BioTechnology Institute and Department of Chemical Engineering and Materials Science1, and BioTechnology Institute and Department of Biochemistry, Molecular Biology and Biophysics2, University of Minnesota, Saint Paul, MN 55108, USA
Author for correspondence: Michael C. Flickinger. Tel: +1 612 624 9259. Fax: +1 612 625 1700. e-mail: mflick{at}biosci.umn.edu
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ABSTRACT |
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Keywords: Gram-positive methylotroph, ribulose monophosphate cycle, formaldehyde oxidation, methanol pulse, formaldehyde toxicity
Abbreviations: RuMP, ribulose monophosphate
a Present address: Pfizer Inc., Groton, CT, 06340, USA.
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INTRODUCTION |
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B. methanolicus is capable of rapid growth on methanol or mannitol in minimal media. Growth on glucose as a sole source of carbon and energy is very slow. Maximum growth rates on methanol occur at 5053 °C (Schendel et al., 1990). Endospore formation is minimal at 50 °C, but more extensive when cultures are shifted from 50 to 37 °C during exponential growth (Schendel et al., 1990 ).
Aerobic methylotrophic proteobacteria possess tetrahydromethanopterin (H4MPT)-dependent enzymes for methanol assimilation (Vorholdt et al., 1999 ). Such enzymes have so far not been found in Gram-positive methylotrophs. B. methanolicus has been shown to contain an NAD-dependent methanol dehydrogenase for the oxidation of methanol to formaldehyde (De Vries et al., 1992
). Formaldehyde is assimilated by the ribulose monophosphate (RuMP) pathway (Arfman et al., 1989, 1991; Dijkuizen et al., 1988
; Vonk et al., 1991
). This pathway may function to detoxify accumulating formaldehyde by assimilation into RuMP and may also dissimilate methanol carbon as CO2 in a cyclic version of the RuMP pathway similar to that in Methylobacillus flagellatus KT (Chistoserdova et al., 2000
). In addition to methanol dehydrogenase, crude cell extracts of B. methanolicus MGA3 grown on methanol contain a high specific activity of hexulose-6-phosphate synthase [3·726·27 mmol formaldehyde (mg protein)-1 min-1; Schendel et al., 1990]. However, little else is known about the pathways of formaldehyde assimilation or dissimilation (as CO2) that may play a role in detoxifying formaldehyde.
This study utilized continuous, steady-state methanol-limited cultures of B. methanolicus MGA3 growing at 50 °C to investigate the growth-inhibitory effects of pulses of methanol that perturb steady-state methanol concentrations. Using the methods described here, the degree of methanol toxicity could be quantified, and the physiological response elucidated using 13C NMR and isotope-ratio mass spectrometry. In recent years, NMR and GC-MS techniques have become well established as powerful tools in identifying novel metabolic pathways and flux patterns by unambiguous in vivo detection of intermediates (Bacher et al., 1998 ; Shimizu, 2000
). Representative examples are the investigation of the metabolism of cosubstrates in Penicillium chrysogenum (Christensen & Nielsen, 2002
), the identification of pathway intermediates in fluoranthene metabolism in mycobacteria (Rehmann et al., 2001
), and the in situ monitoring of biotransformations (Brecker & Ribbons, 2000
; Brecker et al., 2000
). In the case of B. methanolicus MGA3, in vivo evidence supporting a pathway of methanol dissimilation via formate to CO2 was found using 13C NMR and isotope-ratio mass spectrometry that has previously not been reported in Gram-positive methylotrophic bacilli.
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METHODS |
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Continuous-culture growth conditions.
B. methanolicus MGA3 was grown continuously in a stirred-tank, 2 litre jacketed glass bioreactor (Applikon Dependable Instruments), which was operated with a constant liquid volume of 1000 ml. Containers with sterile feed medium were placed on a top-loading electronic balance (Mettler PE16), which was interfaced with a microprocessor-controlled pump (Scilog Expert CP-120). A mass-flow control program was used so that the feed rate was constant and independent of tubing fatigue. A pressurized feed port was designed (as described by Evans et al., 1970 ) in order to reduce back-growth contamination from the reactor into the feed carboy. A sample port constructed in the feed line allowed sampling from the medium under sterile conditions for determination of the bioreactor inlet methanol concentration. The pH of the culture was controlled at 6·7±0·05 (Metrohm) using 8 M potassium hydroxide. The dissolved O2 tension was monitored with a galvanic oxygen probe (Johnson et al., 1964
). Both the pH and the dissolved O2 tension were recorded on a PC. The temperature in the reactor was controlled at 50±0·5 °C. The entire apparatus including the media feed tanks was enclosed in a walk-in incubator. The agitation speed was 600 r.p.m. The culture was oxygenated with air at a rate of 1 litre min-1 (at standard conditions: 105 Pa, 21 °C) to maintain a dissolved O2 tension of approximately 7 kPa. About 2 % (20 ml min-1) of the total gas flow into the reactor was used to create a jet in the pressurized feed port. The flow meter measuring the total gas flow was calibrated for an operating pressure of 1·3 atm (1 atm=105 Pa) in the reactor. The inlet and outlet gas streams were analysed on-line using a quadropole mass spectrometer (Questor High Speed Process Analyser, Extrel Corporation). Calibration was carried out once a week for nitrogen, O2, CO2, argon, water, ammonia and methanol. The total scan time required to measure all components in a sample stream was 6 s. The lag time between a change in the concentration in the reactor and the mass spectrometer response was 1·5 min. The analysis of the inlet and exit gas streams was used to determine on-line the O2 uptake rate, the CO2 evolution rate and the respiratory quotient of the continuously growing culture of B. methanolicus MGA3.
Using this apparatus, a methanol-limited continuous culture could be maintained for several weeks. Negligible wall growth above the liquid level in the reactor occurred after 2 weeks. Direct gravimetric measurements of the vessel wall growth dry biomass showed that this fraction of the biomass never exceeded 1% of the total biomass generated during the continuous-culture experiment.
Determination of residual methanol, cell yield and formic acid.
Residual methanol concentration in the reactor and culture samples was measured by immediately filtering reactor samples (Acrodisc, 0·2 µm pore size, low-protein-binding HT Tuffryn membrane) followed by analysis by gas chromatography (Hewlett Packard, model 5890) using a flame-ionization detector and a 30 m DB-WAX column (Chrom Tech). The dry biomass concentration in the reactor was determined directly by drying and weighing. A 25 ml sample of culture suspension was centrifuged for 10 min at 4 °C and 17000 g in a Beckman centrifuge (model J2-21, JA 20 rotor). The supernatant was discarded, the cell pellet resuspended in 12 ml minimal salts solution (MS), and centrifuged again for 10 min. The cell pellet was resuspended in 12 ml fresh MS and dried at 80 °C in aluminium cups to a constant mass. Two 12 ml samples of MS were also dried to correct for salt mass. MS was used instead of distilled water in order to prevent any cell lysis during centrifugation or resuspension. The dry biomass concentration (g l-1) was calculated as the mean of four replicate determinations.
Formic acid was measured by the combined use of gas chromatography and isotope-ratio mass spectrometry (Kratos MS25 GC/MS) equipped with a 30 m DB-WAX capillary column (Chrom Tech). Ionization was accomplished by electron impact at 70 eV. A 100 mM aqueous solution of [13C]formic acid (99% 13C, Cambridge Isotope Laboratories) was diluted tenfold in 0·3 M H2SO4 and then mixed 1:1 with samples of culture supernatant. Calibration was performed by using aqueous solutions with known concentrations of [12C]formic acid (Mallinckrodt, analytical reagent) between 0 and 20 mM. One millilitre was injected into the gas chromatograph. The oven temperature was held at 80 °C for 1 min, and then increased to 200 °C at a rate of 25 °C min-1, with a holding time of 5 min. The ratio of the ion intensities measured at mass 46 and mass 47 was used as the measure of the [12C]formic acid concentration in the sample. Samples were measured in triplicate and the results averaged.
Transient changes in methanol concentration.
The effect of transient changes in the concentration of methanol in the reactor were investigated at a dilution rate of 0·25 h-1, limited by 100 mM methanol in the feed. Steady-state conditions were disturbed by injecting 613 mmol methanol through a septum directly into the reactor. The amount of methanol injected was varied in order to study the effect of different initial methanol concentrations on the cultures response. One sample of the culture was taken immediately after methanol addition, rapidly sterile-filtered, and the initial concentration of methanol measured by gas chromatography. Subsequent samples were taken to follow the time-course of the dry biomass and the methanol concentration in the reactor in response to each methanol pulse. Mass spectrometry was used to monitor the effect of the transient increase in methanol on the O2 uptake rate and the CO2 evolution rate of the perturbed (non-steady-state) culture.
13C NMR methods.
In vivo 13C NMR experiments were performed on oxygenated suspensions of B. methanolicus MGA3 taken from a continuous culture growing at a dilution rate (D) of 0·1 h-1. Methanol was the limiting substrate at a feed concentration of 300 mM. A sample volume of 25 ml was taken from the chemostat and immediately centrifuged for 10 min at 4 °C and 17000 g in a centrifuge (Beckman model J2-21). The cell pellet was then resuspended in 5 ml fresh, chilled (approx. 4 °C) MY medium that did not contain methanol. A cell density of about 20 g l-1 was needed to achieve sufficient NMR signal intensity. This concentrated cell suspension was kept cold on ice for no more than 10 min. Just before use, the suspension was warmed to 50 °C in a water bath. Measurements were made using 4 ml culture in a 12 mm NMR tube (514A-7PP, Wilmad) equipped with a glass capillary to allow in situ aeration (see below); 75·46 MHz 13C NMR spectra were obtained with a Nicolet NT300WB spectrometer. 3-Trimethylsilylpropionate (TMSP) was used to calibrate the chemical shift prior to the experiment. Generally, 132 transients were acquired every 5 min, using a 70° pulse, and 8096 data points over 18180 Hz spectral width. High-level (2 W) proton irradiation was used during the pulse and acquisition to ensure good proton decoupling. Before Fourier transformation, 15 Hz line broadening was applied to the signal to improve the signal-to-noise ratio.
13C NMR investigations were carried out to determine the flow of carbon in B. methanolicus MGA3 when the cells were exposed to a pulse of methanol. During these NMR experiments, the temperature was maintained at 50 °C. In situ aeration (approx. 20 ml min-1; 40% O2 in air) was achieved with a small glass capillary fixed in place inside the NMR tube and connected to a supply of pressurized air and O2. Maintaining aerobic conditions and controlling the temperature at 50 °C was necessary, because otherwise neither significant methanol consumption nor accumulation of metabolites was observed. After establishing a baseline for 5 min, a 40 µl pulse of methanol (99% 13C, Cambridge Isotope Laboratories) was added to the aerated cell suspension, resulting in an initial concentration of 250 mM methanol. The flux of carbon was monitored by continuing to acquire and superimpose 132 spectra every 5 min for a total time period of 3 h.
The chemical shifts of formaldehyde (82 p.p.m.) and formate (split peak at 170 p.p.m., 172 p.p.m.) were confirmed by acquiring and superimposing approximately 1600 scans of aqueous solutions of these compounds (natural 13C enrichment) for 1 h. For formaldehyde, 3 ml water was mixed with 1 ml of a 30 g l-1 solution of formaldehyde freshly prepared from paraformaldehyde (Sigma) and 200 µl methanol (49 p.p.m.) as a reference. For formate, 4 ml of a 30 g l-1 solution of sodium formate (Mallinckrodt, analytical reagent) was mixed with 200 µl methanol.
Detection of conversion of formic acid to CO2.
Experiments were designed to investigate whether B. methanolicus MGA3 was able to metabolize formic acid to CO2 by growing the strain in continuous culture at a dilution rate of 0·25 h-1 under methanol-limiting conditions (100 mM feed concentration). At steady state, 250 ml of reactor exhaust gas was collected and sealed in a glass bomb (Fisher). A pulse of [13C]formic acid (99% 13C, Cambridge Isotope Laboratories) was then applied to the cells by injection through a septum in the reactor head plate, resulting in an initial concentration of approximately 2 mM. After this pulse, a second sample of exhaust gas was collected. From both gas samples, the CO2 was purified cryogenically by first applying a strong vacuum (0·13 Pa) at -79 °C, and then freezing the CO2 and sealing it in a glass tube cooled to liquid nitrogen temperature. These CO2 samples were subsequently analysed using a dual-inlet isotope-ratio mass spectrometer (Finnigan MAT Delta E).
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RESULTS |
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Fig. 1(a, b
, c
) shows examples of how B. methanolicus MGA3, growing at steady state under methanol-limited conditions, responded to a pulse of methanol which abruptly increased the ambient methanol concentration. The steady-state culture had a dry biomass concentration of 1·59±0·03 g l-1, an O2 uptake rate of 17·3±0·37 mmol l-1 h-1 and a CO2 evolution rate of 6·68±0·10 mmol l-1 h-1. The resulting respiratory quotient was 0·39.
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The data acquired in an experiment in which the methanol pulse was increased to an initial concentration of 10·9 mM in the reactor are summarized in Fig. 1(b). The characteristics of the response were analogous to those described above for a pulse of 8·9 mM, but more strongly pronounced. Within the first hour after application of the additional methanol, the residual concentration was reduced to 3·5 mM concomitantly with a transient rise in the O2 uptake rate and a decrease in the respiratory quotient. The biomass was partially washed out of the reactor and reached its minimum concentration of 0·8 g l-1 (50% of the steady-state value) at approximately 4·5 h. Simultaneously, the remaining cells were unable to consume all the methanol entering the reactor, causing the residual concentration to rise to a maximum of almost 20 mM at 6·5 h. This increase occurred gradually over a time period of 5 h and is therefore distinctly different from the sudden pulse to the methanol-limited culture at the beginning. It took 12 h for the culture to return to steady state.
Fig. 1(c) shows how the continuous, methanol-limited culture of B. methanolicus MGA3 responded to a methanol pulse resulting in a change in concentration to 12·8 mM in the reactor. Contrary to the previous cases described, the culture was now unable to return to steady state. Instead, after 14 h, the biomass was almost completely washed out of the reactor.
A computational analysis was carried out in order to compare steady-state characteristics with the cases in which the culture was disturbed by a transient increase in methanol concentration. A 12 h time period, beginning with the application of the methanol pulse, was chosen as the basis for comparison. Only those cases were considered in which the culture was able to return to steady state, i.e. the size of the pulse was 10·9 mmol methanol. Integration of the CO2 evolution rate, the O2 uptake rate, the residual methanol concentration and the dry biomass concentration was performed for all cases. Under the given conditions, the non-steady-state mass balances for methanol and biomass simplified to:
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where F is the feed rate (0·25 l h-1), cin the methanol concentration in the feed (100 mM), c the methanol concentration in the reactor (mM), CH3OHpulse the methanol added with the pulse (mmol), t time (h) and x the biomass concentration in the reactor (g l-1).
The trapezoidal rule was applied to integrate the discrete data. O2 consumption and CO2 production were calculated similarly using the on-line data. The results of the analysis are summarized in Table 1. In comparison to steady-state conditions, the biomass production was reduced by 2% (6·4 mmol methanol pulse) to 27% (10·9 mmol methanol pulse). Similarly, the biomass yield on methanol decreased by 2% to 22% with increasing pulse size, which is also reflected in the increase of the mean specific rate of methanol consumption. Furthermore, the sudden transient increase in the ambient methanol concentration caused an overall increase in the amount of CO2 produced and O2 consumed during the production of a fixed amount of dry biomass. CO2 production increased by 4% to 21% over steady-state production, reflected in an equivalent decrease in the biomass yield on evolved CO2, YX/CO2 (g mol-1). Simultaneously, O2 consumption rose by 4% to 27%, expressed in the decline of the biomass yield on consumed O2, YX/O2 (g mol-1). Carbon balances were calculated for all cases, using a biomass composition of 51·8% (w/w) carbon (Pluschkell, 1999
). For steady-state conditions, >95% of all carbon is recovered in biomass, CO2 and residual methanol. With increasing strength of the methanol pulse, carbon recovery declined from approximately 94% to 80%, indicating that metabolites that were not accounted for probably accumulated intra- or extracellularly as the size of the methanol pulse was raised.
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Fig. 2 summarizes the response of B. methanolicus MGA3, taken from a methanol-limited continuous culture, to a pulse of [13C]methanol (initial concentration 250 mM). Each spectrum shown represents 132 scans superimposed over a time period of 5 min. The methanol pulse was applied after acquiring a baseline for the first 5 min. The experiment was completed after 3 h (36 spectra). The decline in the intensity of the methanol signal (chemical shift 49 p.p.m.) with time indicates consumption by the cells. Cell-free experiments in the aerated NMR tube showed that the rate of loss of methanol due to evaporation was negligible over this same time period. Assuming a linear relationship between the methanol concentration and the NMR signal, the data were integrated to determine the time-course of the methanol concentration and to estimate the specific rate of methanol consumption at a cell density of 20 g l-1 (Fig. 3
). The steady-state specific rate of methanol consumption in the chemostat was approximately 7·5 mmol g-1 h-1 using a 300 mM methanol feed and D=0·1 h-1. The initial rate in the NMR experiment was significantly higher at approximately 18·5 mmol g-1 h-1, approaching the steady-state rate at about 0·5 h, and gradually declining as methanol was being consumed. After 2·5 h, methanol was almost completely metabolized. This increased rate of methanol consumption in the beginning of the experiment was expected from the results of the transient chemostat studies, where immediately after a methanol pulse, the initial specific rate of methanol consumption was 25 mmol g-1 h-1. Simultaneous with methanol consumption was the appearance of three peaks identified as metabolites. Two of them were formaldehyde (82 p.p.m.) and formate (171 p.p.m.). The third compound (65 p.p.m.) was more difficult to identify conclusively because the 13C spectra of many phosphorylated monosaccharides display signals of similar chemical shift. When methanol is assimilated into the RuMP pathway, it is first incorporated into hexulose 6-phosphate as the C-1 carbon atom, and then becomes the C-1 atom of fructose 6-phosphate in the next reaction (Anthony, 1982
). 13C NMR data support the hypothesis that the signal at 65 p.p.m. may be caused by 1-[13C]fructose 6-phosphate (Levy et al., 1980
). The 13C spectrum of hexulose 6-phosphate is not reported. This signal may be a 1-[13C]hexose phosphate; however, further evidence is required for a more conclusive identification. The signal is not glucose 6-phosphate since the C-1 carbon atom of
-D-glucose in water has a much higher chemical shift of approximately 94 p.p.m. (Levy et al., 1980). Glucose 6-phosphate is the product of fructose 6-phosphate isomerization in the dissimilatory RuMP cycle proposed by Arfman et al. (1989)
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Within 5 min after the application of the methanol pulse, formaldehyde began to accumulate. A small signal for a hexose phosphate was also detected, whereas no formate had yet accumulated to a detectable concentration (in the order of 1 mM). Within 15 min, the formaldehyde signal increased to its maximum intensity. Formate was first detected 10 min after application of the methanol pulse. Over the 3 h time period, the methanol signal continued to decline in intensity and almost vanished by the end of the experiment. The formaldehyde peak decreased slowly after 15 min, but never completely disappeared. The signals corresponding to formate and hexose phosphate followed a parallel time-course, increasing for approximately the first 45 min and then remaining nearly constant.
Oxidation of formate by B. methanolicus: detection by isotope-ratio mass spectrometry
The 13C NMR investigation described above demonstrated that, under certain conditions, methanol metabolism by B. methanolicus MGA3 results in the biosynthesis of formate. The next step was to determine whether formate could be further oxidized to CO2 by an enzyme such as an NAD-dependent formate dehydrogenase (Anthony, 1978 ). Dissolved 13CO2 or bicarbonate is usually too dilute to be detected in 13C NMR studies of aerated cell suspensions, or may only generate a very low-intensity signal (Cornish et al., 1984
). It was therefore necessary to find a different approach to investigate potential CO2 production from formate. The method chosen was to measure 13CO2 enrichment in the gas phase of a continuous culture of B. methanolicus MGA3 in response to a pulse of [13C]formic acid using isotope-ratio mass spectrometry. An enrichment as low as 0·01% can be detected.
A preliminary experiment was performed to determine whether B. methanolicus MGA3 growing continuously under methanol limitation is able to take up formate from the culture supernatant. Fig. 5 summarizes the response of B. methanolicus MGA3 to a pulse of sodium formate (Mallinckrodt, analytical reagent) resulting in an initial concentration of 15·7 mM at time zero. Prior to adding the pulse, the culture was at steady state, growing at a dilution rate D=0·25 h-1 with 100 mM methanol in the feed. The concentration of formate in samples of culture supernatant was measured by combined gas chromatography and isotope-ratio mass spectrometry (see above). The formate pulse caused a transient decrease in the dry biomass concentration. This was expected from batch-culture experiments, which showed that formate pulse additions can reduce the growth rate of B. methanolicus MGA3 by up to 30% in the presence of methanol (Pluschkell, 1999
). In this continuous-culture experiment, the cells washed out at an initial rate of approximately 0·22 h-1, i.e. they grew only at a mean rate of 0·03 h-1. The minimum dry biomass concentration of 1·14 g l-1 almost 30% less than at steady state was reached after approximately 3 h. The cultures biomass level then returned to steady state. Interestingly, the formate pulse provoked a transient increase in the specific CO2 evolution rate and the respiratory quotient. The specific CO2 evolution rate reached a maximum of approximately 5·2 mmol g-1 h-1 2 h after the pulse, a value 20% higher than at steady state. This temporary increase may have been caused either by an increase in the specific rate of methanol dissimilation or by CO2 production from formate. In Fig. 5
, the time-course of the measured residual formate concentration in the culture supernatant is compared with the concentration profile predicted for simple washout of formate, i.e. the case of no uptake of formate by B. methanolicus MGA3. The concentration declined more quickly with time than could be explained by washout alone. If a constant rate of formate uptake by the culture is assumed, this rate can be estimated by:
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Integration from c0 (at t=0) to c (at t) under the assumption that q is constant, gives:
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Thus, the formate uptake rate q can be estimated from a linear regression of c versus exp(-Dt). Using the measured concentration data for the time period of 0 to 4 h, the following result was obtained:
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and with D=0·25 h-1 and c0=15·7 mM:
q=(0·85±0·15) mmol l-1 h-1
Formate uptake by continuously growing, methanol-limited B. methanolicus MGA3 was significant. The observed volumetric uptake rate of 0·85 mmol l-1 h-1 translates into a specific uptake rate in this experiment of approximately 0·650·77 mmol g-1 h-1. If all of the formate taken up was oxidized to CO2 at the same rate, it would approximately account for the transient increase in the specific CO2 evolution rate by 0·620·86 mmol g-1 h-1 above the steady-state value.
With these data indicating that B. methanolicus may be able to consume formate, an experiment was designed to measure 13CO2 production in response to a pulse of [13C]formic acid. A continuous culture of B. methanolicus MGA3 was grown at steady state and limited by 100 mM methanol in the feed, when [13C]formic acid was injected to yield an initial concentration of approximately 2 mM in the reactor. Samples of exhaust gas were collected before and after the pulse, the CO2 was purified and then analysed for the fraction of the 13C isotope by dual-inlet isotope-ratio mass spectrometry. Before [13C]formic acid addition, a fraction of 1·02% of the 13C isotope was found in the CO2 sample, which is equivalent to natural abundance. After [13C]formic acid addition, the fraction of 13CO2 was increased to 2·15%. With the sensitivity of the method being in the order of 0·01%, these data indicate a significant enrichment of 13CO2 in the sample taken after application of the [13C]formic acid pulse. This result is in agreement with all other observations and provides further evidence that B. methanolicus MGA3 is able to oxidize formic acid to CO2.
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DISCUSSION |
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Evidence for the toxicity of transient accumulation of formaldehyde in response to fluctuating methanol concentration
The 13C NMR experiments indicate that the transient partial and the complete biomass washout are probably caused by a transient toxic accumulation of formaldehyde, the first intermediate of methanol metabolism. This agrees with previous investigations of methylotrophic bacteria (Al-Awadhi et al., 1988 , 1990
; Brooke et al., 1989
, 1990
; Gírio et al., 1995
). Formaldehyde accumulation in response to a methanol pulse may be a sign that B. methanolicus MGA3 is unable to rapidly increase formaldehyde detoxification when a sudden increase in the rate of methanol oxidation occurs by methanol dehydrogenase. The rate of formaldehyde consumption appears to be slow, with formaldehyde still being detected 3 h after addition of the pulse (Fig. 2
). This may be caused either by a decrease in B. methanolicus MGA3 cell viability due to in vivo reaction of free formaldehyde, or by the in vivo kinetics of the activity of either hexulose-6-phosphate synthase or formaldehyde dehydrogenase. The initial rate of methanol utilization by the cells was similar in the NMR studies and the transient chemostat experiments (18·5 and 25 mmol g-1 h-1, respectively), indicating that formaldehyde probably accumulated transiently in the chemostat as well. According to Arfman et al. (1989
, 1991
), the syntheses of methanol dehydrogenase and hexulose-6-phosphate synthase are not under coordinate control in thermotolerant, methylotroph bacilli. In addition, methanol dehydrogenase may constitute up to 22% of total soluble protein in the strain B. methanolicus C1 growing in continuous culture under methanol limitation (Arfman et al., 1989
). This implies that growth of B. methanolicus strains may generally be very sensitive to sudden changes in the dissolved methanol concentration due to the risk of formaldehyde accumulation.
Evidence for formate accumulation in B. methanolicus in response to fluctuating methanol concentration
The 13C NMR data show accumulation of formate, indicating that B. methanolicus contains formaldehyde dehydrogenase activity. In addition, the studies using isotope-ratio mass spectrometry provided further evidence for the continuation of this pathway via formate dehydrogenase, resulting in a methanol dissimilation pathway via formate to CO2. B. methanolicus MGA3, growing continuously under methanol limitation, consumed formate pulsed into the culture at a rate of approximately 0·85 mmol l-1 h-1. Furthermore, significant accumulation of 13CO2 in the reactor exhaust gas was measured in response to a pulse of [13C]formic acid to the culture. The biosynthesis of formate in the dissimilation of methanol by a Gram-positive methylotrophic Bacillus has not to our knowledge been reported before. Arfman et al. (1989 , 1992
) investigated similar thermotolerant, methylotrophic Bacillus strains, among them B. methanolicus PB1, whose 16S rRNA sequences match that of MGA3 to 99%. Using enzyme activity assays, this group concluded that formaldehyde dissimilation is by way of the dissimilatory RuMP cycle. However, the conditions of the cell extract preparation and the assay itself may not have been sufficiently sensitive to detect formaldehyde and formate dehydrogenase activity.
Distribution of 13C-labelled methanol carbon in B. methanolicus
Fig. 6 shows the proposed flow of 13C-labelled carbon in B. methanolicus MGA3 from methanol into the dissimilatory and assimilatory pathways. [13C]Methanol dissimilation to formaldehyde, formic acid and CO2 has been shown by our investigations using 13C NMR techniques and isotope-ratio mass spectrometry. The 65 p.p.m. signal detected in the 13C NMR studies is likely to be the C-1 atom of hexulose 6-phosphate, fructose 6-phosphate, or fructose 1,6-bisphosphate (Levy et al., 1980
). These three compounds are the first intermediates in all variants of the assimilatory RuMP cycle (Anthony, 1982
). Activities of the enzymes involved in this cycle have been detected in thermotolerant, methylotrophic Bacillus strains similar to B. methanolicus MGA3 (Arfman et al., 1989
). Arfman et al. (1989)
also found enzyme activities in these strains for dissimilation of methanol via glucose 6-phosphate in the dissimilatory RuMP cycle (Anthony, 1982
). The activity of glucose-6-phosphate isomerase catalysing the initial reaction that produces glucose 6-phosphate from fructose 6-phosphate was measured in extracts of methanol-grown Bacillus sp. C1 to be approximately 1·4 µmol min-1 (mg protein)-1 (Arfman et al., 1989
). The 13C flux investigations carried out with B. methanolicus MGA3 suggest the activity of both the linear and the cyclic dissimilation pathways. The pathway via formate may play a specific role as a detoxifying reaction, and may be undetectable in cultures that have not been exposed to rapid transients in the dissolved methanol concentration. Similar observations were made by Jones & Bellion (1991)
, who applied an in vivo 13C NMR method to cultures of the methylotrophic yeast Hansenula polymorpha. Only cells exposed to high methanol concentrations oxidized the substrate very rapidly, resulting in formaldehyde accumulation.
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ACKNOWLEDGEMENTS |
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Received 8 January 2002;
revised 17 May 2002;
accepted 9 July 2002.