Effect of Selected Monoterpenes on Methane Oxidation, Denitrification, and Aerobic Metabolism by Bacteria in Pure Culture

This Article

	Abstract
	Full Text (PDF)
	An erratum has been published
	Alert me when this article is cited
	Alert me if a correction is posted

Services

	Similar articles in this journal
	Similar articles in PubMed
	Alert me to new issues of the journal
	Download to citation manager
	Reprints and Permissions
	Copyright Information
	Books from ASM Press
	MicrobeWorld

Citing Articles

	Citing Articles via HighWire
	Citing Articles via Google Scholar

Google Scholar

	Articles by Amaral, J. A.
	Articles by Knowles, R.
	Search for Related Content

PubMed

	PubMed Citation
	Articles by Amaral, J. A.
	Articles by Knowles, R.


Agricola

	Articles by Amaral, J. A.
	Articles by Knowles, R.

Previous Article | Next Article

Appl Environ Microbiol, February 1998, p. 520-525, Vol. 64, No. 2
0099-2240/98/$04.00+0
Copyright © 1998, American Society for Microbiology. All rights reserved.

Effect of Selected Monoterpenes on Methane Oxidation, Denitrification, and Aerobic Metabolism by Bacteria in Pure Culture

J. A. Amaral,^* A. Ekins, S. R. Richards, and R. Knowles

Department of Natural Resource Sciences, Macdonald Campus of McGill University, Ste. Anne-de-Bellevue, Québec, Canada

Received 29 July 1997/Accepted 14 November 1997

	ABSTRACT

Top Abstract Introduction Materials & Methods Results Discussion References

Selected monoterpenes inhibited methane oxidation by methanotrophs (Methylosinus trichosporium OB3b, Methylobacter luteus),denitrification by environmental isolates, and aerobic metabolismby several heterotrophic pure cultures. Inhibition occurred tovarious extents and was transient. Complete inhibition of methaneoxidation by Methylosinus trichosporium OB3b with 1.1 mM ( $-$ )- $alpha$ -pinenelasted for more than 2 days with a culture of optical densityof 0.05 before activity resumed. Inhibition was greater underconditions under which particulate methane monooxygenase was expressed.No apparent consumption or conversion of monoterpenes by methanotrophswas detected by gas chromatography, and the reason that transientinhibition occurs is not clear. Aerobic metabolism by severalheterotrophs was much less sensitive than methanotrophy was; Escherichiacoli (optical density, 0.01), for example, was not affected byup to 7.3 mM ( $-$ )- $alpha$ -pinene. The degree of inhibition was monoterpeneand species dependent. Denitrification by isolates from a pollutedsediment was not inhibited by 3.7 mM ( $-$ )- $alpha$ -pinene, $gamma$ -terpinene,or $beta$ -myrcene, whereas 50 to 100% inhibition was observed for isolatesfrom a temperate swamp soil. The inhibitory effect of monoterpeneson methane oxidation was greatest with unsaturated, cyclic hydrocarbonforms [e.g., ( $-$ )- $alpha$ -pinene, (S)-( $-$ )-limonene, (R)-(+)-limonene,and $gamma$ -terpinene]. Lower levels of inhibition occurred with oxideand alcohol derivatives [(R)-(+)-limonene oxide, $alpha$ -pinene oxide,linalool, $alpha$ -terpineol] and a noncyclic hydrocarbon ( $beta$ -myrcene).Isomers of pinene inhibited activity to different extents. Giventheir natural sources, monoterpenes may be significant factorsaffecting bacterial activities in nature.

	INTRODUCTION

Top Abstract Introduction Materials & Methods Results Discussion References

Monoterpenes are naturally occurring compounds produced by plants and animals. The majority of these compounds are unsaturatedhydrocarbons (C₁₀), but there are also oxygenated derivatives,such as alcohols, ketones, and carboxylic acids, and collectivelythese compounds are known as monoterpenoids (12). These compounds,the main components in volatile essential oils of plants, arewidely distributed throughout vegetation types but are found inespecially high concentrations in plants such as the conifers(12, 23). The monoterpenes are a significant natural sourceof atmospheric nonmethane hydrocarbons. They are involved in avariety of atmospheric reactions (16, 23, 36) and can contributeto production of tropospheric ozone (16).

Monoterpenoids have long been used in the food, perfume, and pharmaceutical industries because of their flavoring and antimicrobialproperties. They are currently of interest industrially as replacementsfor chlorofluorocarbons and halogenated solvents (21, 24).Recently, it has been suggested that monoterpenes play an importantrole in altering nitrogen (N) and carbon (C) cycling in forestsoils (36).

The inhibition of activity and growth of some microorganisms by monoterpenes is well-known (22, 27). However, other microbesmay be stimulated. Volatile oil from aromatic plants has increasedCO₂ production in soil samples sixfold (31). Microbial degradationof monoterpenes under both aerobic (24) and anaerobic (18)conditions has been described (reviewed in reference 28). Theability to inhibit some microorganisms but not others makes monoterpenespotential factors in the control of microbial processes in environmentswhere they are abundant, such as forest soils (38).

It has been suggested that inhibition of nitrification by monoterpenes in forest soils has a major influence on N cyclingin these environments (33-36). It has been proposed that monoterpeneshave a direct effect on the primary enzyme of this process, ammoniamonooxygenase (AMO) (34, 35). Methane (CH₄) monooxygenase(MMO), the primary enzyme in the CH₄ oxidation process, and AMOare susceptible to many of the same inhibitors (8). Thus, itmight be expected that monoterpenes that inhibit nitrificationshould also inhibit CH₄ oxidation. We recently found that a varietyof monoterpenes inhibit methane consumption by forest soils underfield-moist and slurry conditions (3). These compounds, whichare typically most concentrated in the forest litter, along withother soluble, inhibitory soil components (5) may explain thelack of methane consumption in the top layers of many forest soils(1, 6). Preliminary studies showed that pure cultures ofmethanotrophs were also inhibited (3, 36).

In this study, we examined the effect of several monoterpenes on methane oxidation by pure cultures of the methanotrophs Methylosinustrichosporium OB3b and Methylobacter luteus, denitrification bysix environmental isolates, and aerobic metabolism by severalheterotrophic laboratory cultures.

	MATERIALS AND METHODS

Top Abstract Introduction Materials & Methods Results Discussion References

Bacterial cultures. The methane oxidizers, Methylosinus trichosporium OB3b and Methylobacter luteus, were gifts from R. S. Hanson (Universityof Minnesota). Cells were grown in a nitrate mineral salts medium(NMS) (37) supplemented with 10 µM copper (Cu) under an atmospherecontaining 20% CH₄ in air. Methylosinus trichosporium OB3b wasalso grown in NMS containing no Cu in order to stimulate productionof soluble MMO (sMMO) (17) under the same atmosphere. Cultures(volume, 0.5 liter) were grown in 2-liter Erlenmeyer flasks witha side arm at 25°C, with agitation provided by a magnetic stirbar.

Denitrifying isolates were obtained from a temperate swamp (isolates D1 and D3; obtained from Mt. St. Hilaire, Québec, Canada[4]) and a polluted sediment (isolates HH1, HH3, HH4, and HH6;obtained from Hamilton Harbour, Ontario, Canada [26]). Theseisolates were grown on a rotary shaker (250 rpm) in nutrient broth(NB) (BBL) supplemented with 10 mM KNO₃ at 25°C under a heliumatmosphere.

The effect of monoterpenes on aerobic activity was tested by using laboratory cultures of Pseudomonas aeruginosa, Escherichiacoli, Serratia marcescens, Bacillus subtilis, and Staphylococcusaureus. Cells were grown in the presence of the ambient atmospherein 50 ml of NB in 125-ml Erlenmeyer flasks at 25°C on a rotaryshaker (250 rpm).

Incubations. The effect of monoterpenes on CH₄ oxidation by methanotrophs was tested by using 58-ml serum bottles capped with grey butylstoppers and aluminum crimps. The bottles were acid washed (0.12N HCl) and rinsed four times with deionized water to minimizecontamination in experiments in which no Cu was added. Medium(10 ml) was added to the bottles and sterilized before monoterpeneswere added. Pure monoterpenoids (approximately 0.6 to 6 µl) wereadded with a Hamilton glass microsyringe directly to the bottlesto give final concentrations of 0.37 to 3.7 mM (0.5 to 5 ppm [wt/vol]for hydrocarbon monoterpenoids). These values are well below theaqueous solubilities of the compounds (32), but due to volatilizationand adsorption they should be considered the upper limits of thedissolved concentrations. The bottles were then inoculated withlate-log-phase methanotroph cells to give final optical densitiesat 600 nm (OD₆₀₀) ranging from 0.04 to 0.095. Some bottles werepreincubated without cells for 3 days to allow the monoterpenelevels in the headspace to equilibrate. Incubations were carriedout in the dark at 25°C on a rotary shaker (230 rpm) under atmospherescontaining 4 to 20% CH₄ in air. Consumption of CH₄ and productionof CO₂ were monitored for 2 to 5 days, as described below.

Experiments with denitrifying isolates were carried out as described above except that NB containing KNO₃ and a helium atmospherewere used. The bottles also received acetylene (10%, vol/vol),a monoterpene (3.1 mM), or acetylene plus a monoterpene to determineif N₂O production (and hence denitrification) was affected bythe monoterpene addition. The initial culture OD₆₀₀ varied from0.03 to 0.12.

The remaining laboratory cultures were grown aerobically in NB at 25°C on a rotary shaker (250 rpm) in 50-ml Erlenmeyer flaskscapped with Suba-Seal stoppers (William Freeman Co., Barnsley,United Kingdom) in the presence of various concentrations of monoterpenes.Microbial activity was measured by measuring the production ofCO₂ over an incubation period of 38 h. The initial cell concentrationswere equivalent to an OD₆₀₀ of 0.01.

The data given below are the means ± standard errors of the means from duplicate or triplicate incubations.

Analyses. Samples (0.3 to 0.5 ml) of the gases in the headspaces of incubation vessels were obtained with a syringe, and the gases werequantified by gas chromatography. The CH₄ and CO₂ levels weremeasured by thermal conductivity detection, while the N₂O levelwas measured by electron capture detection (2, 4, 26).Standard gas mixtures were used to calibrate each measurement.The volatile monoterpenes in the headspaces were measured by usinga Varian model 1700 gas chromatograph equipped with a flame ionizationdetector and a 3-m packed column containing 20% Carbowax 4000(39) coated onto Chromsorb W, HP (80/100 mesh; ChromatographicSpecialties Inc., Brockville, Ontario, Canada). The injector anddetector temperatures used were 175 and 250°C, respectively. Thecolumn temperature was programmed to increase from 100 to 150°Cat a rate of 4°C min¹. The measurements were not calibrated with a known standard andthus were measurements of the relative amounts of the volatilemonoterpenes present in each flask. Changes in machine sensitivitywere determined each day by injecting a freshly prepared volatilesample of ( $-$ )- $alpha$ -pinene. No significant difference in sensitivitywas observed during the experiment (data not shown). The minimumdetection limits were estimated to be about 0.1 mM.

Cell densities were measured with a Spectronic 21 spectrophotometer at 600 nm.

Monoterpenoids. The following compounds were tested for their effects on microbial activities: ( $-$ )- $alpha$ -pinene, $alpha$ -terpinene, and $beta$ -myrcene fromICN Biochemicals, Aurora, Ohio; and (+)- $alpha$ -pinene, ( $-$ )- $beta$ -pinene, $gamma$ -terpinene, (R)-(+)-limonene, (S)-( $-$ )-limonene, (+)-limoneneoxide, $alpha$ -pinene oxide, $alpha$ -terpineol, and (±)-linalool from AldrichChemical Co., Milwaukee, Wis. The monoterpenoids used are commonlyfound in nature, and their chemical structures are given in Fig.1. The sterility of the monoterpenoids was confirmed by asepticallyintroducing 1 µl of each compound into 10 ml of NB. No growthwas observed over a 15-day incubation period (data not shown).

View larger version (17K):
[in this window]
[in a new window]

FIG. 1. Representative structural formulae of the monoterpenoids used. 1, (R)-(+)-limonene; 2, (+)-limonene oxide; 3, (+)- $alpha$ -pinene oxide; 4, $alpha$ -pinene; 5, ( $-$ )- $beta$ -pinene; 6, $gamma$ -terpinene; 7, $alpha$ -terpinene; 8, $alpha$ -terpineol; 9, $beta$ -myrcene; 10, linalool.

	RESULTS

Top Abstract Introduction Materials & Methods Results Discussion References

Effects of pinenes on CH₄ oxidation. ( $-$ )- $alpha$ -Pinene inhibited CH₄ oxidation by Methylosinus trichosporium OB3b, as observed in preliminary studies (3, 36).After 2 days of incubation, significant inhibition (>50%) occurredwith $>=$ 0.73 mM ( $-$ )- $alpha$ -pinene (0.1 mg ml¹) (Fig. 2). One-half this amount had no effect on CH₄ oxidation,while a pinene concentration of 1.1 mM inhibited essentially allactivity over a 2-day period. There was no lag phase in CH₄ oxidationwith 0.37 mM pinene, but 0.73 mM pinene resulted in a lag of about1 day before oxidation began (Fig. 2). After an additional 2 to3 days of incubation the culture to which 1.1 mM pinene was addedalso showed CH₄ oxidation (data not shown). Thus, the inhibitoryeffect of this compound is transient under the experimental conditionsdescribed above. Furthermore, the more dilute the culture, thelonger the lag period during which no oxidation occurred (datanot shown). Because ( $-$ )- $alpha$ -pinene was a strong inhibitor of CH₄oxidation, this compound was used extensively in further experiments.

View larger version (16K):
[in this window]
[in a new window]

FIG. 2. Effects of different levels of ( $-$ )- $alpha$ -pinene on CH₄ oxidation by Methylosinus trichosporium OB3b. $alpha$ -Pinene at final concentrations of 0 mM ( $open circle$ ), 0.37 mM ( $black-square$ ), 0.73 mM ( $black-triangle$ ), and 1.10 mM ( $black-down-triangle$ ) was added to cultures having an initial OD₆₀₀ of 0.05. The values are means ± standard errors of the means determined from triplicate experiments. d, day.

View larger version (15K):
[in this window]
[in a new window]

FIG. 3. Changes in the levels of total CH₄ (A) and headspace ( $-$ )- $alpha$ -pinene (B) during CH₄ oxidation by Methylosinus trichosporium OB3b. Control, inoculated flasks were incubated without ( $-$ )- $alpha$ -pinene ( $open circle$ ). ( $-$ )- $alpha$ -Pinene (1.10 mM) was added to both inoculated ( $black-square$ ) and uninoculated ( $black-triangle$ ) flasks. An initial OD₆₀₀ of 0.045 was used. The values are means ± standard errors of the means determined from duplicate experiments. d, day.

To determine if loss or degradation of the monoterpene was responsible for the observed transient inhibition, we monitoredthe headspace ( $-$ )- $alpha$ -pinene content over time in inoculated anduninoculated serum bottles (Fig. 3). CH₄ oxidation again occurredafter a 2-day lag period and was nearly complete after 5 dayswhen 1.1 mM ( $-$ )- $alpha$ -pinene was added. However, the rate of oxidationwas lower than the rate of oxidation in the inoculated controlwithout ( $-$ )- $alpha$ -pinene. The uninoculated control showed little changein CH₄ concentration. The headspace pinene levels (and hence dissolvedlevels) decreased by one-half and at the same rate in both inoculatedand uninoculated flasks (Fig. 3), indicating that microbial degradationor conversion of pinene was not significant. Furthermore, pineneaddition did not stimulate CO₂ production by the methanotrophs,and no conversion products were detected by gas chromatography(data not shown). Thus, it is likely that the decrease in headspace( $-$ )- $alpha$ -pinene content was due to adsorption to the walls or rubberstopper of the incubation vessel.

However, this decrease did not explain the transient nature of pinene inhibition. The level of volatile ( $-$ )- $alpha$ -pinene in theheadspace became stable after about 3 days of preincubation withshaking (Fig. 4). In preincubated flasks, in which the headspace( $-$ )- $alpha$ -pinene levels remained the same over the entire incubationperiod, the same pattern of inhibition was observed. Omittingthe preincubation step resulted in a slightly longer lag phasein CH₄ oxidation (Fig. 4).

View larger version (14K):
[in this window]
[in a new window]

FIG. 4. Changes in the levels of total CH₄ (A) and headspace ( $-$ )- $alpha$ -pinene (B) in preincubated ( $black-square$ ) and nonpreincubated ( $black-triangle$ ) flasks inoculated with Methylosinus trichosporium OB3b. Preincubated flasks were supplemented with ( $-$ )- $alpha$ -pinene and shaken for 3 days before inoculation. Nonpreincubated flasks were inoculated immediately after ( $-$ )- $alpha$ -pinene was added. Control flasks were incubated without ( $-$ )- $alpha$ -pinene ( $open circle$ ). An initial cell OD₆₀₀ of 0.075 and 1.80 mM ( $-$ )- $alpha$ -pinene were used. The values are means ± standard errors of the means determined from triplicate experiments. d, day.

The mechanism of this inhibition is not known. One possibility is that the ( $-$ )- $alpha$ -pinene has a direct effect on the MMO enzyme,as has been suggested for the AMO enzyme (34, 36). Group IImethanotrophs (e.g., Methylosinus trichosporium) express a sMMOenzyme under Cu-deficient conditions and a membrane-bound, particulateMMO (pMMO) enzyme under Cu-sufficient conditions (14, 17).We tested the effect of different forms of pinene on culturesexpressing one or the other of these enzyme forms. CH₄ consumptionby Methylosinus trichosporium OB3b was the same in control cultures(cultures containing no pinene) grown with and without Cu (Table1). However, when cultures were supplemented with different pinenes,CH₄ consumption by Cu-sufficient cultures was inhibited to a greaterextent than CH₄ consumption by Cu-deficient cultures. This trendwas especially evident when (+)- $alpha$ -pinene and ( $-$ )- $beta$ -pinene wereadded; in these cases inhibition of Cu-sufficient cultures wasapproximately 40% greater. Methylobacter luteus, a Group I methanotrophwhich produces only the Cu-dependent pMMO (14, 17), also exhibitedlittle CH₄ consumption with (+)- $alpha$ -pinene compared to Methylosinustrichosporium incubated without Cu (Table 1). Interestingly,( $-$ )- $beta$ -pinene was less inhibitory than the $alpha$ isomers in each case,despite the very similar molecular structures of these compounds(Fig. 1).

View this table:
[in this window]
[in a new window]

TABLE 1. Effects of $alpha$ - and $beta$ -pinenes on CH₄ oxidation by methanotrophs incubated with and without Cu

Effects of different monoterpenoids on CH₄ oxidation. Twelve monoterpenoids, including oxide and alcohol forms, were tested to determine their effects on CH₄ oxidation (Table 2).Activity was measured by measuring the CO₂ produced, since thisprocedure detected low rates of CH₄ oxidation more sensitivelythan measuring CH₄ consumption in a headspace containing 10% CH₄initially. Our experiments showed that no CO₂ production occurredunless CH₄ was present (data not shown), which confirmed the reliabilityof this method. All of the hydrocarbon monoterpenes except $beta$ -myrceneshowed strong inhibition. $beta$ -Myrcene was the only noncyclic unsaturatedhydrocarbon monoterpene used. ( $-$ )- $alpha$ -Pinene, the limonenes, and $gamma$ -terpinene showed the greatest inhibition (>80%). Both $alpha$ -pineneoxide and (R)-(+)-limonene oxide were much less inhibitory thanthe corresponding hydrocarbon forms. (±)-Linalool was significantlymore inhibitory than $beta$ -myrcene, despite the fact that these compoundsare structurally very similar (Fig. 1). This greater inhibitionmay have been related to the much higher aqueous solubility ofthe alcohol monoterpenoids (32). As observed previously (Table1), ( $-$ )- $beta$ -pinene was less inhibitory than ( $-$ )- $alpha$ -pinene. The differencebetween these two forms of pinene is the position of the unsaturatedC-C bond (subterminal in the $alpha$ isomer and terminal in the $beta$ isomer).The results suggest that in general, the lack of a subterminaldouble bond decreases the potential of monoterpenes to inhibitCH₄ oxidation, as shown by the low levels of inhibition observedwith $alpha$ -pinene oxide, ( $-$ )- $beta$ -pinene, and (R)-(+)-limonene oxide,which lack the C-C double bond of the ring (Fig. 1). The presenceof a C ring may also be important, as suggested by the low levelof inhibition observed with $beta$ -myrcene (Table 2).

View this table:
[in this window]
[in a new window]

TABLE 2. Inhibition of CH₄ oxidation by Methylosinus trichosporium OB3b (OD₆₀₀, 0.06) with selected monoterpenes (concentration, 1.8 mM)

Effects of monoterpenes on denitrifiers. Three monoterpenes, ( $-$ )- $alpha$ -pinene, $gamma$ -terpinene, and $beta$ -myrcene, were tested to determine their effects on denitrification byisolates from Hamilton Harbour and Mt. St. Hilaire. The accumulationof N₂O by a Hamilton Harbour isolate (isolate HHI) (Fig. 5A) wasthe same in the presence of acetylene alone and in the presenceof acetylene plus monoterpene, indicating that none of the monoterpenestested inhibited denitrification of nitrate to N₂O. In contrast,a swamp soil isolate (isolate D1) (Fig. 5B) showed N₂O accumulationonly with acetylene alone, and no denitrification occurred when( $-$ )- $alpha$ -pinene was present. Only partial N₂O production (comparedto flasks containing only acetylene) occurred with $gamma$ -terpinene,and $beta$ -myrcene had no effect. A similar pattern was obtained withfour other isolates (HH3, HH4, HH6, and D3), in which case onlyswamp soil isolate D3 showed sensitivity to ( $-$ )- $alpha$ -pinene (datanot shown). Both isolate D1 and isolate D3 also failed to growaerobically in the presence of ( $-$ )- $alpha$ -pinene (data not shown),indicating that this compound exhibited general antimicrobialaction against these organisms. We found no evidence of specificinhibition of N₂O reduction by monoterpenes since no N₂O accumulatedwith monoterpene alone. Our results illustrate the considerabledifferences in tolerance to monoterpenes of different microbes.

View larger version (24K):
[in this window]
[in a new window]

FIG. 5. Effects of selected monoterpenes on denitrification (N₂O accumulation) by environmental isolates from Hamilton Harbour (HH1)(A) and Mt. St. Hilaire (D1)(B). Flasks were incubated with acetylene ( $open circle$ ), monoterpene ( $bullet$ ), and acetylene plus monoterpene ( $black-square$ ). The initial culture densities (OD₆₀₀) were 0.12 (for pinene and terpinene additions) and 0.03 (for myrcene additions). The monoterpene concentrations were 3.70 mM. The results for isolate HH1 (A) are representative of the results obtained with isolates HH3, HH4, HH6, and the results for isolate D1 (B) are similar to the results obtained with isolate D3 (see text). The values are means ± standard errors of the means determined from duplicate experiments. d, day.

Effects of monoterpenes on aerobic activity by several heterotrophs. We compared the sensitivities of methanotrophs and denitrifiers used in this study with the sensitivities of some aerobicallygrown heterotrophic reference strains. ( $-$ )- $alpha$ -Pinene (3.7 mM) hada negligible effect on the final CO₂ concentrations in E. coli,P. aeruginosa, and Serratia marcescens cultures compared to controlcultures, showing that these organisms were not inhibited (Table3). This lack of effect occurred despite the high ratios of monoterpenecontent to cell density used compared to the experiments performedwith methanotrophs (Fig. 1 through 3 and Table 2). However, Staphylococcusaureus produced 33% less CO₂ and B. subtilis produced 98% lessCO₂ in the presence of ( $-$ )- $alpha$ -pinene (Table 3). The levels ofCO₂ evolution during 38 h in E. coli and B. subtilis cultures(initial OD₆₀₀, 0.01) were compared after different ( $-$ )- $alpha$ -pineneconcentrations were added (final concentrations, 0 to 7.3 mM)(Fig. 6). No significant effect was found for E. coli over theconcentration range tested, but for B. subtilis there was a sharpdecrease in CO₂ evolution in the presence of ( $-$ )- $alpha$ -pinene concentrationsgreater than 1.8 mM. Similar inhibition patterns for these bacteriahave been observed with other monoterpenes (7, 27).

View this table:
[in this window]
[in a new window]

TABLE 3. Aerobic metabolism by heterotrophic bacteria (CO₂ evolution over a 38-h period; initial OD₆₀₀, 0.01) in the presence and absence of ( $-$ )- $alpha$ -pinene (concentration, 3.7 mM)

View larger version (15K):
[in this window]
[in a new window]

FIG. 6. Effects of different levels of ( $-$ )- $alpha$ -pinene on aerobic metabolism (CO₂ production) of E. coli ( $bullet$ ) and B. subtilis ( $black-square$ ) over a 38-h period. The initial cell OD₆₀₀ was 0.01. The values are means ± standard errors of the means determined from duplicate experiments.

	DISCUSSION

Top Abstract Introduction Materials & Methods Results Discussion References

The effects of monoterpenoids on microbial growth and activity have been studied primarily to determine the potential useof these compounds in preventing growth of pathogens in the foodindustry (20, 27). Microbial biotransformation of monoterpenoidsinto commercially valuable compounds (10) and degradation ofmonoterpene-containing wastes from industrial sources (19, 24)have also received attention. However, relatively little is knownabout how monoterpenes affect bacterial processes in nature, suchas the cycling of elements. Monoterpene inputs into forest soilsstimulate microbial metabolism (31) and can enhance assimilationof ammonium (9). It has been suggested that monoterpenes areimportant inhibitors of nitrification in some forest soils (34,36) and in cultures of Nitrosomonas europaea (11). Recently,we found that forest soil methanotrophs are similarly inhibited(3). In the current study, we found that cultures of methanotrophsand some denitrifying environmental isolates are more sensitiveto monoterpene inhibition than are several other bacteria.

The magnitude of the inhibitory effect of ( $-$ )- $alpha$ -pinene depended on the concentration of the compound. For example, a ( $-$ )- $alpha$ -pineneconcentration of 0.73 mM was required to cause a significant effecton Methylosinus trichosporium OB3b cultures having an initialOD₆₀₀ of 0.05 (6.75 × 10⁶ cells ml¹ [14]). Other workers have reported that inhibition dependson the ratio of monoterpene to cells for bacteria (27) and yeasts(30). This effect has been interpreted as indicating that cellularuptake of monoterpenes occurs, perhaps into the hydrophobic membrane(30). However, up to tenfold more ( $-$ )- $alpha$ -pinene had little effecton E. coli cultures having much lower initial densities (OD₆₀₀,0.01). Large differences in susceptibility among different bacteria,especially differences among E. coli, Serratia marcescens, andB. subtilis (see above), have also been described by other workers(7, 27), and these differences may depend on the mechanismof action of the compounds (see below). The high sensitivity whichwe observed in methanotrophs, however, is important because ithas an impact on one of the major global CH₄ sinks, biologicalCH₄ consumption (17).

The concentrations of monoterpenes used in this study (0.37 to 3.7 mM or 0.05 to 0.5 mg ml of culture¹) are ecologically relevant. For example, monoterpene levels inexcess of 3 to 5 mg g¹ occur in forest litter layers and fresh foliage (36, 38).Thus, inhibition of methanotrophy in nature by these compoundsis possible, as recently observed with aqueous extracts of otherforest soil components (5). Such an effect is consistent withthe lack of methane consumption seen in the top layers of manyforest soils (1, 6).

The differences in susceptibilities to monoterpenes among denitrifying environmental isolates suggest that any control ofdenitrification by these compounds in different environments dependson the denitrifiers present. The lack of sensitivity of the HamiltonHarbour isolates (HH1, HH3, HH4, and HH6) is interesting in viewof the fact that plant-derived terpenoids induce polychlorinatedbiphenyl degradation by bacteria (13) because of structuralsimilarities between the molecules. Hamilton Harbour is a highlypolluted site containing a variety of industrial wastes, includingaromatic compounds (26). It is possible that bacteria survivingin this environment acquire a tolerance for cyclic organic compounds.Species-specific differences, as observed for E. coli and B. subtilis,may also explain the different levels of tolerance of the denitrifiersto monoterpenes. Although none of the isolates could use ( $-$ )- $alpha$ -pinene, $alpha$ -terpinene, or $beta$ -myrcene as a single carbon source (25), denitrifyingmonoterpene degraders have been isolated from Hamilton Harboursediments (25), as well as from activated sludge and waterloggedforest soil (18). Although we cannot conclude that monoterpenesare specific inhibitors of denitrification, it is clear that thesecompounds inhibit a subset of denitrifiers, which makes them potentialfactors in controlling the process in some environments.

The general antimicrobial properties of monoterpenoids may be related to their interactions with microbial membranes, becauseof their hydrophobicity (30). At high levels (5 mM) they candisrupt electron transport and uncouple oxidative phosphorylationin bacteria (22). Andrews et al. (7) found that $alpha$ -pinene(2 mM) disrupted the cytoplasmic membranes of Saccharomyces cerevisiaeand the gram-positive organism Bacillus thuringiensis, but thatgram-negative bacteria were more resistant to terpenes. $beta$ -Pineneinhibited respiration at the cytochrome b portion of the electrontransport chain of yeast cells (30). White (34, 35) proposeda more specific mechanism for the inhibition of nitrificationby monoterpenes, a mechanism involving direct binding to the AMOenzyme, based on the similarity of these compounds to many knownnitrification inhibitors. Indeed, monoterpene-dependent inhibitionof nitrification by pure cultures of N. europaea does occur (11),but the actual mechanism remains speculative. The similar propertiesof the AMO of nitrifiers and the MMO of methanotrophs (17),including sensitivity to the same inhibitors (8), suggest thatmonoterpenes might inhibit CH₄ oxidation and nitrification insimilar ways.

Green and Dalton (15) found that purified sMMO of Methylococcus capsulatus (Bath) converted $beta$ -pinene to $beta$ -pinene oxide andanother product. This implies that $beta$ -pinene bound to the activesite of the enzyme, a characteristic of a competitive inhibitor.We did not detect any volatile conversion products of $beta$ -pineneor other monoterpenes resulting from incubation with methanotrophiccultures. However, such conversions may have occurred but resultedin products that were below the level of sensitivity of the analyticalmethod used. The higher level of inhibition seen under conditionsthat support expression of the pMMO than under those that supportexpression of the sMMO may indicate that there is an indirecteffect involving membrane disruption by the monoterpenes. It ispossible that a variety of specific and general effects work inconcert to give the inhibition seen with the methanotrophs andother bacteria used in our study.

No matter what the actual mechanisms involved, inhibition showed specificity with regard to monoterpene structure. We foundthat in general, the presence of a C ring and a subterminal C-Cdouble bond was important for inhibition. This differs slightlyfrom White's proposal (34). White postulated that a terminalC-C double bond, when associated with a six-carbon ring structure,should be highly inhibitory to nitrification, since this structureis similar to the structure of many nongaseous inhibitors of AMO.Of course, as discussed above, inhibition by monoterpenes mayoccur via a variety of actions that do not necessarily involvespecific action on an enzyme. Indirect action on associated proteinsand indirect action by chelation of required metals, such as Cu²⁺ (8), are examples of other mechanisms. It should also be notedthat some inhibitors (for example, nitrapyrin) may function differentlyin nitrifiers and methanotrophs (8).

Understanding the mechanism of inhibition should help explain the transient nature of CH₄ oxidation inhibition that we observed.One possible explanation is that, upon initial contact with themonoterpene, a significant fraction of the cells are killed, leadingto a lag phase during which activity by the survivors is undetectable.A variety of physical and chemical factors may also influencethe inhibitory properties of monoterpenes. For example, it hasbeen proposed that molecular aggregation and droplet size affectthe toxicity of monoterpenes (29).

In conclusion, monoterpenes appear to be potentially important inhibitors of processes such as CH₄ oxidation and, in somecases, denitrification. The monoterpene concentrations that weused are environmentally relevant in view of the reported naturallevels (36, 38). Their inhibitory effects of monoterpeneson methanotrophs, for example, may contribute to the stratificationof methane consumption in forest soils (1, 5, 6). Thus,given their widespread distribution, monoterpenes may be regulatorsof microbial processes in nature. Because of the increased useof these compounds by industries (21, 24) and their large-scalerelease by wood pulping processes (19), these effects may beeven more important.

	ACKNOWLEDGMENTS

This work was supported by the Natural Sciences and Engineering Research Council of Canada (NSERC) and by NSERC-BOREAS (BorealEcosystem Atmosphere Study).

	FOOTNOTES

^* Corresponding author. Present address: Department of Biology, University of San Francisco, 2130 Fulton St., San Francisco,CA 94117-1080. Phone: (415) 422-2716. Fax: (415) 422-6363. E-mail:amaral{at}usfca.edu.

REFERENCES

Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References

1. Adamsen, A. P. S., and G. King. 1993. Methane consumption in temperate and subarctic forest soils: rates, vertical zonation, and responses to water and nitrogen. Appl. Environ. Microbiol. 59:485-490[Abstract/Free Full Text].

2. Amaral, J. A., C. Archambault, S. R. Richards, and R. Knowles. 1995. Denitrification associated with Groups I and II methanotrophs in a gradient enrichment system. FEMS Microbiol. Ecol. 18:289-298.

3. Amaral, J. A., and R. Knowles. Unpublished data.

4. Amaral, J. A., and R. Knowles. 1994. Methane metabolism in a temperate swamp. Appl. Environ. Microbiol. 60:3945-3951[Abstract/Free Full Text].

5. Amaral, J. A., and R. Knowles. Inhibition of methane consumption in forest soils and pure cultures of methanotrophs by aqueous forest soil extracts. Soil Biol. Biochem., in press.

6. Amaral, J. A., and R. Knowles. 1997. Localization of methane consumption and nitrification activities in some boreal forest soils and the stability of methane consumption on storage and disturbance. J. Geophys. Res.-Atmos. 102:29,255-29,260.

7. Andrews, R. E., L. W. Parks, and K. D. Spence. 1980. Some effects of Douglas fir terpenes on certain microorganisms. Appl. Environ. Microbiol. 40:301-304[Abstract/Free Full Text].

8. Bédard, C., and R. Knowles. 1989. Physiology, biochemistry, and specific inhibitors of CH₄, NH₄⁺, CO oxidation by methanotrophs and nitrifiers. Microbiol. Rev. 53:68-84[Abstract/Free Full Text].

9. Bremner, J. M., and G. W. McCarty. 1988. Effects of terpenoids on nitrification in soil. Soil Sci. Soc. Am. J. 52:1630-1633. [Abstract/Free Full Text]

10. Chang, H. C., and P. Oriel. 1994. Bioproduction of perillyl alcohol and related monoterpenes by isolates of Bacillus stearothermophilus. J. Food Sci. 59:660-662.

11. Courtney, K. J., B. B. Ward, and J. H. Langenheim. 1991. The effect of coastal redwood monoterpenes on Nitrosomonas europaea. Am. J. Bot. Suppl. 78:144-145.

12. Dev, S. 1982. . Handbook of terpenoids-monoterpenoids, vol. 1 and 2. CRC Press, Boca Raton, Fla.

13. Gilbert, E. S., and D. E. Crowley. 1997. Plant compounds that induce polychlorinated biphenyl biodegradation by Arthrobacter sp. strain B1B. Appl. Environ. Microbiol. 63:1933-1938[Abstract].

14. Graham, D. W., J. A. Chaudhary, R. S. Hanson, and R. G. Arnold. 1993. Factors affecting competition between type I and type II methanotrophs in two-organism, continuous-flow reactors. Microb. Ecol. 25:1-17.

15. Green, J., and H. Dalton. 1989. Substrate specificity of soluble methane monooxygenase: mechanistic implications. J. Biol. Chem. 264:17698-17703[Abstract/Free Full Text].

16. Hakola, H., B. Shorees, J. Arey, and R. Atkinson. 1993. Product formation from the gas-phase reactions of OH radicals and O₃ with $beta$ -phellandrene. Environ. Sci. Technol. 27:278-283.

17. Hanson, R. S., and T. E. Hanson. 1996. Methanotrophic bacteria. Microbiol. Rev. 60:439-471[Abstract/Free Full Text].

18. Harder, J., and C. Probian. 1995. Microbial degradation of monoterpenes in the absence of molecular oxygen. Appl. Environ. Microbiol. 61:3804-3808[Abstract].

19. Keith, L. H. 1976. Identification of organic compounds in unbleached Kraft paper mill wastewaters. Environ. Sci. Technol. 10:555-564.

20. Kim, J., M. R. Marshall, and C. Wei. 1995. Antibacterial activity of some essential oil components against five foodborne pathogens. J. Agric. Food Chem. 43:2839-2845.

21. Kirchner, E. M. 1994. Environment, health concerns force shift in use of organic solvents. Chem. Eng. News 72:13-20.

22. Knobloch, K., H. Weigand, N. Weis, H.-M. Schwarm, and H. Vigenschow. 1986. Action of terpenoids on energy metabolism, p. 429-445. In E.-J. Brunke (ed.), Progress in essential oil research. Walter de Gruyter and Co., Berlin, Germany.

23. Lerdau, M., A. Guenther, and R. Monson. 1997. Plant production and emission of volatile organic compounds. BioScience 47:373-383.

24. Misra, G., S. G. Pavlostathis, E. M. Perdue, and R. Araujo. 1996. Aerobic biodegradation of selected monoterpenes. Appl. Microbiol. Biotechnol. 45:831-838[Medline].

25. Richards, S. R., and R. Knowles. Unpublished data.

26. Richards, S. R., and R. Knowles. 1995. Inhibition of nitrous oxide reduction by a component of Hamilton Harbour sediment. FEMS Microbiol. Ecol. 17:39-46.

27. Subba, M. S., T. C. Soumithri, and R. Suryanarayana Rao. 1967. Antimicrobial action of citrus oils. J. Food Sci. 32:225-227.

28. Trudgill, P. W. 1990. Microbial metabolism of monoterpenes $---$ recent developments. Biodegradation 1:93-105[Medline].

29. Uribe, S., and A. Peña. 1990. Toxicity of allelopathic monoterpene suspensions on yeast. J. Chem. Ecol. 16:1399-1408.

30. Uribe, S., J. Ramirez, and A. Peña. 1985. Effects of $beta$ -pinene on yeast membrane functions. J. Bacteriol. 161:1195-1200[Abstract/Free Full Text].

31. Vokou, D., and N. S. Margaris. 1988. Decomposition of terpenes by soil microorganisms. Pedobiologia 31:413-419.

32. Weidenhamer, J. D., F. A. Macias, N. H. Fischer, and G. B. Williamson. 1993. Just how insoluble are monoterpenes? J. Chem. Ecol. 19:1799-1807.

33. White, C. S. 1986. Volatile and water-soluble inhibitors of nitrogen mineralization and nitrification in forest ecosystems in New Mexico. Biol. Fertil. Soils 2:97-104.

34. White, C. S. 1988. Nitrification inhibition by monoterpenoids: theoretical mode of action based on molecular structures. Ecology 69:1631-1633.

35. White, C. S. 1990. Comments on "Effects of terpenoids on nitrification in soil." Soil Sci. Soc. Am. J. 54:296-297. [Free Full Text]

36. White, C. S. 1994. Monoterpenes: their effects on ecosystem nutrient cycling. J. Chem. Ecol. 20:1381-1405.

37. Whittenbury, R., K. C. Phillips, and J. F. Wilkinson. 1970. Enrichment, isolation and some properties of methane-utilizing bacteria. J. Gen. Microbiol. 61:205-218[Abstract/Free Full Text].

38. Wilt, F. M., G. C. Miller, R. L. Everett, and M. Hackett. 1993. Monoterpene concentrations in fresh, senescent, and decaying foliage of single-leaf pinyon (Pinus monophylla Torr. & Frem.:Pinaceae) from the western Great Basin. J. Chem. Ecol. 19:185-194.

39. Zubyk, W. J., and A. Z. Conner. 1960. Analysis of terpene hydrocarbons and related compounds by gas chromatography. Anal. Chem. 32:912-917.

This article has been cited by other articles:

Nanba, K., King, G. M. (2000). Response of Atmospheric Methane Consumption by Maine Forest Soils to Exogenous Aluminum Salts. Appl. Environ. Microbiol. 66: 3674-3679 [Abstract] [Full Text]
Henckel, T., Jäckel, U., Schnell, S., Conrad, R. (2000). Molecular Analyses of Novel Methanotrophic Communities in Forest Soil That Oxidize Atmospheric Methane. Appl. Environ. Microbiol. 66: 1801-1808 [Abstract] [Full Text]
Cowan, M. M. (1999). Plant Products as Antimicrobial Agents. Clin. Microbiol. Rev. 12: 564-582 [Abstract] [Full Text]
Bodelier, P. L.�E., Frenzel, P. (1999). Contribution of Methanotrophic and Nitrifying Bacteria to CH4 and NH4+ Oxidation in the Rhizosphere of Rice Plants as Determined by New Methods of Discrimination. Appl. Environ. Microbiol. 65: 1826-1833 [Abstract] [Full Text]

This Article

	Abstract
	Full Text (PDF)
	An erratum has been published
	Alert me when this article is cited
	Alert me if a correction is posted

Services

	Similar articles in this journal
	Similar articles in PubMed
	Alert me to new issues of the journal
	Download to citation manager
	Reprints and Permissions
	Copyright Information
	Books from ASM Press
	MicrobeWorld

Citing Articles

	Citing Articles via HighWire
	Citing Articles via Google Scholar

Google Scholar

	Articles by Amaral, J. A.
	Articles by Knowles, R.
	Search for Related Content

PubMed

	PubMed Citation
	Articles by Amaral, J. A.
	Articles by Knowles, R.


Agricola

	Articles by Amaral, J. A.
	Articles by Knowles, R.

1.	Adamsen, A. P. S., and G. King. 1993. Methane consumption in temperate and subarctic forest soils: rates, vertical zonation, and responses to water and nitrogen. Appl. Environ. Microbiol. 59:485-490[Abstract/Free Full Text].
2.	Amaral, J. A., C. Archambault, S. R. Richards, and R. Knowles. 1995. Denitrification associated with Groups I and II methanotrophs in a gradient enrichment system. FEMS Microbiol. Ecol. 18:289-298.
3.	Amaral, J. A., and R. Knowles. Unpublished data.
4.	Amaral, J. A., and R. Knowles. 1994. Methane metabolism in a temperate swamp. Appl. Environ. Microbiol. 60:3945-3951[Abstract/Free Full Text].
5.	Amaral, J. A., and R. Knowles. Inhibition of methane consumption in forest soils and pure cultures of methanotrophs by aqueous forest soil extracts. Soil Biol. Biochem., in press.
6.	Amaral, J. A., and R. Knowles. 1997. Localization of methane consumption and nitrification activities in some boreal forest soils and the stability of methane consumption on storage and disturbance. J. Geophys. Res.-Atmos. 102:29,255-29,260.
7.	Andrews, R. E., L. W. Parks, and K. D. Spence. 1980. Some effects of Douglas fir terpenes on certain microorganisms. Appl. Environ. Microbiol. 40:301-304[Abstract/Free Full Text].
8.	Bédard, C., and R. Knowles. 1989. Physiology, biochemistry, and specific inhibitors of CH₄, NH₄⁺, CO oxidation by methanotrophs and nitrifiers. Microbiol. Rev. 53:68-84[Abstract/Free Full Text].
9.	Bremner, J. M., and G. W. McCarty. 1988. Effects of terpenoids on nitrification in soil. Soil Sci. Soc. Am. J. 52:1630-1633. [Abstract/Free Full Text]
10.	Chang, H. C., and P. Oriel. 1994. Bioproduction of perillyl alcohol and related monoterpenes by isolates of Bacillus stearothermophilus. J. Food Sci. 59:660-662.
11.	Courtney, K. J., B. B. Ward, and J. H. Langenheim. 1991. The effect of coastal redwood monoterpenes on Nitrosomonas europaea. Am. J. Bot. Suppl. 78:144-145.
12.	Dev, S. 1982. . Handbook of terpenoids-monoterpenoids, vol. 1 and 2. CRC Press, Boca Raton, Fla.
13.	Gilbert, E. S., and D. E. Crowley. 1997. Plant compounds that induce polychlorinated biphenyl biodegradation by Arthrobacter sp. strain B1B. Appl. Environ. Microbiol. 63:1933-1938[Abstract].
14.	Graham, D. W., J. A. Chaudhary, R. S. Hanson, and R. G. Arnold. 1993. Factors affecting competition between type I and type II methanotrophs in two-organism, continuous-flow reactors. Microb. Ecol. 25:1-17.
15.	Green, J., and H. Dalton. 1989. Substrate specificity of soluble methane monooxygenase: mechanistic implications. J. Biol. Chem. 264:17698-17703[Abstract/Free Full Text].
16.	Hakola, H., B. Shorees, J. Arey, and R. Atkinson. 1993. Product formation from the gas-phase reactions of OH radicals and O₃ with $beta$ -phellandrene. Environ. Sci. Technol. 27:278-283.
17.	Hanson, R. S., and T. E. Hanson. 1996. Methanotrophic bacteria. Microbiol. Rev. 60:439-471[Abstract/Free Full Text].
18.	Harder, J., and C. Probian. 1995. Microbial degradation of monoterpenes in the absence of molecular oxygen. Appl. Environ. Microbiol. 61:3804-3808[Abstract].
19.	Keith, L. H. 1976. Identification of organic compounds in unbleached Kraft paper mill wastewaters. Environ. Sci. Technol. 10:555-564.
20.	Kim, J., M. R. Marshall, and C. Wei. 1995. Antibacterial activity of some essential oil components against five foodborne pathogens. J. Agric. Food Chem. 43:2839-2845.
21.	Kirchner, E. M. 1994. Environment, health concerns force shift in use of organic solvents. Chem. Eng. News 72:13-20.
22.	Knobloch, K., H. Weigand, N. Weis, H.-M. Schwarm, and H. Vigenschow. 1986. Action of terpenoids on energy metabolism, p. 429-445. In E.-J. Brunke (ed.), Progress in essential oil research. Walter de Gruyter and Co., Berlin, Germany.
23.	Lerdau, M., A. Guenther, and R. Monson. 1997. Plant production and emission of volatile organic compounds. BioScience 47:373-383.
24.	Misra, G., S. G. Pavlostathis, E. M. Perdue, and R. Araujo. 1996. Aerobic biodegradation of selected monoterpenes. Appl. Microbiol. Biotechnol. 45:831-838[Medline].
25.	Richards, S. R., and R. Knowles. Unpublished data.
26.	Richards, S. R., and R. Knowles. 1995. Inhibition of nitrous oxide reduction by a component of Hamilton Harbour sediment. FEMS Microbiol. Ecol. 17:39-46.
27.	Subba, M. S., T. C. Soumithri, and R. Suryanarayana Rao. 1967. Antimicrobial action of citrus oils. J. Food Sci. 32:225-227.
28.	Trudgill, P. W. 1990. Microbial metabolism of monoterpenes $---$ recent developments. Biodegradation 1:93-105[Medline].
29.	Uribe, S., and A. Peña. 1990. Toxicity of allelopathic monoterpene suspensions on yeast. J. Chem. Ecol. 16:1399-1408.
30.	Uribe, S., J. Ramirez, and A. Peña. 1985. Effects of $beta$ -pinene on yeast membrane functions. J. Bacteriol. 161:1195-1200[Abstract/Free Full Text].
31.	Vokou, D., and N. S. Margaris. 1988. Decomposition of terpenes by soil microorganisms. Pedobiologia 31:413-419.
32.	Weidenhamer, J. D., F. A. Macias, N. H. Fischer, and G. B. Williamson. 1993. Just how insoluble are monoterpenes? J. Chem. Ecol. 19:1799-1807.
33.	White, C. S. 1986. Volatile and water-soluble inhibitors of nitrogen mineralization and nitrification in forest ecosystems in New Mexico. Biol. Fertil. Soils 2:97-104.
34.	White, C. S. 1988. Nitrification inhibition by monoterpenoids: theoretical mode of action based on molecular structures. Ecology 69:1631-1633.
35.	White, C. S. 1990. Comments on "Effects of terpenoids on nitrification in soil." Soil Sci. Soc. Am. J. 54:296-297. [Free Full Text]
36.	White, C. S. 1994. Monoterpenes: their effects on ecosystem nutrient cycling. J. Chem. Ecol. 20:1381-1405.
37.	Whittenbury, R., K. C. Phillips, and J. F. Wilkinson. 1970. Enrichment, isolation and some properties of methane-utilizing bacteria. J. Gen. Microbiol. 61:205-218[Abstract/Free Full Text].
38.	Wilt, F. M., G. C. Miller, R. L. Everett, and M. Hackett. 1993. Monoterpene concentrations in fresh, senescent, and decaying foliage of single-leaf pinyon (Pinus monophylla Torr. & Frem.:Pinaceae) from the western Great Basin. J. Chem. Ecol. 19:185-194.
39.	Zubyk, W. J., and A. Z. Conner. 1960. Analysis of terpene hydrocarbons and related compounds by gas chromatography. Anal. Chem. 32:912-917.