Skip to main page content

• HOME
• Current Issue
• Archive
• Alerts
• About ASM
• Contact us
• Tech Support
• Journals.ASM.org

This Article Abstract Full Text (PDF) Supplemental material 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 Fuhrer, T. Articles by Sauer, U. Search for Related Content PubMed PubMed Citation Articles by Fuhrer, T. Articles by Sauer, U.

 Previous Article  |  Next Article 

Journal of Bacteriology, March 2005, p. 1581-1590, Vol. 187, No. 5
0021-9193/05/$08.00+0     doi:10.1128/JB.187.5.1581-1590.2005
Copyright © 2005, American Society for Microbiology. All Rights Reserved.

Experimental Identification and Quantification of Glucose Metabolism in Seven Bacterial Species

Tobias Fuhrer,¹ Eliane Fischer,¹ and Uwe Sauer^1*

Institute of Biotechnology, ETH Zürich, Zürich, Switzerland¹

Received 3 October 2004/ Accepted 17 November 2004

Top Abstract Introduction Materials and Methods Results Discussion References

 
The structurally conserved and ubiquitous pathways of central carbon metabolism provide building blocks and cofactors for the biosynthesis of cellular macromolecules. The relative uses of pathways and reactions, however, vary widely among species and depend upon conditions, and some are not used at all. Here we identify the network topology of glucose metabolism and its in vivo operation by quantification of intracellular carbon fluxes from ¹³C tracer experiments. Specifically, we investigated Agrobacterium tumefaciens, two pseudomonads, Sinorhizobium meliloti, Rhodobacter sphaeroides, Zymomonas mobilis, and Paracoccus versutus, which grow on glucose as the sole carbon source, represent fundamentally different metabolic lifestyles (aerobic, anaerobic, photoheterotrophic, and chemoheterotrophic), and are phylogenetically distinct (firmicutes, -proteobacteria, and -proteobacteria). Compared to those of the model bacteria Escherichia coli and Bacillus subtilis, metabolisms of the investigated species differed significantly in several respects: (i) the Entner-Doudoroff pathway was the almost exclusive catabolic route; (ii) the pentose phosphate pathway exhibited exclusively biosynthetic functions, in many cases also requiring flux through the nonoxidative branch; (iii) all aerobes exhibited fully respiratory metabolism without significant overflow metabolism; and (iv) all aerobes used the pyruvate bypass of the malate dehydrogenase reaction to a significant extent. Exclusively, Pseudomonas fluorescens converted most glucose extracellularly to gluconate and 2-ketogluconate. Overall, the results suggest that metabolic data from model species with extensive industrial and laboratory history are not representative of microbial metabolism, at least not quantitatively.

Top Abstract Introduction Materials and Methods Results Discussion References

 
Based on ¹³C tracer experiments, metabolic-flux analysis emerged as a key methodology to identify the network topology of active reactions and to quantify the in vivo distribution of molecular fluxes throughout metabolism (38, 47). In contrast to global protein, mRNA, or metabolite concentration analyses that assess network composition, flux methods directly assess the operation of metabolic networks by quantifying in vivo reaction velocities. The general principle is based on mass spectrometry (MS) or nuclear magnetic resonance detection of ¹³C patterns in products of metabolism. Often, protein-bound amino acids that preserve the carbon backbone of eight metabolic key intermediates are used. The detected ¹³C isotope patterns then reflect the activity of intracellular pathways and reactions, whose fluxes can be quantified from the isotope data by using mathematical models with various levels of complexity. In the simplest approach, algebraic equations are used to determine strictly local ratios of converging fluxes analytically by so-called metabolic-flux ratio (METAFoR) analysis (3, 16, 41, 44). Absolute intracellular fluxes in millimoles per gram of biomass per hour may be estimated indirectly by combining such ¹³C data with quantitative physiological data on fluxes in and out of cells (47). In this case, the estimated fluxes are the best fit to the available data within the specified metabolic model. Beyond the quantification of flux through the well-known biochemical pathways, flux methods have recently demonstrated their value for the identification of novel (17) or unexpected (22, 34, 39, 40) metabolic pathways.

For obvious reasons, such flux methods were applied primarily to model microbes with industrial relevance, such as Escherichia coli (15, 24, 41), Bacillus subtilis (9, 40), Corynebacterium glutamicum (30, 48), and Saccharomyces cerevisiae (3, 19). While the accumulated biochemical and metabolic data on these species are also the basis of much of our textbook knowledge, it is clear that these model species are not representative for all, and perhaps not even for most, microbes. One example is the widely distributed Entner-Doudoroff (ED) pathway (6, 26), the genes for which are absent from B. subtilis, S. cerevisiae, and C. glutamicum and which is used by E. coli mainly during growth on gluconate (14). For glucose metabolism, all four model species rely primarily on the Emden-Meyerhof-Parnas (EMP) pathway and, in some cases, to a substantial extent also on the pentose phosphate (PP) pathway (9, 16, 19, 48, 53). These facts raise the general question of how representative the accumulated metabolic knowledge on these model species is. Here we attempt a quantitative comparison of the intracellular metabolisms of the two model microbes E. coli and B. subtilis with those of seven metabolically and phylogenetically distinct species that can grow on glucose as the sole carbon source.

In particular, we identify the network topology of active reactions by METAFoR analysis based on gas chromatography (GC)-MS analysis of proteinogenic amino acids from [U-¹³C]glucose and [1-¹³C]glucose batch experiments (16). Quantification of in vivo molecular fluxes is then achieved by ¹³C-constrained flux analysis (18, 40). In particular, we chose the anaerobic organism Zymomonas mobilis; members of the family Rhizobiaceae, i.e., Agrobacterium tumefaciens and Sinorhizobium meliloti; the metabolically versatile facultative phototroph Rhodobacter sphaeroides; the facultative autotroph Paracoccus versutus; and the versatile pseudomonads Pseudomonas fluorescens and Pseudomonas putida.

Top Abstract Introduction Materials and Methods Results Discussion References

 
Strains, media, and growth conditions. The following nine bacterial species or strains were analyzed: A. tumefaciens C58 (F. Narberhaus), P. fluorescens 52-1C (B. Witholt), P. putida KT2440 (B. Witholt), R. sphaeroides ATH 2.4.1 (German Collection of Microorganisms and Cell Cultures, DSMZ 158), Paracoccus versutus A2 (DSMZ 582), S. meliloti (DSMZ 1981), Z. mobilis NRRL B-806 (DSMZ 424), E. coli MG1655 (E. coli Genetic Stock Center, 6300), and B. subtilis 168 trpC2 (Bacillus Genetic Stock Center). Aerobic batch cultures were grown at 30°C in 500-ml baffled flasks with 50 ml of M9 minimal medium (Paracoccus versutus and Z. mobilis were grown in special minimal media) on a gyratory shaker at 225 rpm (250 rpm for P. fluorescens). Anaerobic cultures of Z. mobilis were grown at 30°C in 125-ml sealed glass flasks with 50 ml of minimal medium on magnetic stirrers at 225 rpm. The sterile medium was gassed with sterilely filtered N₂ for 15 min.

The M9 minimal medium contained, per liter of deionized water, 7.52 g of Na₂HPO₄ · 2H₂O, 3.0 g of KH₂PO₄, 0.5 g of NaCl, and 2.5 g of (NH₄)₂SO₄. The following components (in indicated quantities per liter of final medium) were sterilized separately and then added: 1 ml of 0.1 M CaCl₂, 1 ml of 1 M MgSO₄, 0.6 ml of 100 mM FeCl₃, 2 ml of vitamin solution (filter sterilized), and 10 ml of M9 trace salts solution. The vitamin solution contained (per 50 ml) 25 mg each of biotin, cyanocobalamin, niacin, calcium pantothenate, pyridoxine HCl, and thiamine HCl. The M9 trace salts solution contained (per liter) 0.18 g of ZnSO₄ · 7H₂O, 0.12 g of CuCl₂ · 2H₂O, 0.12 g of MnSO₄ · H₂O, and 0.18 g of CoCl₂ · 6H₂O. For R. sphaeroides, we used a special trace salts solution that contained (per liter) 1.5 g of nitrilotriacetic acid, 3.0 g of MgSO₄ · 7H₂O, 0.5 g of MnSO₄ · H₂O, 1.0 g of NaCl, 0.1 g of FeSO₄ · 7H₂O, 0.1 g of CoCl₂ · 6H₂O, 0.135 g of CaCl₂ · 2H₂O, 0.1 g of ZnSO₄ · 7H₂O, 0.01 g of CuSO₄ · 5H₂O, 0.01 g of H₃BO₃, 0.01 g of Na₂MoO₄ · 2H₂O, 0.015 g of NiCl₂, and 0.02 g of Na₂SeO₃; the pH was adjusted to 6.5 with KOH.

The Z. mobilis minimal medium contained (per liter) 0.18 g of KH₂PO₄, 0.082 g of MgSO₄ · 7H₂O, 0.002 g of FeSO₄ · 7H₂O, 0.87 g of NH₄Cl, 0.142 g of trisodium citrate dihydrate, 10 g of potassium hydrogen phthalate, and 2 ml of the vitamin solution (filter sterilized) described above. The pH was adjusted to 5.8 with KOH. The Paracoccus versutus minimal medium was composed of two solutions that were mixed at a ratio of 1:10 after heat sterilization. Solution A contained (per 100 ml) 4.2 g of Na₂HPO₄ · 2 H₂O, 1.5 g of KH₂PO₄, and 1.0 g of NH₄Cl; the pH was adjusted to 9.0. Solution B contained (per liter) 0.1 g of MgSO₄ · 7 H₂O and 5.0 ml of trace metal solution; the pH was adjusted to 6.0 with KOH. The trace solution contained (per liter) 50.0 g of EDTA, 22.0 g of ZnSO₄ · 7 H₂O, 5.54 g of CaCl₂ · 2 H₂O, 5.06 g of MnCl₂ · 4 H₂O, 4.99 g of FeSO₄ · 7 H₂O, 1.10 g of MoNH₄ · 4 H₂O, 1.57 g of CuSO₄ · 5 H₂O, and 1.61 g of CoCl₂ · 6 H₂O.

In all experiments, sterile glucose was supplemented at a final concentration of 3 g of glucose/liter (4 g/liter for P. fluorescens and 10 g/liter for Z. mobilis). For ¹³C-labeling experiments, glucose was added either entirely in the form of the 1-¹³C-labeled isotope isomer (99% pure; Omicron Biochemicals, Inc., South Bend, Ind.) or in the form of a mixture of 20% (wt/wt) [U-¹³C]glucose (>99% pure; Martek Biosciences Corporation, Columbia, Md.) and 80% (wt/wt) natural glucose. To elucidate the influence of unlabeled CO₂ on the ¹³C-labeling patterns of Z. mobilis, cultures were continuously flushed with filter-sterilized technical CO₂ through an inlet-and-outlet needle.

Analytical procedures and physiological parameters. Cell growth was monitored by measuring the optical density at 600 nm (OD₆₀₀). Glucose and acetate concentrations were determined enzymatically with commercially available kits (Beckman, Enzytec, and Boehringer Mannheim). Ethanol concentrations were quantified by GC in a Hewlett Packard 5890 Series II Plus chromatograph with a Macherey-Nagel fused-silica capillary column (model CW20M-0.25, 25-m length, 0.25-mm inside diameter; Permabond) with butyrate as the internal standard. Organic acids in culture supernatants were detected by high-pressure liquid chromatography analysis (Perkin Elmer) at a wavelength of 210 nm, using a Supelcogel C₈ column (4.6 by 250 mm) and 0.2% (vol/vol) sulfuric acid as the mobile phase at a flow rate of 0.3 ml/min at 30°C. The following physiological parameters were determined by regression analysis during the exponential growth phase in the batch culture, as described previously (41): maximum specific growth rate, biomass yield on glucose, specific glucose consumption, and by-product formation rates. Cellular dry weight (CDW) was inferred from OD₆₀₀ measurements with a predetermined correlation factor, k. To determine k, CDW was determined from at least four parallel 2-ml cell suspensions that were harvested by centrifugation at 15,800 x g in an Eppendorf tabletop centrifuge using predried and weighed 2-ml Eppendorf cups. The pellets were washed with 0.9% NaCl and dried at 105°C for 24 h to a constant weight.

For P. fluorescens, the theoretical extracellular pool concentration of gluconate-2-ketogluconate, f, was calculated from the integrated product of the specific growth rate, µ_max, and the gluconate-2-ketogluconate accumulation rate, c, as follows:

where m was a coefficient, c was the glucose decrease rate minus the total carbon uptake rate (see Results), and t was the time in hours for growth on glucose.

Sample preparation and GC-MS analysis. Cell aliquots were harvested during mid-exponential growth by centrifuging 35 to 40 ml of culture broth at 1,200 x g and 4°C for 20 min. The pellet was washed twice with 1 ml of 0.9% NaCl, hydrolyzed in 1.5 ml of 6 M HCl for 24 h at 110°C in sealed 2-ml Eppendorf tubes, and desiccated overnight in a heating block at 85°C under a constant air stream. The hydrolyzate was dissolved in 50 µl of 99.8% pure dimethyl formamide and transferred into a new Eppendorf cup within a few seconds. For derivatization, 30 µl of N-methyl-N-(tert-butyldimethylsilyl)-trifluoroacetamide, which readily silylates hydroxyl groups, thiols, primary amines, amides, and carboxyl groups, (7) was added, and the mixture was incubated at 85°C with shaking at 550 rpm for 60 min. One microliter of the derivatized sample was injected into a series 8000 GC combined with a model MD 800 mass spectrometer (Fisons Instruments) and analyzed as described previously (7, 16).

Metabolic-flux ratio analysis. For METAFoR analysis, mass spectra of the derivatized amino acids alanine, glycine, valine, leucine, isoleucine, proline, serine, threonine, phenylalanine, aspartate, glutamate, histidine, and tyrosine were corrected for the natural abundance of all stable isotopes and unlabeled biomass from the inoculum. Lysine and methionine are not required for the METAFoR analysis used in this study, whereas arginine, asparagine, cysteine, glutamine, and tryptophane are not detectable. The amino acids are synthesized from one or more metabolic intermediates, and the mass isotopomer distribution vectors (MDV) of these metabolites could easily be derived from the MDV of the amino acids (16). The metabolite MDV were then used to calculate the fractional contribution of a given pathway or reaction to a target metabolite pool (metabolic-flux ratios) by using sets of algebraic equations implemented in the MATLAB-based program Fiat Flux version 1.04 as described previously (16). The result is direct and quantitative evidence for strictly local ratios of two or more reactions and pathways to a metabolic intermediate.

Net-flux analysis and master reaction network. The metabolic models used for net-flux analysis were based on the master reaction network, which included 45 reactions and 33 metabolites and is shown in Fig. 1. Respiration, biomass formation, and a transhydrogenase reaction were included as additional reactions, and ATP and the cofactors NADH and NADPH were included as additional metabolites. Net fluxes were then calculated using (i) the stoichiometric reaction matrix, (ii) the METAFoR analysis-derived flux ratios, (iii) physiological data, and (iv) precursor requirements for biomass synthesis, as described previously (18). Specifically, the following flux ratios were used: serine derived through the EMP pathway, pyruvate derived through the ED pathway, oxaloacetate (OAA) originating from phosphoenolpyruvate (PEP) or pyruvate, PEP originating from OAA, the lower and upper bounds of pyruvate originating from malate, and the upper bound of PEP derived through the PP pathway. For the particular stoichiometric matrix of each organism, several reactions were omitted from the master network based on information from the ¹³C-labeling experiments and literature knowledge (see below). The stoichiometric matrix was then solved with the MATLAB-based program Netto version 1.04 (18) by minimizing the sum of the weighted square residuals of the constraints from both metabolite balances and flux ratios to obtain estimated net fluxes.

View larger version (35K): [in this window] [in a new window]

FIG. 1. Master reaction network that was used as the basis for net-flux analysis. Metabolites in bold were precursors for amino acid biosynthesis, and metabolites in boxes were extracellular substrates or products. Doubled-headed arrows indicate reactions assumed to be reversible. Abbreviations: S7P, sedoheptulose-7-P; Acetyl-CoA, acetyl coenzyme A.

Biomass requirements and organism-specific networks. E. coli and B. subtilis were routinely analyzed as control experiments using the previously established growth rate-dependent biomass requirements and network models (8, 15). For gram-negative P. fluorescens, P. putida, S. meliloti, A. tumefaciens, and R. sphaeroides, the biomass requirements were assumed to be similar to that of E. coli (15), and for the gram-positive organism Paracoccus versutus, the requirements were taken from the B. subtilis model (8). For Z. mobilis, the precursor requirements were based on the published biomass composition (10).

The metabolic network used for Z. mobilis lacks a functional EMP pathway due to the absence of the key enzyme phosphofructokinase. Furthermore, the tricarboxylic acid (TCA) cycle is incomplete and does not contain a transaldolase; thus, pentoses are synthesized from fructose-6-P and glyceraldehyde-3-P via the reversible transketolase (10, 32, 33). The resulting network of Z. mobilis included the following reactions in Fig. 1: 1 to 3, 6 to 14, 16 to 18, 21 to 23, 30, and 31. The network model for P. fluorescens and P. putida was adapted from previous literature (28, 46). Besides the direct uptake, glucose may also be converted extracellularly to gluconate and 2-ketogluconate, both of which can be taken up by the cell. Additionally, the EMP pathway is absent due to the lack of phosphofructokinase. Thus, the network of both pseudomonads included the following reactions: 1 to 3, 5 to 22, 24, 25, 37, and 39 to 42. Reaction 5 principally enables a cyclic flux through the ED pathway that could not be resolved by the present ¹³C-labeling experiments; nevertheless, a weak flux was obtained through reaction 5 in P. putida (see Table S1 in the supplemental material). The network models for A. tumefaciens and S. meliloti were basically the same as that for P. fluorescens (1, 12, 21, 25, 36). Since we did not detect gluconate or 2-ketogluconate accumulation, however, glucose uptake was assumed to be direct in both organisms. Thus, the networks consisted of the reactions 1 to 3, 5 to 22, 24, and 25. The network models for the metabolically versatile organisms R. sphaeroides (5, 6, 23, 52) and Paracoccus versutus (51) included the reactions 1 to 4, 6 to 22, 24, and 25.

Top Abstract Introduction Materials and Methods Results Discussion References

 
Network identification and flux analysis. To experimentally identify metabolic networks of active reactions, we used ¹³C-constrained metabolic-flux analysis that relies on the detection of mass isotopomer pattern in proteinogenic amino acids (16, 18). Since pathways of amino acid biosynthesis may differ among species, we first verified the biosynthetic routes. For each amino acid, the labeling pattern depended on that of the precursor from which it was synthesized; for example, the alanine carbon skeleton is derived from pyruvate. Since valine and leucine are typically synthesized also from pyruvate, the redundant information in all three amino acids must be the same if they are indeed synthesized from pyruvate. Generally, all detected labeling patterns were consistent with the amino acid biosynthesis pathways of E. coli (44), and no discrepancies were detected within the labeling patterns of the redundant amino acids.

Based on the established amino acid biosynthesis schemes, we then calculated intracellular-flux ratios from the labeling patterns of the amino acids by using the algebraic equations of METAFoR analysis (16). These flux ratios represent direct, local evidence for the in vivo activity of particular pathways and reactions. From the thus-elucidated network topology of active reactions and from literature data, organism-specific metabolic-reaction models were deduced from the master network model (Fig. 1). Absolute net fluxes were then calculated with these network models from the physiological data (Table 1) and the flux ratios (Table 2) (18, 40). Since the analytically determined flux ratios constrain the ratios of at least two fluxes within their margins of experimental error, this approach is referred to as ¹³C-constrained flux analysis.

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

TABLE 1. Growth physiologya

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

TABLE 2. Metabolic flux ratios obtained by METAFoR analysis of experiments with 100% [1-13C]glucose, 20% [U-13C]glucose, and 80% naturally labeled glucosea

Z. mobilis. Without a respiratory chain, Z. mobilis is an obligate fermenter and produces a single ATP molecule per molecule of metabolized glucose. This energetically ineffective metabolism leads to very high fermentative fluxes with a very low biomass yield of 20 mg of cells per g of glucose (11). Among the species investigated here, the glucose uptake rate of Z. mobilis was at least an order of magnitude higher than those of most others (Fig. 2A; Table 1). This flux was exclusively catalyzed by the ED pathway (Fig. 2A; Table 2), the enzymes of which constitute up to 50% of a cell's total protein (42). The absence of the EMP pathway was confirmed by [1-¹³C]glucose experiments, where no ¹³C label was detected at the C-3 position of pyruvate, due to the missing phosphofructokinase (data not shown). The absence of transaldolase (10) was also verified from the pentose-labeling patterns found in the 20% [U-¹³C]glucose experiment, which were consistent with those expected when only transketolase B is active (Table 3).

View larger version (43K): [in this window] [in a new window]

FIG. 2. In vivo carbon flux distribution in Z. mobilis (A), P. fluorescens (B), S. meliloti (C), and A. tumefaciens (D). All fluxes were normalized to the glucose uptake rate that is given at the top of each panel, and the widths of the arrows are scaled to the relative percentages of flux. Fluxes below 2.6% of the glucose uptake rate are represented by nonscaled hairlines. Possible cyclic fluxes through the ED pathways of P. fluorescens and S. meliloti are not resolved by the data and are not shown. Generally, the 95% confidence intervals were between 5 and 10% for the major fluxes. Larger confidence intervals were estimated for reactions with low flux. Abbreviations: G6P, glucose-6-P; 6PG, 6-P-gluconate; F6P, fructose-6-P; P5P, pentose-5-P; E4P, erythrose-4-P; S7P, sedoheptulose-7-P; G3P, glyceraldehyde-3-P; OGA, 2-ketoglutarate; PPP, PP pathway; Acetyl-CoA, acetyl coenzyme A.

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

TABLE 3. Mass isotopomer distribution in pentose-5-P in Z. mobilisa

Although the EMP pathway was inactive, a ¹³C label was detected at the C-3 position of serine from 100% [1-¹³C]glucose experiments (Table 4). Thus, labeled carbon must have been introduced through C₁ metabolism (Fig. 3). The tetrahydrofolyl (THF) cycle is replenished with C₁ that originates from formate, which in turn is generated from pyruvate via pyruvate formate lyase or from CO₂ via formate dehydrogenase. To differentiate between the two routes, we (i) added formate to strongly reduce the fraction of labeled formate in the medium and (ii) continuously gassed the culture with unlabeled CO₂, which should have diluted the serine label if the formate dehydrogenase were active. Although noticeable, the influence of unlabeled CO₂ on the m₁ mass fraction signal of serine was far less significant than the effect of adding formate (Table 4). This finding indicates that pyruvate formate lyase rather than formate dehydrogenase generates the formate in Z. mobilis that leads to the labeling of C-3 of serine.

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

TABLE 4. Mass isotopomer distribution of serine in Z. mobilis at different formate concentrations

View larger version (23K): [in this window] [in a new window]

FIG. 3. Possible reactions that introduce C1 fragments into serine, methionine, and histidine (31). Abbreviations: AICAR-P, 5-aminoimidazole-4-carboxamide-1-ribotide; THFPG, tetrahydrofolylpolyglutamate; 10-Fo-THF, 10-formyl-tetrahydrofolyl; 5,10-Me-THF, 5,10-methyl-tetrahydrofolyl; 3PG, 3-P-glycerate; AcCoA, acetyl coenzyme A.

Pseudomonads. In P. fluorescens, but not in P. putida, extracellular glucose was converted to gluconate and 2-ketogluconate, which were subsequently consumed during the later growth phase (Fig. 4), as described previously (13, 28, 45). Considering the simplified glucose uptake scheme shown in Fig. 5, the total gluconate-2-ketogluconate accumulation rate, c, during growth on glucose was calculated as 15.21 mmol g^–1 h^–1 from the experimentally determined extracellular glucose decrease rate (a = 19.75 mmol g^–1 h^–1) minus the total carbon uptake rate (b = 4.54 mmol g^–1 h^–1). The experimentally determined extracellular concentration of gluconate and 2-ketogluconate was consistent with that calculated with the above equation, which strongly suggests that there was no cocatabolism of gluconate-2-ketogluconate during growth on glucose. Upon glucose depletion, the carbon uptake rate from both gluconate and 2-ketogluconate almost doubled to 9.42 mmol g^–1 h^–1. Based on the above conclusions, the total carbon uptake rate for net-flux analysis was assumed to be exclusively from glucose in the first phase and from gluconate-2-ketogluconate (g) in the second phase. The relative proportion of gluconate and 2-ketogluconate uptake could not be resolved, because the carbon skeleton remained unchanged, which led to identical labeling patterns.

View larger version (21K): [in this window] [in a new window]

FIG. 4. Time courses of OD600 (squares) and concentrations of extracellular glucose (circles), gluconate (triangles), and 2-ketogluconate (diamonds) in P. fluorescens.

View larger version (20K): [in this window] [in a new window]

FIG. 5. Glucose uptake in P. fluorescens. The following fluxes (shown by arrows) are involved in glucose uptake: direct glucose uptake (r1), membrane-bound glucose dehydrogenase (r2), gluconate dehydrogenase (r3), uptake of gluconate (r4), and 2-ketogluconate (r5). The experimentally determined extracellular glucose decrease rate, a, is defined as r1 plus r2; the total carbon uptake rate by the cell, b, is defined as r1 plus r4 plus r5; and the total gluconate-2-ketogluconate uptake rate, g, is defined as r4 plus r5.

During growth on glucose, P. fluorescens secreted very little in the way of metabolic by-products (Table 1), and the ED pathway and the TCA cycle were the almost exclusive catabolic pathways prior to (Fig. 2B; Table 2) and after (data not shown) glucose depletion. Unlike those in most other bacteria, however, the TCA cycle did not operate via malate dehydrogenase but mostly via the so-called pyruvate shunt, which is catalyzed by malic enzyme and pyruvate carboxylase (from malate to pyruvate to OAA). Moreover, a relatively high gluconeogenic flux of 17% through the PEP carboxykinase was detected. The higher carbon uptake rate of 9.42 mmol g^–1 h^–1 during the second growth phase resulted in a higher TCA cycle flux and a decreased biomass yield of 0.29, compared to a yield of 0.44 (CDW in grams per gram of glucose) produced during growth on glucose.

In P. putida, very little gluconate or 2-ketogluconate accumulated (below 2 mM); hence, carbon uptake was most likely via the direct glucose uptake route. Net-flux analysis with a lumped total carbon uptake resulted in a distribution that was very similar to that of P. fluorescens (data not shown).

Rhizobiaceae. As a fast-growing rhizobium with a generation time of less than 6 h on complex medium, S. meliloti was reported to be able to convert glucose to gluconate, which then enters metabolism (36, 43). Since <1 mM gluconate accumulated and the labeling data did not allow the resolution of the different uptake routes, both were lumped for net-flux analysis. In S. meliloti, pyruvate carboxylase was assumed to be the anaplerotic reaction by analogy to A. tumefaciens (12). Both the PP and ED pathways were reported to be present, and glycolysis was reported to be absent, in both rhizobia (1, 43), which was confirmed by METAFoR analysis (Table 2). In both rhizobia, the ED pathway was basically the exclusive pathway of glucose degradation, while the pentose-5-P precursors for biomass were generated through the oxidative and nonoxidative branches of the PP pathway (Fig. 2C and D). With a flux well above 100% relative to the glucose uptake rate, both species exhibited higher TCA cycle fluxes than those of most species investigated here (Fig. 2C and D).

Paracoccus versutus. As a member of the genus Paracoccus, Paracoccus versutus (synonyms, Thiobacillus versutus and Paracoccus strain A2) belongs to the group of -proteobacteria and is closely related to the Rhodobacteraceae and distantly to pseudomonads (2). As a facultative autotroph, Paracoccus versutus is capable of heterotrophic growth on a wide rage of organic substrates that include mono-, di-, and trisaccharides (49). Extensive radiorespirometric and enzymatic analyses of the main carbon-degrading pathways indicated the presence of the EMP, ED, and PP pathways (49-51). Consistent with the reported adaptation to growth solely on glucose, the specific rate of growth increased from 0.29 to 0.70 h^–1 (Table 1). In the rapidly growing culture, METAFoR analysis revealed an inactive EMP pathway, some PP pathway activity, and predominant catabolic flux through the ED pathway (Table 2). Since Paracoccus versutus exhibited the highest aerobic glucose uptake rate of all species investigated, it was surprising that its metabolism was fully respirative, with very high TCA cycle flux (Fig. 6A).

View larger version (44K): [in this window] [in a new window]

FIG. 6. In vivo carbon flux distribution in Paracoccus versutus (A), R. sphaeroides (B), E. coli (C), and B. subtilis (D). All fluxes were normalized to the glucose uptake rates that are given at the top of each panel, and the widths of the arrows are scaled to the relative fluxes, expressed as percentages of the glucose uptake rates. Fluxes below 2.6% are represented by nonscaled hairlines. Generally, the 95% confidence intervals were between 5 and 10% for the major fluxes. Larger confidence intervals were estimated for reactions with low flux. Abbreviations: G6P, glucose-6-P; 6PG, 6-P-gluconate; F6P, fructose-6-P; FBP, fructose-1,6-bisphosphate; P5P, pentose-5-P; G3P, glyceraldehyde-3-P; OGA, 2-ketoglutarate; PPP, PP pathway; Acetyl-CoA, acetyl coenzyme A.

R. sphaeroides. The purple, facultatively photosynthetic bacterium R. sphaeroides has an unusually versatile metabolism, capable of aerobic chemoheterotrophic and anaerobic photoheterotrophic growth (27). Aerobic growth on glucose, however, was rather slow (Table 1). While the EMP and ED pathways were reported to be present (4, 5), only the ED pathway was active during aerobic growth on glucose (Table 1; Fig. 6B). The m₁ mass fractions of pyruvate fragments 1 to 3 and 2 to 3 (52 and 2%, respectively; detected in alanine, isoleucine, leucine, lysine, and valine) directly demonstrated exclusive use of the ED pathway, whereas the almost completely unlabeled PEP (detected in phenylalanine, tryptophane, and tyrosine) verified the absence of EMP pathway flux (data not shown). In a manner akin to that of most previously analyzed bacteria, glucose was catabolized almost exclusively via the ED pathway and the TCA cycle, with slight by-product formation but some contribution on the part of the pyruvate shunt via malic enzyme and pyruvate carboxylase (Fig. 6B). The PP pathway operated exclusively to provide precursors for biosynthesis, and the EMP pathway catalyzed even small gluconeogenic fluxes from glyceraldehyde-3-P to fructose-6-P.

E. coli and B. subtilis. In sharp contrast to all other bacteria analyzed here, the gram-positive and gram-negative model bacteria E. coli and B. subtilis rely primarily on the EMP pathway for glucose catabolism (Fig. 6C and D). Moreover, the relative TCA cycle flux was much lower than that in the other species because secretion of the incompletely oxidized overflow product acetate was extensive. At 38%, the PP pathway flux in B. subtilis was the highest observed in all species (Table 5). Generally, the overall estimated flux distribution in both species was similar to that obtained previously from 37°C batch cultures, except for the elevated TCA cycle activity in E. coli at 30°C and the elevated anaplerosis (OAA from pyruvate) in B. subtilis at 30°C, which was due to lower relative acetate formation (39, 53). Apart from the about 30- to 50%-lower growth rates, there were only minor changes that are related to the lower overall rate of metabolism at 30°C, the temperature used here.

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

TABLE 5. Relative molecular carbon flow into the PP pathway and catabolic PP pathway flux

Top Abstract Introduction Materials and Methods Results Discussion References

 
In all seven newly investigated species, the ED pathway was the almost exclusive route of glucose catabolism, while the EMP pathway was mostly absent and the PP pathway served exclusively biosynthetic functions. Although the ED pathway is widely distributed (6, 26) and is probably the oldest catabolic pathway (37), its predominance was unexpected for species capable of all three routes of glucose catabolism, such as Paracoccus versutus (49) and R. sphaeroides (5). The generally held view that the EMP pathway is the major route of glucose catabolism may thus be a misconception, because most quantitative metabolic studies were done with the model microbes E. coli, B. subtilis, C. glutamicum, and S. cerevisiae, which exhibit unusually high glycolytic fluxes.

Beyond the ED pathway, the flux data presented here reveal a number of additional abnormalities in the glucose catabolism of the more frequently investigated model bacteria. First, all nonmodel species used the PP pathway exclusively for biosynthesis of biomass precursors, and in many cases the flux to the building blocks was through both the oxidative and the nonoxidative branches of the pathway (Table 5). In sharp contrast, the E. coli and B. subtilis PP pathway flux contributed substantially to catabolism (12 and 27%, respectively), which is consistent with the results of previous analyses (39, 53) and also true for C. glutamicum (48). Second, the E. coli and B. subtilis TCA cycle flux was relatively low, metabolism was not fully respiratory, and there was extensive overflow metabolism that is also referred to as aerobic fermentation. None of the aerobic species investigated here exhibited this phenomenon to a significant extent, which is particularly surprising for species such as Paracoccus versutus that exhibit much higher catabolic rates than do the model microbes. Thus, it is not unreasonable to speculate that overflow metabolism is not a typical microbial trait but rather an adaptation to industrial or laboratory conditions. The most prominent example is baker's yeast, which has been cultivated and selected over millennia by mankind and strongly increases its rate of aerobic fermentation at high growth rates (3). Third, all aerobic nonmodel species routed between 29 and 35% of their carbon flux through the so-called pyruvate shunt, which bypasses malate dehydrogenase. In the case of P. fluorescens, the pyruvate shunt was the predominant route of malate-to-OAA conversion. Although B. subtilis was reported to use the pyruvate bypass under glucose limitation (40), its activity is very low in glucose batch cultures (Fig. 6D) (53).

In addition to the linear ED pathway, which may be inducible in E. coli during growth on gluconate or constitutive, as it is in Z. mobilis, cyclic operation of the ED pathway was reported for organisms that lack phosphofructokinase, e.g., pseudomonads (28) and S. meliloti (25). In the absence of both phosphofructokinase and fructose-1,6-P aldolase, A. tumefaciens cannot operate a cyclic ED pathway but may alternatively use a cyclic PP pathway (1). Cyclic operation of either pathway is known from studies of members of the phylum Proteobacteria such as Acetobacter, Agrobacterium, Azotobacter, Pseudomonas, Rhizobium, Paracoccus, and Xanthomonas spp., which preferentially utilize organic acids rather than sugars and secrete exopolysaccharides (35). The cyclic pathway operation may facilitate the formation of the polysaccharide precursor fructose-6-P in cases where the EMP pathway is absent (21). The extent to which glyceraldehyde-3-P is recycled into the ED pathway is unclear from the present data and may vary between species. However, an increased demand for fructose-6-P and also glucose-6-P due to (exo)polysaccharide synthesis was assumed to be negligible under non-nitrogen-limited batch culture conditions (20, 35, 54).

Ideally, identification of reaction networks and quantification of metabolic fluxes is based on annotated genome data, a large body of biochemical data, and comprehensive tracer experiments. Here we demonstrate that important quantitative information can also be inferred from a much smaller data basis than is typically available for model microbes by using well-designed ¹³C experiments. Besides the above quantification of the different catabolic routes in each species, several new findings were made. Although the overall glucose flux was, of course, from hexoses to trioses, low but significant gluconeogenic flux occurred in R. sphaeroides and Paracoccus versutus from glyceraldehyde-3-P to glucose-6-P. These two were also the only species where pentose phosphates were mostly synthesized via the nonoxidative branch of the PP pathway, despite high catabolic fluxes passing through the other possible precursor, 6-P-gluconate. During the first growth phase, P. fluorescens converts a major fraction of glucose extracellularly to gluconate and 2-ketogluconate, which are metabolized during the later growth phases; this conversion is in contrast with the physiological data that suggested direct utilization of glucose (29). In Z. mobilis, C₁ metabolism introduces a significant fraction of (¹³C-labeled) pyruvate formate lyase-derived formate into serine. Such experimental identification of metabolic networks and quantification of in vivo molecular fluxes by ¹³C tracer experiments has great potential for application in novel or not-yet-characterized species.

 
* Corresponding author. Mailing address: Institute of Biotechnology, ETH Zürich, CH-8093 Zürich, Switzerland. Phone: 41-1-633 3672. Fax: 41-1-633 1051. E-mail: sauer{at}biotech.biol.ethz.ch.

Supplemental material for this article may be found at http://jb.asm.org/.

Top Abstract Introduction Materials and Methods Results Discussion References

 

1
1. Arthur, L. O., L. A. Bulla, Jr., G. St. Julian, and L. K. Nakamura. 1973. Carbohydrate metabolism in Agrobacterium tumefaciens. J. Bacteriol. 116:304-313.[Abstract/Free Full Text]
2
2. Baker, S. C., S. J. Ferguson, B. Ludwig, M. D. Page, O.-M. Richter, and R. J. M. van Spanning. 1998. Molecular genetics of the genus Paracoccus: metabolically versatile bacteria with bioenergetic flexibility. Microbiol. Mol. Biol. Rev. 62:1046-1078.[Abstract/Free Full Text]
3
3. Blank, L. M., and U. Sauer. 2004. TCA cycle activity in Saccharomyces cerevisiae is a function of the environmentally determined specific growth and glucose uptake rates. Microbiology 150:1085-1093.[Abstract/Free Full Text]
4
4. Conrad, R., and H. G. Schlegel. 1977. Different degradation pathways for glucose and fructose in Rhodopseudomonas capsulata. Arch. Microbiol. 112:39-48.[CrossRef][Medline]
5
5. Conrad, R., and H. G. Schlegel. 1977. Influence of aerobic and phototrophic growth conditions on the distribution of glucose and fructose carbon into the Entner-Doudoroff and Embden-Meyerhof pathways in Rhodopseudomonas sphaeroides. J. Gen. Microbiol. 101:277-290.
6
6. Conway, T. 1992. The Entner-Doudoroff pathway: history, physiology and molecular biology. FEMS Microbiol. Rev. 9:1-27.[Medline]
7
7. Dauner, M., and U. Sauer. 2000. GC-MS analysis of amino acids rapidly provides rich information for isotopomer balancing. Biotechnol. Prog. 16:642-649.[CrossRef][Medline]
8
8. Dauner, M., and U. Sauer. 2001. Stoichiometric growth model for riboflavin-producing Bacillus subtilis. Biotechnol. Bioeng. 76:132-143.[CrossRef][Medline]
9
9. Dauner, M., T. Storni, and U. Sauer. 2001. Bacillus subtilis metabolism and energetics in carbon-limited and excess-carbon chemostat culture. J. Bacteriol. 183:7308-7317.[Abstract/Free Full Text]
10
10. De Graaf, A. A., K. Striegel, R. M. Wittig, B. Laufer, G. Schmitz, W. Wiechert, G. A. Sprenger, and H. Sahm. 1999. Metabolic state of Zymomonas mobilis in glucose-, fructose-, and xylose-fed continuous cultures as analysed by ¹³C- and ³¹P-NMR spectroscopy. Arch. Microbiol. 171:371-385.[CrossRef][Medline]
11
11. Doelle, H. W., L. Kirk, R. Crittenden, H. Toh, and M. B. Doelle. 1993. Zymomonas mobilis—science and industrial application. Crit. Rev. Biotechnol. 13:57-98.[Medline]
12
12. Dunn, M. F., G. Araiza, and T. M. Finan. 2001. Cloning and characterization of the pyruvate carboxylase from Sinorhizobium meliloti Rm1021. Arch. Microbiol. 176:355-363.[CrossRef][Medline]
13
13. Eisenberg, R. C., S. J. Butters, S. C. Quay, and S. B. Friedman. 1974. Glucose uptake and phosphorylation in Pseudomonas fluorescens. J. Bacteriol. 120:147-153.[Abstract/Free Full Text]
14
14. Eisenberg, R. C., and W. J. Dobrogosz. 1967. Gluconate metabolism in Escherichia coli. J. Bacteriol. 93:941-949.[Abstract/Free Full Text]
15
15. Emmerling, M., M. Dauner, A. Ponti, J. Fiaux, M. Hochuli, T. Szyperski, K. Wüthrich, J. E. Bailey, and U. Sauer. 2002. Metabolic flux responses to pyruvate kinase knockout in Escherichia coli. J. Bacteriol. 184:152-164.[Abstract/Free Full Text]
16
16. Fischer, E., and U. Sauer. 2003. Metabolic flux profiling of Escherichia coli mutants in central carbon metabolism using GC-MS. Eur. J. Biochem. 270:880-891.
17
17. Fischer, E., and U. Sauer. 2003. A novel metabolic cycle catalyzes glucose oxidation and anaplerosis in hungry Escherichia coli. J. Biol. Chem. 278:46446-46451.[Abstract/Free Full Text]
18
18. Fischer, E., N. Zamboni, and U. Sauer. 2004. High-throughput metabolic flux analysis based on gas chromatography-mass spectrometry derived ¹³C constraints. Anal. Biochem. 325:308-316.[CrossRef][Medline]
19
19. Gombert, A. K., M. Moreira dos Santos, B. Christensen, and J. Nielsen. 2001. Network identification and flux quantification in the central metabolism of Saccharomyces cerevisiae under different conditions of glucose repression. J. Bacteriol. 183:1441-1451.[Abstract/Free Full Text]
20
20. Gonzalez, J. E., G. M. York, and G. C. Walker. 1996. Rhizobium meliloti exopolysaccharides: synthesis and symbiotic function. Gene 179:141-146.[CrossRef][Medline]
21
21. Gosselin, I., O. Wattraint, D. Riboul, J. Barbotin, and J. Portais. 2001. A deeper investigation on carbohydrate cycling in Sinorhizobium meliloti. FEBS Lett. 499:45-49.[CrossRef][Medline]
22
22. Gunnarsson, N., U. H. Mortensen, M. Sosio, and J. Nielsen. 2004. Identification of the Entner-Doudoroff pathway in an antibiotic-producing actinomycete species. Mol. Microbiol. 52:895-902.[CrossRef][Medline]
23
23. Hickman, J. W., R. D. Barber, E. P. Skaar, and T. J. Donohue. 2002. Link between the membrane-bound pyridine nucleotide transhydrogenase and glutathione-dependent processes in Rhodobacter sphaeroides. J. Bacteriol. 184:400-409.[Abstract/Free Full Text]
24
24. Hua, Q., C. Yang, T. Baba, H. Mori, and K. Shimizu. 2003. Responses of the central metabolism in Escherichia coli to phosphoglucose isomerase and glucose-6-phosphate dehydrogenase knockouts. J. Bacteriol. 185:7053-7067.[Abstract/Free Full Text]
25
25. Irigoyen, J. J., M. Sanchez-Diaz, and D. W. Emerich. 1990. Carbon metabolism enzymes of Rhizobium meliloti cultures and bacteroids and their distribution within alfalfa nodules. Appl. Environ. Microbiol. 56:2587-2589.[Abstract/Free Full Text]
26
26. Kersters, K., and J. De Ley. 1968. The occurrence of the Entner-Doudoroff pathway in bacteria. Antonie Leeuwenhoek 34:393-408.
27
27. Klamt, S., S. Schuster, and E. D. Gilles. 2002. Calculability analysis in underdetermined metabolic networks illustrated by a model of the central metabolism in purple nonsulfur bacteria. Biotechnol. Bioeng. 77:734-751.[CrossRef][Medline]
28
28. Lessie, T. G., and P. V. Phibbs, Jr. 1984. Alternative pathways of carbohydrate utilization in pseudomonads. Annu. Rev. Microbiol. 38:359-388.[CrossRef][Medline]
29
29. Lynch, W. H., and M. Franklin. 1978. Effect of temperature on uptake of glucose, gluconate, and 2-ketogluconate by Pseudomonas fluorescens. Can. J. Microbiol. 24:56-62.[Medline]
30
30. Marx, A., A. A. deGraaf, W. Wiechert, L. Eggeling, and H. Sahm. 1996. Determination of the fluxes in the central metabolism of Corynebacterium glutamicum by nuclear magnetic resonance spectroscopy combined with metabolite balancing. Biotechnol. Bioeng. 49:111-129.[CrossRef]
31
31. Michal, G. 1999. Biochemical pathways. Spektrum Akademischer Verlag GmbH, Heidelberg, Germany.
32
32. Nipkow, A., B. Sonnleitner, and A. Fiechter. 1985. Effect of carbon-dioxide on growth of Zymomonas mobilis in continuous culture. Appl. Microbiol. Biotechnol. 21:287-291.
33
33. Osman, Y. A., T. Conway, S. J. Bonetti, and L. O. Ingram. 1987. Glycolytic flux in Zymomonas mobilis: enzyme and metabolite levels during batch fermentation. J. Bacteriol. 169:3726-3736.[Abstract/Free Full Text]
34
34. Petersen, S., A. A. de Graaf, L. Eggeling, M. Mollney, W. Wiechert, and H. Sahm. 2000. In vivo quantification of parallel and bidirectional fluxes in the anaplerosis of Corynebacterium glutamicum. J. Biol. Chem. 275:35932-35941.[Abstract/Free Full Text]
35
35. Portais, J. C., and A. M. Delort. 2002. Carbohydrate cycling in micro-organisms: what can (13)C-NMR tell us? FEMS Microbiol. Rev. 26:375-402.[Medline]
36
36. Portais, J. C., P. Tavernier, I. Gosselin, and J. N. Barbotin. 1999. Cyclic organization of the carbohydrate metabolism in Sinorhizobium meliloti. Eur. J. Biochem. 265:473-480.[Medline]
37
37. Romano, A. H., and T. Conway. 1996. Evolution of carbohydrate metabolic pathways. Res. Microbiol. 147:448-455.[Medline]
38
38. Sauer, U. 2004. High-throughput phenomics: experimental methods for mapping fluxomes. Curr. Opin. Biotechnol. 15:58-63.[CrossRef][Medline]
39
39. Sauer, U., F. Canonaco, S. Heri, A. Perrenoud, and E. Fischer. 2004. The soluble and membrane-bound transhydrogenases UdhA and PntAB have divergent functions in NADPH metabolism of Escherichia coli. J. Biol. Chem. 279:6613-6619.[Abstract/Free Full Text]
40
40. Sauer, U., V. Hatzimanikatis, J. E. Bailey, M. Hochuli, T. Szyperski, and K. Wüthrich. 1997. Metabolic fluxes in riboflavin-producing Bacillus subtilis. Nat. Biotechnol. 15:448-452.[CrossRef][Medline]
41
41. Sauer, U., D. R. Lasko, J. Fiaux, M. Hochuli, R. Glaser, T. Szyperski, K. Wüthrich, and J. E. Bailey. 1999. Metabolic flux ratio analysis of genetic and environmental modulations of Escherichia coli central carbon metabolism. J. Bacteriol. 181:6679-6688.[Abstract/Free Full Text]
42
42. Sprenger, G. A. 1996. Carbohydrate metabolism in Zymomonas mobilis: a catabolic highway with some scenic routes. FEMS Microbiol. Lett. 145:301-307.[CrossRef]
43
43. Stowers, M. D. 1985. Carbon metabolism in Rhizobium species. Annu. Rev. Microbiol. 39:89-108.[CrossRef][Medline]
44
44. Szyperski, T. 1995. Biosynthetically directed fractional ¹³C-labeling of proteinogenic amino acids. An efficient analytical tool to investigate intermediary metabolism. Eur. J. Biochem. 232:433-448.[Medline]
45
45. Temple, L. M., A. E. Sage, H. P. Schweizer, and P. V. Phibbs, Jr. 1998. Carbohydrate metabolism in Pseudomonas aeruginosa. Biotechnol. Handb. 10:35-72.
46
46. Vicente, M., and J. L. Cánovas. 1973. Glucolysis in Pseudomonas putida: physiological role of alternative routes from the analysis of defective mutants. J. Bacteriol. 116:908-914.[Abstract/Free Full Text]
47
47. Wiechert, W. 2001. ¹³C metabolic flux analysis. Metab. Eng. 3:195-206.[CrossRef][Medline]
48
48. Wittmann, C., and E. Heinzle. 2002. Genealogy profiling through strain improvement by using metabolic network analysis: metabolic flux genealogy of several generations of lysine-producing corynebacteria. Appl. Environ. Microbiol. 68:5843-5859.[Abstract/Free Full Text]
49
49. Wood, A. P., and D. P. Kelly. 1980. Carbohydrate degradation pathways in Thiobacillus A2 grown on various sugars. J. Gen. Microbiol. 120:333-345.
50
50. Wood, A. P., and D. P. Kelly. 1977. Heterotrophic growth of Thiobacillus A2 on sugars and organic acids. Arch. Microbiol. 113:257-264.[CrossRef][Medline]
51
51. Wood, A. P., D. P. Kelly, and C. F. Thurston. 1977. Simultaneous operation of three catabolic pathways in the metabolism of glucose by Thiobacillus A2. Arch. Microbiol. 113:265-274.[CrossRef][Medline]
52
52. Yakunin, A. F., and P. C. Hallenbeck. 1997. Regulation of synthesis of pyruvate carboxylase in the photosynthetic bacterium Rhodobacter capsulatus. J. Bacteriol. 179:1460-1468.[Abstract/Free Full Text]
53
53. Zamboni, N., and U. Sauer. 2003. Knockout of the high-coupling cytochrome aa₃ oxidase reduces TCA cycle fluxes in Bacillus subtilis. FEMS Microbiol. Lett. 226:121-126.[CrossRef][Medline]
54
54. Zevenhuizen, L. P. 1981. Cellular glycogen, beta-1,2,-glucan, poly beta-hydroxybutyric acid and extracellular polysaccharides in fast-growing species of rhizobium. Antonie Leeuwenhoek 47:481-497.

---

Journal of Bacteriology, March 2005, p. 1581-1590, Vol. 187, No. 5
0021-9193/05/$08.00+0     doi:10.1128/JB.187.5.1581-1590.2005
Copyright © 2005, American Society for Microbiology. All Rights Reserved.

This article has been cited by other articles:

• Ruhl, J., Schmid, A., Blank, L. M. (2009). Selected Pseudomonas putida Strains Able To Grow in the Presence of High Butanol Concentrations. Appl. Environ. Microbiol. 75: 4653-4656 [Abstract] [Full Text]  
• de Werra, P., Pechy-Tarr, M., Keel, C., Maurhofer, M. (2009). Role of Gluconic Acid Production in the Regulation of Biocontrol Traits of Pseudomonas fluorescens CHA0. Appl. Environ. Microbiol. 75: 4162-4174 [Abstract] [Full Text]  
• Fuhrer, T., Sauer, U. (2009). Different Biochemical Mechanisms Ensure Network-Wide Balancing of Reducing Equivalents in Microbial Metabolism. J. Bacteriol. 191: 2112-2121 [Abstract] [Full Text]  
• Meijnen, J.-P., de Winde, J. H., Ruijssenaars, H. J. (2008). Engineering Pseudomonas putida S12 for Efficient Utilization of D-Xylose and L-Arabinose. Appl. Environ. Microbiol. 74: 5031-5037 [Abstract] [Full Text]  
• Essington, M. E., Anderson, R. M. (2008). Competitive Adsorption of 2-Ketogluconate and Inorganic Ligands onto Gibbsite and Kaolinite. Soil Sci. 72: 595-604 [Abstract] [Full Text]  
• del Castillo, T., Ramos, J. L. (2007). Simultaneous Catabolite Repression between Glucose and Toluene Metabolism in Pseudomonas putida Is Channeled through Different Signaling Pathways. J. Bacteriol. 189: 6602-6610 [Abstract] [Full Text]  
• Price-Whelan, A., Dietrich, L. E. P., Newman, D. K. (2007). Pyocyanin Alters Redox Homeostasis and Carbon Flux through Central Metabolic Pathways in Pseudomonas aeruginosa PA14. J. Bacteriol. 189: 6372-6381 [Abstract] [Full Text]  
• del Castillo, T., Ramos, J. L., Rodriguez-Herva, J. J., Fuhrer, T., Sauer, U., Duque, E. (2007). Convergent Peripheral Pathways Catalyze Initial Glucose Catabolism in Pseudomonas putida: Genomic and Flux Analysis. J. Bacteriol. 189: 5142-5152 [Abstract] [Full Text]  
• Tang, Y. J., Chakraborty, R., Martin, H. G., Chu, J., Hazen, T. C., Keasling, J. D. (2007). Flux Analysis of Central Metabolic Pathways in Geobacter metallireducens during Reduction of Soluble Fe(III)-Nitrilotriacetic Acid. Appl. Environ. Microbiol. 73: 3859-3864 [Abstract] [Full Text]  
• Poysti, N. J., Oresnik, I. J. (2007). Characterization of Sinorhizobium meliloti Triose Phosphate Isomerase Genes. J. Bacteriol. 189: 3445-3451 [Abstract] [Full Text]  
• Tang, Y. J., Hwang, J. S., Wemmer, D. E., Keasling, J. D. (2007). Shewanella oneidensis MR-1 Fluxome under Various Oxygen Conditions. Appl. Environ. Microbiol. 73: 718-729 [Abstract] [Full Text]  
• Tang, Y. J., Meadows, A. L., Kirby, J., Keasling, J. D. (2007). Anaerobic Central Metabolic Pathways in Shewanella oneidensis MR-1 Reinterpreted in the Light of Isotopic Metabolite Labeling. J. Bacteriol. 189: 894-901 [Abstract] [Full Text]  
• Teusink, B., Wiersma, A., Molenaar, D., Francke, C., de Vos, W. M., Siezen, R. J., Smid, E. J. (2006). Analysis of Growth of Lactobacillus plantarum WCFS1 on a Complex Medium Using a Genome-scale Metabolic Model. J. Biol. Chem. 281: 40041-40048 [Abstract] [Full Text]  
• Fong, S. S., Nanchen, A., Palsson, B. O., Sauer, U. (2006). Latent Pathway Activation and Increased Pathway Capacity Enable Escherichia coli Adaptation to Loss of Key Metabolic Enzymes. J. Biol. Chem. 281: 8024-8033 [Abstract] [Full Text]  
• Eisenreich, W., Slaghuis, Jör., Laupitz, R., Bussemer, J., Stritzker, J., Schwarz, C., Schwarz, R., Dandekar, T., Goebel, W., Bacher, A. (2006). 13C isotopologue perturbation studies of Listeria monocytogenes carbon metabolism and its modulation by the virulence regulator PrfA. Proc. Natl. Acad. Sci. USA 103: 2040-2045 [Abstract] [Full Text]  
• Vertes, A. A., Inui, M., Yukawa, H. (2005). Manipulating Corynebacteria, from Individual Genes to Chromosomes. Appl. Environ. Microbiol. 71: 7633-7642 [Full Text]  
• Perrenoud, A., Sauer, U. (2005). Impact of Global Transcriptional Regulation by ArcA, ArcB, Cra, Crp, Cya, Fnr, and Mlc on Glucose Catabolism in Escherichia coli. J. Bacteriol. 187: 3171-3179 [Abstract] [Full Text]  

This Article Abstract Full Text (PDF) Supplemental material 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 Fuhrer, T. Articles by Sauer, U. Search for Related Content PubMed PubMed Citation Articles by Fuhrer, T. Articles by Sauer, U.