number of studies investigating the effects of
phenolics, terpenes, and other organic molecules derived from plants on
nitrification activity in soils (4, 7, 25, 26, 32). In
general, these studies were concerned with the process of nitrification
in soils and not with specific nitrifying bacteria.
Through the action of AMO, N. europaea can oxidize
a number of aliphatic and aromatic compounds in
addition to NH3. Examples of cooxidants include alkanes
(17, 20), alkenes (17, 21), aromatics
(24), ethers (18), and thioethers
(22). The oxidation of these alternative substrates does not
provide any known energy benefit to the cell and is dependent on
NH3 oxidation for a sustained supply of reductant.
The substrate range of AMO also extends to several halogenated
hydrocarbons such as trichloroethylene, methyl bromide, vinyl chloride
and dibromochloropropane (2, 9, 19, 28-30). For many
of these substrates, oxidation is followed by dehalogenation
which decreases the recalcitrance of these compounds. Many of these
halogenated compounds are soil contaminants resulting from industrial,
agricultural, or military activities, and it is possible that
nitrifiers, among other bacteria, may play some role in natural
bioremediation processes.
In previous experiments, the degradation of cosubstrates by N. europaea was extensively studied in liquid culture, but the degree
to which these results can be extrapolated to soil environments has not
been addressed. Because some of the potential applications of
biodegradation by ammonia-oxidizing bacteria would take place in soils,
it is desirable to relate the oxidative activities seen in liquid
cultures to situations where these reactions occur in the presence of
soil. Toward this end, three representative cosubstrates were chosen
for experiments designed to analyze the effect of soil on their
oxidation. The three cosubstrates, ethylene, chloroethane, and
1,1,1-trichloroethane (TC), are well-characterized inhibitors of AMO
activity in N. europaea (21, 23, 28, 30). TC is oxidized by AMO but yields products that inactivate ammonia oxidation, while ethylene and chloroethane are oxidized by AMO with little or no
toxic effect on the cell in short time course experiments (23,
28).
Growth and preparation of cells.
N. europaea ATCC
19718 cells were grown in shaken (150 rpm) batch cultures (1.5 liters)
at 30°C in an unlit room in previously described media
(10). The cells were harvested by centrifugation after
3 days of growth and suspended in buffer (50 mM
NaH2PO4 and 2 mM MgCl2 [pH 7.8]
at 1.0 ml of buffer/liter of culture). Cell suspensions were prepared
daily, stored on ice, and used within 8 h. Storage on ice for
periods up to 24 h caused little or no loss of activity.
Collection and preparation of soil.
Soil was collected from
the North Willamette Research and Extension Center, Aurora, Oreg. The
soil is classified as a Willamette silt loam (fine-silty, mixed, mesic,
Pachic Ultic Haploxeroll) in the soil survey of Clackamas County, Oreg.
Soil was sampled from depths of 0 to 20 cm. Particle size analysis
showed the soil to be composed of 13.4, 53.5, and 33.1% (wt/wt) clay,
silt, and sand size particles, respectively. Whole-soil samples were
ground with a mortar and pestle to pass through a 0.25-mm-pore-size
sieve, and total soil organic carbon was determined by direct
combustion to CO2 in a DC-80 carbon analyzer (Dohrmann
Inc., Santa Clara, Calif.) equipped with an infrared detector. The
cation-exchange capacity (CEC) of the soil was determined by the
ammonium acetate displacement method used by the soil testing
laboratory of the Department of Crop and Soil Sciences at Oregon State
University. The Willamette soil was found to contain about 28 µg of
ammonium-N per gram of soil, as determined by the ammonia diffusion
method described below (Table 1). The pHs
of the soil slurries were determined by measuring the pHs of the
supernatants after the soil was removed by centrifugation. Because the
initial pH of the soil (2:1, water:soil [vol/wt]) ranged between 6.0 and 6.2, the soil was neutralized (pH 7.2) by the addition of 3 g
of Ca(OH)2/kg of soil. Furthermore, the pHs of reaction
mixtures containing 0.5 g of neutralized Willamette soil in 1 ml
of buffer (50 mM NaH2PO4, 2 mM
MgCl2 [pH 7.8]) were adjusted to 7.8 by the addition of
NaOH and monitored for 30 min to ensure that the pH was stable prior to
the addition of cells.
0099-2240/98/$04.00+0
Copyright © 1998, American Society for Microbiology. All rights reserved.
Effects of Soil on Ammonia, Ethylene, Chloroethane,
and 1,1,1-Trichloroethane Oxidation by Nitrosomonas
europaea
ABSTRACT
Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References
INTRODUCTION
Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References
MATERIALS AND METHODS
Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References
TABLE 1.
Ammonium binding to Willamette
soila
Substrate oxidations. Reactions were carried out in 6.5-ml serum vials stoppered with gray butyl rubber stoppers (Baxter Scientific, McGraw Park, Ill.) or Teflon-lined gray butyl rubber stoppers (Alltech Associates Inc., Deerfield, Ill.) and capped with aluminum seals (VWR Scientific, Seattle, Wash.). The reaction mixtures were made up to a volume of 1 ml. Each reaction was buffered with 50 mM NaH2PO4-2 mM MgCl2 (pH 7.8). Reactions were run in the presence of 10 mM NH4+ unless indicated otherwise. All reactions were initiated by the addition of 20 µl of cell suspension (ca. 400 µg of protein). Each reaction was incubated in a 30°C water bath while being shaken at 150 cycles/min for 30 min unless indicated otherwise. Samples were removed with gastight syringes at the indicated times and analyzed as described below. In the cooxidation experiments, after the addition of ethylene, chloroethane, or TC to the sealed vials containing the reaction components, the cosubstrate was allowed to equilibrate for 30 min at 30°C while being shaken before the reaction was started by the addition of cells.
Analytical procedures. The protein contents of the cell suspensions were estimated by the biuret assay (14) after the cells were solubilized in 3 N NaOH for 30 min at 65°C. Bovine serum albumin was used as a standard. An ammonia diffusion assay (8) was used to determine the ammonia (NH3 plus NH4+) concentration. In this assay, the solution to be tested is made basic with K2CO3, converting any NH4+ to NH3. The stoppered vial contains a wick in the headspace which is saturated with H2SO4. Ammonia diffuses into the headspace and is trapped on the wick. The wick is then removed and dipped into a solution containing Nessler's reagent (8), and the resulting color development is measured spectrophotometrically at 490 nm. For nitrite analyses, liquid samples (5 µl; test performed in duplicate) were taken at specified time intervals and analyzed as described previously (15). For samples containing soil, the soil was removed by centrifugation in a microcentrifuge at 16,000 × g for 5 min prior to taking samples for nitrite analyses. Gas samples were analyzed by a gas chromatograph (model GC-8A; Shimadzu, Kyoto, Japan) equipped with a stainless-steel column packed with Porapak Q 80-100 mesh (Waters Associates Inc., Framingham, Mass.) and a flame ionization detector interfaced to an integrator (model C-R3A; Shimadzu). To determine the amount of ethylene oxide produced from ethylene, gas samples (500 µl) were injected into a Porapak Q 80-100 mesh stainless-steel column (1/8 by 48 in [0.3 by 121.9 cm]) at 130°C. To determine the amount of acetaldehyde formed from the oxidation of chloroethane, gas samples (1 ml) were injected into a Porapak Q 80-100 mesh column (1/8 by 48 in [0.3 by 121.9 cm]) at 90°C. To determine the amount of 2,2,2-trichloroethanol produced from TC, liquid samples (10 µl) were injected into a Porapak Q 80-100 mesh column (1/8 by 36 in [0.3 by 91.4 cm]) at 175°C. Within a given type of experiment, replicate analyses indicated standard errors of about 5% for the nitrite assays, about 6% for the ammonium diffusion assays, and about 8% for the gas chromatography experiments. Between experiment types, the variability was greater, as indicated below.
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RESULTS |
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Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References
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Ammonia oxidation by cell suspensions of N. europaea
was affected by the presence of unsterilized soil. The amount of
NO2
produced by cells was measured over time
in the presence of varying amounts of Willamette silt loam soil ranging
from 0 to 1.0 g per ml of reaction mixture. The addition of soil
to cultures had a pronounced inhibitory effect on the oxidation of
NH3 (Fig. 1). The degree of
inhibition increased with increasing amounts of soil present. The
addition of soil potentially could influence NO2 production in a number of ways, e.g., by
altering the pH, by adsorbing ammonium (NH4+),
or through endogenous ammonium- and nitrite-oxidizing activities. Therefore, experiments were done to identify and characterize the
nature of the inhibition of NH3 oxidation by soil.
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; 0.1 g of soil, 
; 0.25 g
of soil, 
; 0.5 g of soil, 
; 1.0 g of soil, 
.
When nonsterilized soil not augmented with N. europaea was
tested for endogenous NH3-oxidizing activity,
NO2 production was not detected after a
60-min incubation (data not shown). In addition,
NH4+ added to soil samples was almost
completely recoverable after a 90-min incubation (Table 1), suggesting
that there was little if any endogenous NH4+
oxidation or assimilation activity in the soil under the conditions tested. Likewise, soil samples did not consume added
NO2, indicating that endogenous
NO2-oxidizing activity was also not
significant in these experiments (data not shown). In the short-term
assays used in this study, we obtained no evidence for any biological
activity of the air-dried soil that compromised the measurements that
we made. Therefore, nonsterilized soil was used in subsequent
experiments, and NO2 production was used as a
measure of NH3 oxidation. In a separate experiment, the
addition of washed sand instead of Willamette soil was tested for its
effect on nitrification. The sand did not bind
NH4+ or alter the reaction pH, and no decrease
in NO2 production was observed (data not
shown).
Because NH3 oxidation by N. europaea is
sensitive to pH, the addition of soil could affect activity simply by
lowering the pH of the reaction medium. Indeed, the addition of
Willamette soil (pH 6.1 in a 1:2 [wt/vol] soil-deionized-water
mixture) resulted in a soil-buffer suspension with a pH of 6.8 before
ammonia oxidation was initiated. Furthermore, when soil neutralized
with Ca(OH)2 (to pH 7.2) was used, the initial soil-buffer
pH was 7.2. Nitrite production was determined in reactions with
different starting pHs both in the presence and absence of 0.5 g
of soil (Fig. 2). In the presence of
soil, it can be seen that substantially less NO2 was produced as the starting pH was
lowered from 8.0. The addition of soil reduced
NO2 production by as little as 12% at pH 8.0 and by greater percentages (33 to 40%) at pH values lower than 8.0. Thus, changes in the initial pH of the reaction mixture (caused by the
addition of unbuffered soil) had a significant effect on
NO2 production. For this reason, in
subsequent experiments the pHs of the reaction mixtures containing soil
were adjusted to 7.8 prior to the start of the reaction.
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The soil might also be expected to affect the buffering capacity of the
reaction mixture. To determine if this was a significant factor, an
experiment was done in which 1 ml of buffer, with and without the
addition of 0.5 g of soil, was adjusted to pH 7.8. Cells were
added, and the mixture was incubated at 30°C for 30 min. In the
absence of soil, 5.5 mM NO2 was produced and
the final pH was 7.21, while in the presence of soil, 4.6 mM
NO2 was produced and the final pH was 7.33. Therefore, when the pHs of the assay buffers of the soil and nonsoil
samples were both adjusted to an initial value of 7.8, the effects of
any changes in buffering capacity on NO2
production were small.
Most soils have a capacity to bind cations from aqueous solutions.
Therefore, we considered the possibility that part of the observed
decrease in NO2 formation was a result of
NH4+ bound to the soil surfaces and thereby
lowering the free-NH4+ concentration governing
the rate of ammonia oxidation. The amount of
NH4+ which bound to 0.5 g of soil was
determined for amounts ranging from 0 to 20 µmol of
NH4+/ml. After a 1.5-h incubation in buffer
containing NH4+, the soil was sedimented by
centrifugation and the NH4+ concentrations in
the supernatant and sediment were measured (Table 1). Our data clearly
indicated that the concentration of ammonium in the solution
phase was lower than anticipated if soil was not present. The
sedimented soil retained a large proportion of the
NH4+, ranging from 40 to 62% of the initial
amount. For 10 µmol of NH4+, 55% of the
added NH4+ was bound to the soil.
Given that the Willamette soil bound a large portion of the added
NH4+, we wished to determine if increasing the
NH4+ concentration in the reaction mixture
could restore activity in the presence of soil. The rate of
NO2 production as a function of the
NH4+ concentration in the presence of various
amounts of soil (Fig. 3) was measured. As
before, for a given NH4+ concentration,
increasing the amount of soil in the reaction decreased the rate of
NO2 formation. However, the inhibition of
activity by a given amount of soil could be overcome by the addition of
more NH4+. More soil required more
NH4+ to reach maximal activity. Plots of the
data with the best least-squares fit to the equation v = [Vmax × S/(Ks + S)] (Fig. 3)
showed that the net effect of the addition of soil was to raise the
apparent Ks values for ammonium from 0.83 mM (in
the absence of soil) to 1.9 and 3.6 mM in the presence of 0.25 and
0.5 g of soil/ml of reaction mixture, respectively. Given an
apparent Ks of 3.6 mM, the lowering of the
NH4+ concentration in solution from 10 to 4.5 mM upon the addition of 0.5 g of soil should result in a 21%
decrease in activity ([1 
(0.73 Vmax/0.92
Vmax)] × 100). This predicted decrease in
activity is compared to the 22% decrease for 0.5 g of soil at 30 min seen in Fig. 1 and the 14% decrease seen in Fig. 3 with 0.5 g
of soil at 10 mM NH4+.
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The availability of soil-bound ammonium for nitrifying bacteria can vary and is strongly influenced by the availability of competing cations such as potassium (27, 36). In our system, it should be noted that we routinely used a sodium phosphate buffer. However, the use of KH2PO4 buffer and KOH for pH adjustments instead of NaH2PO4 and NaOH made no difference with regard to the observed pH effects or the amount of nitrite produced in 30 min at the same pH.
Having characterized the effect of Willamette soil on nitrite production by cultures of N. europaea, we next wished to determine the effect of soil on the oxidation of the cosubstrates ethylene, chloroethane, and TC. We first considered the possibility that these compounds might bind to the soil, thereby changing the effective concentrations of the compounds, as we had observed with ammonium. However, there was no detectable change in the headspace concentrations of these compounds over 2 h after the addition of soil to the reaction mixture, which indicates that there was no substantial binding of these three compounds to the soil nor endogenous biological oxidation activity under the conditions tested. Our results do not rule out the possibility that these compounds may bind to the soil over longer time periods and especially under conditions where the soil structure remains intact. Ammonia is a required component in the reaction mixtures because the oxidation of ammonia provides the reductant for AMO-catalyzed transformation of these alternative substrates. The experiments were done in the presence of 10 mM NH4+.
Ethylene is a competitive inhibitor of ammonia oxidation (with a
Ki of about 660 µM) by AMO (23).
Both the production of NO2 and the formation
of ethylene oxide from ethylene were measured as functions of
increasing ethylene concentration in the presence or absence of soil.
As expected of a competitive inhibitor, NO2
production decreased as the cosubstrate concentration increased (Fig.
4B). The addition of soil increased the inhibition of
NO2 production by ethylene. The point of 50%
inhibition of NO2 formation was at about 0.41 mM ethylene in the absence of soil and about 0.12 mM ethylene in the
presence of 0.5 g of soil. The addition of soil had two effects on
the oxidation of ethylene. First, the maximal amount of ethylene oxide
produced was about 50% less in the presence of soil (Fig.
4A). Second, the maximum activity we
observed was shifted downward from a 0.36 mM concentration of added
ethylene to about 0.09 mM. In the presence of soil, at the
highest ethylene concentrations, about 0.5 µmol of ethylene oxide was produced, even though little NO2
was produced. Apparently, the oxidation of endogenous storage compounds
provided the reductant for the AMO-catalyzed transformation of ethylene
to ethylene oxide.
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The second cosubstrate examined was chloroethane, which is oxidized to
acetaldehyde and Cl by AMO (28). Chloroethane
is a noncompetitive inhibitor of NH3 oxidation
(KiE and
KiES of 1.4 mM) and does not
inactivate AMO (23, 30). Nitrite production (from
ammonia) and acetaldehyde production (from chloroethane) were
monitored at various concentrations of chloroethane. Nitrite production
steadily declined with increasing chloroethane concentration (Fig.
5B). The addition of soil lowered the
50% inhibition point in nitrite formation from about 3.8 mM chloroethane to about 2.4 mM. As expected, the amount of
acetaldehyde produced first increased with increasing chloroethane
concentration and then decreased as reductant became limiting (due to
the inhibition of ammonia oxidation) (Fig. 5A). The addition of soil
reduced the maximal activity by about 37% and shifted the peak of
maximal activity from about 2.8 mM chloroethane to about 1.1 mM. A
residual acetaldehyde production of about 0.3 µmol was observed at
the higher chloroethane concentrations.
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The third cosubstrate tested, TC, is a potent inactivator of
NH3 oxidation (30). TC is oxidized to
2,2,2-trichloroethanol. Even low concentrations of TC (0.2 mM)
drastically lowered the amount of NO2
produced (Fig. 6B). The inhibition of
nitrite production in the presence of soil was only slightly greater
than that observed in its absence and in the presence of TC. As with
chloroethane and ethylene, the profile for 2,2,2-trichloroethanol
production first increased with increasing TC concentrations and then
decreased (Fig. 6A). Unlike with ethylene and chloroethane, however,
the addition of soil appeared to have only a small effect on the
oxidation of TC. The maximum for 2,2,2-trichloroethanol production was
not shifted to a lower value in the presence of soil. The maximal amount of 2,2,2-trichloroethanol produced (0.33 µmol) was also much
less than that observed for ethylene oxide (2.7 µmol) or acetaldehyde
(2.1 µmol). Another distinction between the results with this
compound and those with the other two cosubstrates was that no residual
activity was observed at high concentrations of TC. Apparently this is
a result of the ability of TC to inhibit AMO.
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Higher concentrations of NH4+ added to the
reaction mixture could compensate for the inhibitory effects of soil on
NO2 production in the absence of a
cosubstrate (Fig. 3). To determine if increased
NH4+ concentrations could also compensate for
the observed differences in cosubstrate oxidations, the experiment with
chloroethane (Fig. 5) was repeated in the presence of 50 mM
NH4+. Both the maximum activity and the
chloroethane concentration at which this maximum occurred were now the
same, regardless of the presence or absence of soil (Fig.
7). In fact, the curves were similar at
all concentrations of chloroethane. The amounts of nitrite produced
during the incubation were also similar.
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DISCUSSION |
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Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References
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Our primary interest in these experiments was to extend the present knowledge of NH3 and cosubstrate oxidation by N. europaea in liquid cultures to situations where these reactions take place in the presence of soil. The results showed that while the oxidation of NH3 and cosubstrates by N. europaea occurred in the presence of soil, the soil does significantly modify the kinetics of these reactions. We have considered two primary mechanisms by which soil could influence the rate of NH3 oxidation: by changing the pH of the reaction mixture, which consequently influences the NH3-NH4+ equilibrium, and by binding NH4+ and thereby lowering the equilibrium concentration available for the cells. It is well recognized that ammonium binds to a majority of soils because of their CECs (27). Indeed, the CECs of many soils are routinely measured by determining the amount of ammonium that binds to the soil after suspension in an ammonium salt solution (31). Young (37) showed that both organic matter and clay content were influential in the binding of ammonium to Oregon soils. Despite the fact that the Willamette silt loam possesses a relatively low CEC (15 cmol/kg) and organic carbon content (1.8%), this soil lowered the amount of ammonium present in solution significantly, lowered the pH of the reaction mixture, and subsequently influenced the rate of ammonia oxidation. When the pH of the reaction mixture was lowered by the addition of soil with exchangeable acidity, the inhibition could be substantial (Fig. 2). At pH values of 7.5 or lower, the more exaggerated effect of soil could be attributed to a shift in the NH3-NH4+ equilibrium (pKa = 9.2) towards NH4+ and away from NH3, the substrate for AMO. Reduced AMO activity was observed when the NH3 concentration dropped into the range of the Ks value for NH3. For example, at pH 8.0, 4.5 mM NH4+ is in equilibrium with 250 µM NH3, while within the pH range 6.5 to 7.5, the NH3 concentration associated with 4.5 mM NH4+ ranges between 7.9 and 79 µM. These values are similar to the Ks of AMO for NH3 (~29 µM) calculated from the apparent Ks for NH4+ (0.83 mM) at pH 7.8 (Fig. 3).
However, even when the pH of the reaction mixture was carefully
controlled, upon addition of soil, inhibition of nitrite production was
still observed (Fig. 1). In most of our experiments, the addition of
0.5 g of soil decreased the nitrite production 14 to 55%, with a
median decrease near 27%. Considering the kinetic saturation profile
and an apparent Ks of 0.83 mM
NH4+, the decrease from 10 to 4.5 mM
NH4+ which occurred upon addition of 0.5 g
of soil should result in about a 9% decrease in nitrite production
([1 (0.84 Vmax/0.92 Vmax)] × 100). However, the increase in
apparent Ks to 3.6 mM which occurred upon
addition of 0.5 g of soil predicts a 21% decrease in activity
([1 (0.73 Vmax/0.92
Vmax)] × 100). Therefore, while a significant
portion of the soil effect on nitrite production can be attributed to
the loss of free NH4+ due to binding to soil,
there appear to be other factors associated with the addition of soil
which also contribute to the reduction of activity. For example, the
presence of competitive inhibitors of nitrification in the Willamette
soil would be consistent with the data presented in this study. In
light of the literature concerning the presence of naturally occurring
inhibitory compounds in soils, it might not be surprising if Willamette
soil contained organic substances inhibitory to
NO2 production. Although the earlier studies
concerning phenolics and terpenoids in soils were somewhat
contradictory concerning the effects of these substances on
nitrification, recent studies with pure cultures showed that AMO in
N. europaea is inhibited by aromatic compounds
(24). Regardless of the source of the inhibition of nitrite
production, the inhibition was almost completely compensated for by
increasing the NH4+ concentration (Fig. 3).
As was the case with NH3 oxidation, the addition of soil
had a significant impact on the oxidation of the cosubstrates ethylene and chloroethane. The effect of adding soil to these reactions is
complex, since the NH4+ concentration in the
reaction is altered, which in turn affects the competitive inhibition
of AMO by the cosubstrate. The effect of soil on the substrate
inhibition curves for the oxidations of ethylene and chloroethane were
similar in that the peak of maximal activity shifted toward lower
cosubstrate concentrations and the amplitude of the maximal activity
was significantly lowered in the presence of soil. As with
NO2 production, part of the decrease in
substrate oxidation activity would be expected from the adsorption of
NH4+ to the soil particles. Less free
NH4+ would result in less reductant available
for the oxidation of the cosubstrate, lowering the rate of product
formation. Indeed, when the NH4+ concentration
was increased to 50 mM, the results with soil were similar to those
without soil. In the case of the competitive inhibitor ethylene, less
NH4+ also means ethylene competes more
effectively for the active site on AMO, resulting in even greater
inhibition. This fact could explain why soil depressed ethylene
oxidation to a greater extent than chloroethane. Rasche et al.
(28) had previously shown that the concentration of
chloroethane optimal for cooxidation dropped significantly when
ammonium concentrations were lowered from 10 to 1 mM. The effect
of soil on chloroethane oxidation was entirely consistent with a
lowering of ammonium availability.
TC degradation was largely unaffected by the addition of soil. This
result is understandable when one considers that TC is oxidized slowly
relative to the other substrates considered in this study. TC
drastically inhibited NH4+ oxidation, thereby
lowering reductant levels, but sufficient reductant, either from
endogenous respiration or NH3 oxidation, was available to
drive TC oxidation. At 8 mM TC, NO2 was no
longer produced and electrons were no longer available from
NH3 oxidation. Yet TC oxidation continued at a reduced rate at this concentration, suggesting that endogenous sources of reductant could support some TC oxidation (Fig. 6). Similarly, ethylene and
chloroethane oxidation also showed a basal rate at the higher substrate
concentrations, which might also be accounted for by endogenous sources
supplying some low level of reductant. Rates of
NO2 production in the presence of TC were
much lower than with ethylene and chloroethane, which is consistent
with TC being a stronger inhibitor of AMO. The addition of soil
resulted in a slight drop in NO2 production.
However, the effect of soil on nitrite production might be expected to
be less for TC than for ethylene and chloroethane, since the slow rate
of TC turnover would require a lower reductant availability.
Sustaining the rate of cooxidation requires the achievement of a balance between the concentrations of the growth-supporting substrate and the cooxidant so that sufficient energy is generated for the maintenance of cell processes and turnover of the catalytic enzyme. Although several kinds of bacteria possess the ability to cooxidize chlorinated aliphatic hydrocarbons, their primary energy sources are volatile compounds (e.g., toluene, phenol, methane, and butane [3]) whose concentrations are difficult to control accurately under most environmental conditions. In this context, ammonium has some useful attributes, since it can be added and retained by soil in amounts that will be influenced by the magnitude of the CEC of the solid matrix. Furthermore, it is conceptually possible for the solution phase NH4+ concentration to be maintained from this solid phase adsorbed supply at a concentration sufficient to support growth and cooxidation.
Our results show that soil can have a profound impact on the oxidation of alternative substrates as well as on the oxidation of NH3 by N. europaea. With the Willamette silt loam used in this study, NH3 oxidation was influenced both by exchangeable acidity and by the adsorption of NH4+ to the soil. While our work focused on a single soil type, it does serve to highlight some of the soil factors that can influence both NH3 oxidation and cosubstrate oxidation. Although we used soil slurries in our experiments, the factors we identified are also likely to be important in structured soils at or below field moisture capacity. Furthermore, with other soils, or with intact soils with different moisture contents, other factors may be identified that are more or less important. For example, Stark and Firestone (34) described the importance of soil moisture to the availability of NH4+ for nitrification. Fuller and Scow (13) observed biocidal effects of chlorinated aliphatic hydrocarbons on cell growth of ammonia oxidizers in experiments that occurred over long time periods. The effects of soil would be particularly relevant to in situ bioremediation or bioaugmentation plans where rates of cosubstrate oxidation would be sensitive to the sequestering of NH4+ by the soil, with the result that rates of cosubstrate oxidation could be reductant limited.
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ACKNOWLEDGMENT |
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This work was supported by the U.S. Environmental Protection Agency (grant R821405 to D.J.A. and P.J.B.).
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FOOTNOTES |
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* Corresponding author. Mailing address: Laboratory for Nitrogen Fixation Research, Oregon State University, 2082 Cordley Hall, Corvallis, OR 97331-2902. Phone: (541) 737-4214. Fax: (541) 737-3573. E-mail: arpd{at}bcc.orst.edu.
Technical paper 11,230 of the Oregon Agricultural Experiment
Station.
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REFERENCES |
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Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References
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