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Differential C Isotope Discrimination by Fungi during Decomposition of C₃- and C₄-Derived Sucrose

Matthew R. Henn and Ignacio H. Chapela^*

Ecosystem Sciences Division, Department of Environmental Science, Policy, and Management, University of California, Berkeley, California 94720-3110

Received 21 March 2000/Accepted 12 July 2000

	ABSTRACT

Top Abstract Introduction Materials and Methods Results and Discussion References

Stable isotope analysis is a major tool used in ecosystem studies to establish pathways and rates of C exchange between variousecosystem components. Little is known about isotopic effects ofmany such components, especially microbes. Here we report on thediscovery of an unexpected pattern of C isotopic discriminationby basidiomycete fungi with far-reaching consequences for ourunderstanding of isotopic processing in ecosystems where thesemicrobes mediate material transfers across trophic levels. Wemeasured fractionation effects on three ecologically relevantbasidiomycete species under controlled laboratory conditions.Sucrose derived from C₃ and C₄ plants is fractionated differentiallyby these microbes in a taxon-specific manner. The differentiationbetween mycorrhizal and saprotrophic fungi observed in the fieldby others is not explained by intrinsic discrimination patterns.Fractionation occurs during sugar uptake and is sensitive to thenonrandom distribution of stable isotopes in the sucrose molecule.The balance between respiratory physiology and fermentative physiologymodulates the degree of fractionation. These discoveries disprovethe assumption that fungal C processing does not significantlyalter the distribution of stable C isotopes and provide the basisfor a reevaluation of ecosystem models based on isotopic evidencethat involve C transfer across microbial interfaces. We providea mechanism to account for the observed differential discriminationeffects.

	INTRODUCTION

Top Abstract Introduction Materials and Methods Results and Discussion References

In the last decade, the analysis of stable C isotopes has emerged as a major tool to trace and quantify C transfers acrosstrophic levels in a variety of ecosystems (10, 21, 28).Two major premises concerning stable C isotopes in the environmentare frequently assumed. First, it is known that the mechanismof CO₂ uptake from the atmosphere and incorporation of CO₂ intoplant organic matter through photosynthesis result in characteristicisotopic ratios, which distinguish C₃ plants from C₄ plants (37).Second, it is frequently assumed that the effects of other biologicaltransformations on the natural distribution of stable C isotopesare relatively insignificant compared to the photosynthesis-determinedisotopic discrimination (17, 18, 41, 42). These two assumptionsare at the core of isotope-based models of ecosystem functionand global nutrientcycling.

While much refinement in knowledge has occurred with respect to photosynthetic pathways under various ecological conditions(11, 37), other equally important processes, such as decomposition,have remained mostly unexplored with respect to their isotopicdiscrimination effects, although they are critical for understandingecosystem C flows. Previous studies have shown that microbialmetabolic processes can be associated with characteristic fractionationpatterns at the subcellular scale (1, 7), but the discriminationeffects are often masked at the whole-organism level, resultingin the assumption that, overall, C isotopic discrimination dueto microbial processing is not significant (<1.0). Circumstantialevidence supporting this assumption is derived from the observationthat, in general, the isotopic ratios in ecosystem-respired CO₂roughly match those of the dominant vegetation (12, 13). Similarly,when ecosystems are transformed from C₃-dominant vegetation toC₄-dominant vegetation, the relative abundance of stable C isotopesin the soil is roughly maintained and is similar to that in theoriginal vegetation, suggesting that only minor changes due tomicrobial transformations occur (5, 43). Nevertheless, moredetailed measurements of C isotopic distributions have revealedpatterns that suggest that significant discrimination by microbesoccurs during soil formation; these patterns include the consistentenrichment of ¹³C often observed with increasing depth in soil profiles (34)and the relative enrichment observed in the CO₂ produced fromsoil respiration compared with canopy measurements (12, 13).

More directly, recent studies of fungi indicate that significant isotopic effects can be apparent when fungal tissues arecompared to their presumed plant substrates (20, 22, 24,25, 27, 44, 45), and a consistent difference in isotopicfractionation between mycorrhizal and saprotrophic basidiomyceteshas also been found in the field (22, 25, 27). Given theimportance of fungi in terrestrial ecosystems (15, 35, 40),the implications of isotopic discrimination associated with fungalC processing are of great consequence for isotope-based nutrientcycling models. The question remains as to whether fractionationpatterns observed in the field result from intrinsic fungal processingor are due to substrate effects (20, 44, 45).

In this work we documented intrinsically determined isotopic fractionation in fungi and studied the basis for a newly discoveredisotopic discrimination mechanism that is sensitive to differencesin C₃- and C₄-derived sugars during their catabolism. We concentratedon three basidiomycete species chosen for their contrasting fractionationpatterns and ecophysiological roles in pine-dominatedecosystems.

	MATERIALS AND METHODS

Top Abstract Introduction Materials and Methods Results and Discussion References

Cultures. Live mycelia were isolated from fresh fungal sporocarps of Cryptoporus volvatus (a wood decayer), Marasmius androsaceus (alitter decomposer), and Suillus granulatus (an ectomycorrhizalorganism) on solid modified Melin-Norkrans medium (MMN) (30).These three fungal species were chosen from a larger collectionof higher fungi associated with Monterey pines in California becauseof their relative importance in the ecosystems as well as theircontrasting ecological roles. Fewer than three subculturings wereperformed between the initial isolation from sporocarp tissuesand the experiments. Liquid MMN was further modified to make sucrosethe dominant C source (1.17% [wt/vol] sucrose, 0.13% [wt/vol]malt). A malt concentration of 0.13% (wt/vol) was experimentallydetermined to be the minimum concentration necessary for growthof the three fungal species (data not shown). Four sources ofsucrose were used: pure beet sucrose (98% pure as assayed by theBeet Sugar Foundation), impure maple sucrose (Andronico's Market),pure cane sucrose (C&H Sugar Company), and impure cane sucrose(Cumberland Packing Corporation). N was supplied as ammonium phosphate,and the medium was autoclaved for 15 min at 120°C. The initialmedium pH was 5.9 to 6.4. The growth vessels (open system) were125-ml Erlenmeyer flasks that contained 75 ml of MMN and werecapped with foam and aluminum foil. Two small mycelial plugs wereobtained from the edge of fast-growing colonies on solid mediumand used to inoculate liquid MMN vessels. The inoculum plugs were1 mm in diameter and contained less than 0.5 µg of C; thus, carryoverof C from stock cultures was minimized. Cultures were incubatedat 25°C on a shaker at 175 rpm and were grown on the experimentalC source until the inoculated fungal biomass grew by 4 to 5 ordersof magnitude. Blanks contained no fungus but were otherwise treatedlike the inoculated vessels. The final pH of the filtered mediumwas 6.25 ± 0.02 (mean ± standard deviation) for blanks and 2.90to 3.60 for fungally processed medium. The low pH of the mediumafter growth prevented reabsorption of respired CO₂ into the mediumas carbonate (pH 10.33). At harvesting, samples were plated onsolid MMN to check for contamination and to check the identifyof the fungus. Culture identity was confirmed by morphology andalso by matching rDNA internal transcribed spacer (ITS)-restrictionfragment length polymorphism patterns of cultures and the originalsporocarps used for isolation (19). PCR amplification of DNAwas performed with primers ITS1F and ITS4, and restriction fragmentlength polymorphism patterns were obtained by restriction of theamplicons with AluI and HinfIII. The numbers of replicate flasksused for each treatment were 14, 16, 18, and 15 for the blank,C. volvatus, M. androsaceus, and S. granulatus treatments on C₃sucrose, respectively, and 8, 3, 8, and 8 for the blank, C. volvatus,M. androsaceus, and S. granulatus treatments on C₄ sucrose, respectively.Except for the experiments in which three replicates were used,all experiments were performed on at least two separate occasionsand the results of the runs werepooled.

Mycelia were harvested by filtration through Fisher G8 fiberglass filters. Fungal biomass was placed in 2.5-ml Nalgene cryovials.For each replicate, biomass and a 12-ml aliquot of the filteredmedium were frozen at

80°C and then lyophilized. Two clean stainlesssteel ball bearings were added to cryovials to pulverize the biomassto a fine powder with a Wiggle-L-Bug (Crescent Dental) for 1 minbefore samples were weighed for isotopicanalysis.

CO₂ collection. The CO₂ collection vessels used (closed system) were 250-ml Erlenmeyer flasks containing 75 ml of liquid MMN with pure beetsucrose (pH 6.31) or pure cane sucrose (pH 6.45) as the C source.The vessels were each capped with a rubber stopper perforatedto hold two 5-mm-diameter glass tubes plugged by rubber septa.One of the tubes extended into the medium. After autoclaving,the flasks were inoculated with either C. volvatus or M. androsaceus.We chose these species because of their relatively fast growthrates and contrasting isotopic discrimination characteristics.The flasks were purged of CO₂ by removing the rubber septa andpumping air through two Ascarite II (Thomas Scientific)-packed10-ml VOST traps (Supelco), a fiberglass prefilter, and a 0.2-µm-pore-sizefilter (Millipore). Sterile, CO₂-free air was bubbled throughthe medium at a rate of 200 ml/s for 1 min. The septa were repositioned,and the vessels were incubated as described above for 18 days.On day 17, a 5-ml sample was extracted from the headspace withan air-tight syringe (Air-Tite) and immediately analyzed for CO₂with a mass spectrometer. One day after CO₂ collection, cultureswere harvested and used for mass spectrometry of fungal biomassand media as described above. The CO₂ concentrations in blanksafter 17 days were 0.17% ± 0.06% (mean ± standard deviation).Each system was replicated threetimes.

Mass balance. Mass balance calculations were obtained directly for the closed-system cultures and were estimated for the open-system cultures.Between 89.5 and 102.6% of the original C provided in the growthmedium was recovered in the closed-system cultures (Table 1).Variations in C recovery were attributable to losses during mycelialfiltration, because medium entrapped by mycelia was not forcefullyrecovered to avoid contamination of media with intracellular fungalproducts. C. volvatus and M. androsaceus had utilized between6.8 and 10.0% of the original C supplied for growth by the timeof harvest (Table 1). No significant growth rate differences(Mann-Whitney U test; P > 0.20) between C. volvatus and M. androsaceuswere found when the organisms were grown on either of the sugartypes provided as a C source (data not shown). The amounts ofC utilized by fungal species during growth on C₃-derived sucroseand growth on C₄-derived sucrose did not vary significantly inthe closed- or open-system flasks (Tables 1 and 2). C utilizationcould only be estimated in the open-system cultures since CO₂could not be collected quantitatively (Table 2). For this estimation,the weight of the fungal biomass was determined at the time ofharvest and the amount of CO₂ respired was calculated from theaverage CO₂/fungal biomass ratio obtained from the closed-culturemeasurements (Table 1). Less than 12% of the C originally suppliedwas utilized by C. volvatus or S. granulatus in the open-systemcultures according to these estimates; for M. androsaceus theestimated values were 25 and 24% (Table 2). We believe that latterfinding was an anomaly perhaps related to specific efficienciesin C use by this fast-growing fungus. Otherwise, the small proportionof the total C utilized over the experimental period ensured thatmeasurements were obtained when the substrate was not limiting,reducing potential artifacts related to differential growth ratesand saturation dynamics. Under these conditions, isotopic discriminationis expected to be at a maximum (29). Furthermore, preliminaryexperiments with S. granulatus (a slow grower) and M. androsaceus(a fast grower) indicated that the isotopic values of whole-cellpreparations were constant for each species, i.e., independentof incubation time between 25 and 58 days. For these reasons,the isotopic values reported in this paper are not corrected forthe amount of C utilized.

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TABLE 1. C mass balances for closed-system incubations for two fungal species on C₃- and C₄-derived sucrose

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TABLE 2. Estimated C mass balances for open-system incubations for three fungal species on C₃- and C₄-derived sucrose

Isotopic analysis. C isotopic composition was determined with a 20/20 stable-isotope-ratio mass spectrometer (Europa Scientific). For biomass,isotopic signatures represented total C and were not differentiatedbased on cellular fractions. Values are reported in the standardnotation (¹³C; per mille) relative to the international standard Pee-Dee Belemniteusing NIST Peach Leaves no. 1547 as a standard, where ¹³C = [(R_sample/R_standard) 1] × 1,000, and R is the ¹³C/¹²C molar ratio (29). Isotopic discriminationthe change in ¹³C from the medium to the fungal biomass or the biomass to theCO₂is reported as = ¹³C_final - ¹³C_initial. Subscripts of designate the reaction under consideration,so that _bf represents the discrimination observed fromC uptake into fungal biomass (f) compared to the blank growthmedium (b) and _fCO₂ is the discrimination that resultsfrom fungal respiration. The blanks were controls containing uninoculatedmedia that were treated like other experimental flasks. The instrumentalprecision values, estimated by using standard ground peach leaves(NIST no. 1547) for solid samples and pure CO₂ (Matson) for CO₂,were 0.02 to 0.06 and 0.04 (standard deviations for individualruns), respectively. Each sample was run twice, and values wereaveraged; the duplicate values were always within <0.07 of eachother for solid C and within <0.05 for CO₂ samples. The valueswere corrected for linearity relative to the beam area of thestandard. The values reported are averages from all experimentalruns.

An "expected"

¹³C value for media after fungal growth was estimated by calculating the molar amount of ¹³C involved in the shift from blank medium to fungal products,taking into account the total C in the biomass and its correspondingCO₂. This molar amount was subtracted from the equivalent valuefor blank medium to produce the expected

¹³C value for the medium after fungal growth (Table 1).

Statistical analysis. Statistical analyses were performed by using parametric and nonparametric statistical methods in JMP 3.2.1 (SAS Institute)according to the distributions and variances of the data. Sinceno difference was found between pure and impure sugars for eitherC₃ or C₄ sucrose (on C₃ sucrose, the t test values for M. androsaceusand S. granulatus were P = 0.495 and P = 0.949, respectively;on C₄ sucrose, the corresponding values were P > 0.696 and P >0.125, respectively), the data reported correspond to data forall relevant runs performed with impure and pure sucrose. Theresults for C. volvatus represent pooled data obtained with twogenetically differentisolates.

	RESULTS AND DISCUSSION

Top Abstract Introduction Materials and Methods Results and Discussion References

On C₃-derived sucrose, M. androsaceus, C. volvatus, and S. granulatus each had a characteristic isotopic enrichment in ¹³C relative to the substrate, and the _bf values were 0.67± 0.05, 4.87 ± 0.42, and 4.91 ± 0.47 (mean ± standard error),respectively (Fig. 1). On C₃-derived sucrose, significant taxon-specificisotope effects were suggested by the low variability exhibitedby the two C. volvatus genotypes studied (standard error of _bf= 1.04) compared to the variability among different species (P< 0.01), although only one isolate of M. androsaceus and one isolateof S. granulatus were tested. This fractionation was maintainedindependent of incubation time or C₃ plant source (beet or maple).However, when organisms were cultured on C₄-derived sucrose (canesucrose), isotopic fractionation was always reduced to negligiblelevels (Fig. 1). We concluded from these results that (i) thereare significant isotopic effects caused by sucrose utilizationby different basidiomycete species, (ii) these effects are determinedby species-specific factors, and (iii) the isotopic effects canbe markedly different depending on the origin of the sucrose availablefor fungal growth.

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FIG. 1. Isotopic fractionation by three basidiomycete species grown under ambient atmosphere conditions in liquid cultures on either C₃- or C₄-derived sucrose. The species used were C. volvatus (Cv), M. androsaceus (Ma), and S. granulatus (Sg). Isotopic discrimination (

_bf) was calculated from

¹³C values for the blank medium (Blank) and the total cell fungal biomass (cross-hatched bars). The standard error of the mean is also indicated for each bar. For each species, the solid bars represent the growth medium after fungal growth. The

_bf values are significantly different from a hypothesized value of 0.00- for all C₃ treatments (t test; P < 0.001) and for C. volvatus (P = 0.04) and M. androsaccus (P = 0.007) on C₄ sucrose.

It has been suggested recently that isotopic fractionation by fungi is determined by the ecological role of fungi (27).Recent studies in various temperate forest ecosystems have shownthat a distinction can be made between ectomycorrhizal and saprotrophicbasidiomycetes, with the former showing depletion of ¹³C compared to the latter (22, 25, 27). This difference hasbeen proposed as a diagnostic tool for these two major basidiomycetefunctional groups (22, 25, 27). Our results suggest thatsuch a distinction must stem from a mechanism other than intrinsicdiscrimination by fungi. Ecological determinants, such as substrateeffects, should be responsible for the patterns observed by otherauthors in the field, since we were unable to find a correlationbetween ecological role and intrinsic isotopic discriminationeffects in the three species which westudied.

Our discovery of differential fractionation of C₃- and C₄-derived sucrose by different fungi not only reinforces the emergingview that microbial processing can involve significant species-specificdiscrimination of stable C isotopes but also signals that thereis fine-scale regulation of such isotopic discrimination. Sincethe sucrose molecules in both C₃- and C₄-derived media are identicalin chemical structure, differences in intramolecular atomic distributionsmust account for the observed differences in fractionation ofeach sugar type by basidiomycetes. Rossman et al. (38) haveshown that ¹³C is not randomly distributed within the glucose molecule andalso that the distributions in the glucose molecules producedby a C₃ plant (beet) and a C₄ plant (maize) are different. Thisdifferentiation is the only plausible point at which whole-celldifferential discrimination could occur during fungal growth oneither C₃- or C₄-derived sugars. There are two possible mechanismsmediating the selective accumulation of ¹³C-enriched products within the fungal cell, and steric enzymaticeffects are logically ruled out due to the negligible differencebetween C₃- and C₄-derived glucose or sucrose in terms of the¹³C/¹²C molar isotopic ratios in relation to total molecular weight(16). We therefore favor the alternative, that chemical speciesderived from C₃ sucrose having different isotopic ratios are routedthrough specific biochemical pathways at different kinetic rates,resulting in the observed total cellular isotopicdiscrimination.

To shed light on the physiological roots of this problem, we concentrated on the processing of C₃-synthesized sucrose by threebasidiomycetes chosen because of their contrasting fractionationpatterns and ecophysiological roles in pine-dominated ecosystems(Fig. 1). The direction of the fractionation that occurred onC₃-derived sucrose regardless of incubation conditions was alwaysconsistent, resulting in enrichment for ¹³C in the fungal biomass (Fig. 1 and 2). This enrichment was apparentlybalanced stoichiometrically by depletion of the same isotope inthe medium (Fig. 1 and 2; Table 1). This stoichiometric balancewas strongly suggested by the consistent direction of a smallshift towards depletion in the medium, although the relativelylarge volume of medium used made the measured shift in ¹³C too small to be statistically significant in some cases (Fig.1 and 2; Table 1). The expected fractionation in medium valuescalculated from the amount of C contained in fungal biomass andits corresponding CO₂ is undistinguishable from the observed values(Table 1).

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FIG. 2. Isotopic discrimination by C. volvatus (Cv) and M. androsaceus (Ma) grown in closed liquid cultures on either C₃- or C₄-derived sucrose. Solid bars, medium; diagonally cross-hatched bars, fungal biomass; horizontally cross-hatched bars, CO₂. See the text for the definition of

. See Table 1 for mass balance data. The difference between biomass and CO₂ was significant only for C. volvatus grown on C₄ sucrose (t test; P = 0.032). The

_bf values are significantly different from a hypothesized value of 0.00

only for C₃ treatments (t test; P < 0.01).

Since in these experiments isotopic measurements were obtained by using the whole organism (total biomass), enrichment of¹³C in the fungal biomass could occur only from selective uptakeof ¹³C-enriched C or from selective loss of ¹²C from the fungal biomass, presumably through release of depletedCO₂ from respiration. It is generally known that discriminatingbiochemical reactions normally result in apparent depletion ofthe heavier ¹³C isotope in the products compared to the reagents (17, 20),and Gleixner et al. (20) suggested that depleted CO₂ could accountfor their observation that there was significant enrichment offungal tissues in the field. To test this "depleted-CO₂ hypothesis,"we produced closed-atmosphere culture conditions that allowedus to collect CO₂ from the headspace in incubation vessels. Theresults of these experiments contradict the depleted-CO₂ hypothesis,since the isotopic values for CO₂ were virtually identical tothose for the fungal biomass and were not depleted as the hypothesisrequires (Fig. 2). The _fCO₂ values obtained for all fungifor all sugar types (C₃ or C₄) are not significantly different(P > 0.25) (Fig. 2), indicating that the observed difference infractionation of C₃ and C₄ sugars cannot be attributed to differentialisotopic effects on the production of respired CO₂. We concludedfrom these observations that the only explanation which can accountfor the observed enrichment for ¹³C in the fungal biomass must be found in C uptakemechanisms.

From these observations, we propose a model for C uptake in fungi involving two alternative routes leading to differentialisotopic discrimination (Fig. 3). In the first, nonfractionatingroute, hexose molecules are brought into the cell without catabolismat a rate, r₁, so that discrimination between nonrandomly distributed¹³C and ¹²C isotopes in these molecules cannot occur. In the second, fractionatinguptake route, hexoses are broken down into triose fragments extracellularlybefore they are transported into the cell through two separateroutes having different kinetic rates (r₂ and r₃, with r₂ > r₃).If a triose containing a proportionally enriched part of the C₃-derivedhexose molecule is transported at rate r₂, enrichment of the cellularfraction would occur (Fig. 3). We refer to this model as the "dual-uptakehypothesis" of fungal isotopic discrimination. The fact that nocumulative fractionation effects were observed as cultures grewalso supports the dual-uptake hypothesis rather than the depleted-CO₂hypothesis, since if the latter hypothesis were true, a cumulativeeffect should have been observed as increasing amounts of depletedCO₂ were produced.

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FIG. 3. Proposed mechanism of differential isotopic enrichment in fungi grown on C₃ sucrose based on the known asymmetrical distribution of ¹³C and ¹²C in glucose (38). Extracellular digestion of glucose followed by uptake with different apparent uptake rates (r₂ and r₃) for the resulting trioses leads to comparative enrichment of the total cellular biomass. In contrast, direct uptake of glucose does not result in total cellular fractionation. The specific points of enrichment or depletion of glucose molecules depicted are illustrative and are not known for the specific sugars used in this study. An alternative fractionation mechanism could involve isotope asymmetry between fructose and glucose moieties in sucrose. See the text for details.

Rossman et al. (38) observed isotopic asymmetry in glucose which is much sharper in the C₃-derived sugar than in the C₄-derivedsugar. For instance, the values comparing the average isotopiccomposition of the whole molecule and those of individual atomsin the glucose ring analyzed after chemical degradation were asfollows: for C atom number 3, C₃ glucose had enrichment in ¹³C with a _averageC-3 of +2.2, while C₄ glucose had an equivalent_averageC-3 of +1.2; for C atom number 6, C₃ glucose wasdepleted with respect to the average molecular value by a _averageC-6of 5.2, whereas C₄ had a _averageC-3 of 4.0 (38).Other differences between C₃ and C₄ glucose were also shown byRossman et al. (38), and while it would be tempting to use thenumerical values of these authors to provide details of the fractionationmechanism proposed here, this would be inappropriate, given thatthe chemical and fermentation procedures used by Rossman et al.produced numerically different results and given the fact thatwe used sugars with different origins than the origins of thesugars used by these authors (H. L. Schmidt, personal communication,1999). Nevertheless, the results of Rossman et al. clearly identified(i) the existence of an asymmetrical, nonrandom distribution ofstable isotopes within the glucose molecule and (ii) a differencebetween C₃- and C₄-derived glucose in the ¹³C values of individual C atoms, which provides the only currentlyplausible explanation for our observations of differential fungalfractionation of C₃ and C₄sucrose.

A dual-uptake mechanism can also be proposed on the basis of our results showing that isotopic asymmetry could be found betweenthe fructose and glucose moieties in C₃-derived sucrose. Directsucrose uptake would not result in total cellular enrichment,whereas extracellular cleavage of the disaccharide into its monosaccharidecomponents, followed by uptake with different uptake rates forfructose and glucose, could generate the observed enrichment.Although this mechanism is conceptually equivalent to the oneillustrated in Fig. 3, there is no experimental evidence whichsuggests that direct sucrose uptake occurs in fungi or that thereshould be differential C isotopic distribution between glucoseand fructose. We were unable to obtain a reliable source of C₃-derivedglucose to eliminate thispossibility.

Earlier work at the subcellular level by Monson and Hayes with Escherichia coli (32) and Saccharomyces cerevisiae (31)also supports the hypothesis that there is an isotope effect inmicrobial metabolism derived from the asymmetrical distributionof C isotopes in glucose molecules and intermediate metabolites.These authors found that unsaturated fatty acids derived fromdifferent C atoms of acetyl coenzyme A in E. coli differed intheir isotopic signatures, with the moieties derived from theC-1 position showing depletion in ¹³C relative to the source glucose, while the moieties derived fromthe acetyl coenzyme A C-2 position displayed a signature similarto that of the source glucose (32).

In spite of evidence provided here, the dual-uptake mechanism must remain hypothetical in the absence of quantitative analyticalvalues for the specific sugars and fungi utilized in our experiments.Nevertheless, the dual-uptake hypothesis is compatible with knowndifferences in sugar usage during fermentative and respiratoryprocessing (26). It is also known that glucose can be takenup directly through specific transporter proteins for respiratorycatabolism (6, 26). Fungi may catabolize glucose and/or fructosevia an extracellular aldolase into trioses, but conclusive evidencethat this occurs is not available; however, several kinases, aswell as glucose oxidase, modify glucose extracellularly (6,14, 26, 33), and cell-free fermentation is well documented(14, 26). Significantly, we observed a shift towards greaterenrichment of fungal biomass grown on C₃ sucrose as incubationconditions were changed from fully aerated to the closed-atmosphereconditions in our CO₂ capture experiments (Fig. 2). When M. androsaceuswas grown under reduced O₂ tension, significant fractionationoccurred, although discrimination effects for this species werenegligible when it was grown in a fully aerated culture. M. androsaceuswas enriched in ¹³C by 1.01% under reduced O₂ tension compared to the ¹³C level in the aerated culture (150% increase). A similar shift(1.91 or a 40% increase) was observed for C. volvatus. Our resultstherefore suggest that isotopic discrimination in basidiomycetescan occur when C₃-synthesized hexoses are processed through biochemicalpathways that involve extracellular cleavage of the substratesugar and that the degree of discrimination might be correlatedwith environmental conditions that favor extracellular sugar processing,such as microenvironments with reduced [O₂].

It could be suggested that the differential fractionation observed here could be the result of differentially depleted metabolites,such as alcohol and organic acids released into the medium bythe fungus. We find this alternative explanation untenable giventhat (i) the CO₂ yields in our closed cultures (up to 0.85 timesthe amount of C in fungal biomass [Table 1]) suggest that protonacceptors other than oxygen were not predominant in terms of mass;(ii) our wild cultures and nonoptimized culture conditions wouldbe unlikely to produce metabolites predominantly derived froma single biochemical pathway in all fractionating species; and(iii) differentiation of C₃- and C₄-derived sugars after the accumulationof stochastic effects due to multiple enzymatic reactions andintracellular recycling would be highly unlikely. den Hollanderet al. (8) have shown that metabolic intermediaries correspondingto glucose carbons 1, 2, and 3 and 4, 5, and 6 are scrambled byaldolase and triose phosphate isomerase during glycolysis in S.cerevisiae. The intermediate sugars [1- and [6-¹³C]fructose 1,6-bisphosphate and the metabolic end products [1-or [3-¹³C]glycerol and [2-¹³C]ethanol result when S. cerevisiae is grown on [1-¹³C]glucose (8). Similar results were obtained for growth on[6-¹³C]glucose (8). The CO₂ values reported here (Fig. 2) are compatiblewith such an atomic scrambling effect, since they cannot be differentiatedfrom values obtained for the cell as a whole. The consistencyof our results, as shown by the small error values (Fig. 1 and2), therefore suggests that differentiation between C₃ and C₄sugars must occur during early processing stages, such as uptake,while the isotopic differences in the sugars are still maintainedby their stereochemicalconfigurations.

We identified two major factors, substrate atomic composition and microenvironmental conditions, which drive isotopic discrimination(or the lack thereof) by fungi. Our results establish the needto explicitly address the assumption that no isotopic fractionationoccurs during transfers between trophic levels whenever materialexchanges involve a fungal interface. Furthermore, we identifiedthe need to determine the relative influence of physiologicaland substrate effects in each specific ecological context. Nonfractionationby fungi cannot be invoked without independent evidence, but conversely,fractionation cannot be assumed to happen in fungally mediatedecosystem processing unless it is independently supported or atleast not ruled out by substrate quality and specific microenvironmentalconditions. Careful in situ measurements correlated with laboratorysimulations will be exceedingly useful in deciding whether fractionatingor nonfractionating catabolic physiology is dominant in a givenecologicalsituation.

Our results also provide a mechanistic hypothesis to account for the patterns of C isotope distribution in the field, whichhave remained generally unexplained. For example, it is generallyknown that there is a pattern of ¹³C enrichment with depth in well-aerated soil profiles in variousecosystems (5, 9, 34, 36), but there has been no conclusiveexplanation for this pattern. Two competing hypotheses have beenproposed to explain this major isotopic distribution pattern:(i) the incorporation in more recent soil layers of plant materialsderived from atmospheric CO₂ that is known to have experienceda historical trend towards depletion of ¹³C (12) and (ii) the cumulative effect of decomposition processes,particularly the selective preservation of presumably enrichedplant components in the soil organic matter (2, 3, 5,34). While the first of these hypotheses has not been criticallytested, chemical analyses of plant components indicate that theselective preservation of lignin and its derivatives should resultin depletion of ¹³C in deeper soil layers, which contradicts empirical observations(4, 34, 39). Focusing on microbial biomass, our resultssuggest that the observed increase in ¹³C abundance in deeper soil layers can be the direct result ofisotopic discrimination by fungi during decomposition, since weshow here that intrinsic metabolic processing makes fungal biomassenriched in ¹³C when fungi are presented with C₃-derived sucrose (Fig. 1 and2). Compounds derived from microbial biomass can account for alarge percentage of the C contained in soil organic matter, andthe accumulation over time of such compounds in the form of recalcitrantorganic matter in deeper soil layers would therefore result inenrichment for ¹³C with soil depth, as empiricallyobserved.

Our results showing differential fractionation between C₄- and C₃-derived substrates can seriously affect statements basedon isotopic evidence, particularly when land use change betweenC₃- and C₄-dominated ecosystems is studied. Field data supportingthe importance of recognizing differential fractionation betweenC₃ and C₄ substrates has been provided by a recent comparativeanalysis of Brachiaria humidicola (a C₃ legume) and Desmodiumovalifolium (a C₄ grass), which showed that plant materials becameenriched in ¹³C during the decomposition process for the C₃ plant but not forthe C₄ legume under identical experimental conditions (39).Therefore, it can be proposed that the combination of ecosystem-specificphotosynthetic and decomposition physiologies is paramount indetermining the natural distribution and processing of stableC isotopes in terrestrialecosystems.

The increasing reliance on stable isotope analysis to understand ecosystem processing must take into account important fractionationeffects mediated by fungal interfaces. Although some of theseeffects might conveniently mask each other, it is important torecognize that species-specific fractionation of stable C isotopesby fungi does occur and that such fractionation is finely dependenton the interaction of specific physiological processing, substrateeffects, and microenvironmentalconditions.

	ACKNOWLEDGMENTS

We thank M. O'Leary, H. L. Schmidt, M. Firestone, T. Bruns, M. Garbelotto, J. Klinman, J. Kirsch, and G. Cabana for helpfuldiscussions; T. Dawson and R. Amundson for comments on an earlierversion of the manuscript; P. Brooks for spectroscopy support;and A. Brooks for assistance with samplepreparation.

This work was supported in part by grants from the Hellman Family Fund, the USDA Agricultural Research Station, the Collegeof Natural Resources, University of California, Berkeley, andthe William Carol Smith Fellowship, University of California,Berkeley.

	FOOTNOTES

^* Corresponding author. Mailing address: Ecosystem Sciences Division, Department of Environmental Science, Policy, and Management,University of California, Berkeley, CA 94720-3110. Phone: (510)643-2452. Fax: (510) 643-5098. E-mail: ichapela@nature.berkeley.edu.

REFERENCES

Top
Abstract
Introduction
Materials and Methods
Results and Discussion
References

1. Abraham, W.-R., C. Hesse, and O. Pelz. 1998. Ratios of carbon isotopes in microbial lipids as an indicator of substrate usage. Appl. Environ. Microbiol. 64:4202-4209 [Abstract/Full Text] .
2. Agren, G. I., E. Bosatta, and J. Balesdent. 1996. Isotope discrimination during decomposition of organic matter: a theoretical analysis. Soil Sci. Soc. Am. J. 60:1121-1126 .
3. Balesdent, J. 1998. Analysis of soil organic matter dynamics using carbon isotopes. Cah. Agric. 7:201-206 .
4. Benner, R., M. L. Fogel, E. K. Sprague, and R. E. Hodson. 1987. Depletion of carbon-13 in lignin and its implications for stable carbon isotope studies. Nature (London) 329:708-710 .
5. Bernoux, M., C. C. Cerri, C. Neill, and J. F. L. De Moraes. 1998. The use of stable carbon isotopes for estimating soil organic matter turnover rates. Geoderma 82:43-58 [CrossRef] .
6. Bisson, L., and D. M. Coons. 1993. Yeast sugar transporters. Crit. Rev. Biochem. Mol. Biol. 28:259-308 [Medline] .
7. Blair, N., A. Leu, E. Munoz, J. Olsen, E. Kwong, and D. Des Marais. 1985. Carbon isotopic fractionation in heterotrophic microbial metabolism. Appl. Environ. Microbiol. 50:996-1001 [Medline] .
8. den Hollander, J. A., T. R. Brown, K. Ugurbil, and R. G. Shulman. 1979. ¹³C nuclear magnetic resonance studies of anaerobic glycolysis in suspensions of yeast cells. Proc. Natl. Acad. Sci. USA 76:6096-6100 [Medline] .
9. Desjardins, T., F. Andreux, B. Volkoff, and C. C. Cerri. 1994. Organic carbon and ¹³C contents in soils and soil size-fractions, and their changes due to deforestation and pasture installation in eastern Amazonia. Geoderma. 61:103-118 .
10. Ehleringer, J. R. 1991. Carbon-13-carbon-12 fractionation and its utility in terrestrial plant studies, p. 187-200. In D. C. Coleman, and B. Fry (ed.), Isotopic techniques in plant, soil, and aquatic biology: carbon isotope techniques. Academic Press, San Diego, Calif.
11. Farquhar, G. D., J. R. Ehleringer, and K. T. Hubick. 1989. Carbon isotope discrimination and photosynthesis. Annu. Rev. Plant Physiol. Plant Mol. Biol. 40:503-537 .
12. Flanagan, L. B., and J. R. Ehleringer. 1998. Ecosystem-atmosphere CO₂ exchange: interpreting signals of change using stable isotope ratios. Trends Ecol. Evol. 13:10-14 .
13. Flanagan, L. B., D. S. Kubien, and J. R. Ehleringer. 1999. Spatial and temporal variation in the carbon and oxygen stable isotope ratio of respired CO₂ in a boreal forest ecosystem. Tellus Ser. B Chem. Phys. Meteorol. 51:367-384 .
14. Foster, J. W. 1949. Chemical activities of fungi. Academic Press, New York, N.Y.
15. Frey, S. D., E. T. Elliott, and K. Paustian. 1999. Bacterial and fungal abundance and biomass in conventional and no-tillage agroecosystems along two climatic gradients. Soil Biol. Biochem. 31:573-585 .
16. Galimov, E. M. 1985. The biological fractionation of isotopes. Academic Press, Orlando, Fla.
17. Gannes, L. Z., C. Martinez Del Rio, and P. Koch. 1998. Natural abundance variations in stable isotopes and their potential uses in animal physiological ecology. Comp. Biochem. and Physiol. A Comp. Physiol. 119:725-737 .
18. Gannes, L. Z., D. M. O'Brien, and C. M. Del Rio. 1997. Stable isotopes in animal ecology: assumptions, caveats, and a call for more laboratory experiments. Ecology 78:1271-1276 .
19. Gardes, M., and T. D. Bruns. 1996. ITS-RFLP matching for identification of fungi. Methods Mol. Biol. 50:177-186 [Medline] .
20. Gleixner, G., H. J. Danier, R. A. Werner, and H. L. Schmidt. 1993. Correlations between the carbon-13 content of primary and secondary plant products in different cell compartments and that in decomposing basidiomycetes. Plant Physiol. 102:1287-1290 .
21. Griffiths, H. (ed.). 1998. Stable isotopes: integration of biological, ecological, and geochemical processes. Bios Scientific Publishers Ltd., Oxford, United Kingdom.
22. Hobbie, E. A., S. A. Macko, and H. H. Shugart. 1999. Insights into nitrogen and carbon dynamics of ectomycorrhizal and saprotrophic fungi from isotopic evidence Oecologia (Berlin) 118:353-360 .
23. Hobbie, E. A., S. A. Macko, and H. H. Shugart. 1999. Interpretation of nitrogen isotope signatures using the NIFTE model. Oecologia (Berlin) 120:405-415 .
24. Hogberg, P., M. N. Hogberg, M. E. Quist, A. Ekblad, and T. Nasholm. 1999. Nitrogen isotope fractionation during nitrogen uptake by ectomycorrhizal and non-mycorrhizal Pinus sylvestris. New Phytol. 142:569-576 .
25. Hogberg, P., A. H. Plamboeck, A. F. S. Taylor, and P. M. A. Fransson. 1999. Natural ¹³C abundance reveals trophic status of fungi and host-origin of carbon in mycorrhizal fungi in mixed forests. Proc. Natl. Acad. Sci. USA 96:8534-8539 [Abstract/Full Text] .
26. Jennings, D. H. 1995. The physiology of fungal nutrition. Cambridge University Press, Cambridge, United Kingdom.
27. Kohzu, A., T. Yoshioka, T. Ando, M. Takahashi, K. Koba, and E. Wada. 1999. Natural ¹³C and ¹⁵N abundance of field-collected fungi and their ecological implications New Phytol. 144:323-330 .
28. Lajtha, K., and R. H. Michener (ed.). 1994. Stable isotopes in ecology and environmental science. Blackwell Scientific Publications, Oxford, United Kingdom.
29. Lajtha, K., and R. H. Michener. 1994. Introduction, p. xi-xix. In K. Lajtha, and R. H. Michener (ed.), Stable isotopes in ecology and environmental science. Blackwell Scientific Publications, Oxford, United Kingdom.
30. Marx, D. H. 1969. The influence of ectotrophic mycorrhizal fungi on the resistance of pine roots to pathogenic infections. I. Antagonism of mycorrhizal fungi to root pathogenic fungi and soil bacteria. Phytopathology 59:153-163 .
31. Monson, K. D., and J. M. Hayes. 1982. Biosynthetic control of the natural abundance of carbon 13 at specific positions within fatty acids in Saccharomyces cerevisiae. J. Biol. Chem. 257:5568-5575 [Abstract] .
32. Monson, K. D., and J. M. Hayes. 1982. Carbon isotopic fractionation in the biosynthesis of bacterial fatty acids. Ozonolysis of unsaturated fatty acids as a means of determining the intramolecular distribution of carbon isotopes. Geochim. Cosmochim. Acta 46:139-149 .
33. Morrison, S. C., D. A. Wood, and P. M. Wood. 1999. Characterization of a glucose 3-dehydrogenase from the cultivated mushroom (Agaricus bisporus). Appl. Microbiol. Biotechnol. 51:58-64 [CrossRef] .
34. Natelhoffer, K. J., and B. Fry. 1988. Controls on natural nitrogen-15 and carbon-13 abundances in forest soil organic matter. Soil Sci. Soc. Am. J. 52:1633-1640 .
35. Newell, S. Y. 1992. Estimating fungal biomass and productivity in decomposing litter, p. 521-561. In G. C. Carrol, and D. T. Wicklow (ed.), The fungal community: its organization and role in the ecosystem, 2nd ed. Marcel Dekker, Basel, Switzerland.
36. O'Brien, B. J., and J. D. Stout. 1978. Movement and turnover of soil organic matter as indicated by carbon isotope measurements. Soil Biol. Biochem. 10:309-317 .
37. O'Leary, M. H. 1988. Carbon isotopes in photosynthesis. BioScience 38:328-336 .
38. Rossman, A., M. Butzenlechner, and H.-L. Schmidt. 1991. Evidence for a nonstatistical carbon isotope distribution in natural glucose. Plant Physiol. 96:609-614 .
39. Schweizer, M., J. Fear, and G. Cadisch. 1999. Isotopic (¹³C) fractionation during plant residue decomposition and its implications for soil organic matter studies. Rapid Commun. Mass Spectrom. 13:1284-1290 [CrossRef][Medline] .
40. Smith, M. L., J. N. Bruhn, and J. B. Anderson. 1992. The fungus Armillaria bulbosa is among the largest and oldest living organisms. Nature 356:428-431 .
41. Stapp, P., G. A. Polis, and F. S. Pinero. 1999. Stable isotopes reveal strong marine and El Niño effects on island food webs. Nature 401:467-469 [CrossRef] .
42. Vander Zanden, M. J., J. M. Casselman, and J. B. Rasmussen. 1999. Stable isotope evidence for the food web consequences of species invasions in lakes. Nature (London) 401:464-467 [CrossRef] .
43. Wedin, D. A., L. L. Tieszen, B. Dewey, and J. Pastor. 1995. Carbon isotope dynamics during grass decomposition and soil organic matter formation. Ecology 76:1383-1392 .
44. Will, O. H., III, L. L. Tieszen, T. Gerlach, and M. Kellen. 1989. Alteration of carbon isotope ratios by eight Ustilago species on defined media. Bot. Gaz. 150:152-157 .
45. Will, O. H., III, L. L. Tieszen, M. Kellen, and T. Gerlach. 1986. Stable carbon isotope discrimination in the smut fungus Ustilago violacea. Exp. Mycol. 10:83-88 .

1.	Abraham, W.-R., C. Hesse, and O. Pelz. 1998. Ratios of carbon isotopes in microbial lipids as an indicator of substrate usage. Appl. Environ. Microbiol. 64:4202-4209 [Abstract/Full Text] .
2.	Agren, G. I., E. Bosatta, and J. Balesdent. 1996. Isotope discrimination during decomposition of organic matter: a theoretical analysis. Soil Sci. Soc. Am. J. 60:1121-1126 .
3.	Balesdent, J. 1998. Analysis of soil organic matter dynamics using carbon isotopes. Cah. Agric. 7:201-206 .
4.	Benner, R., M. L. Fogel, E. K. Sprague, and R. E. Hodson. 1987. Depletion of carbon-13 in lignin and its implications for stable carbon isotope studies. Nature (London) 329:708-710 .
5.	Bernoux, M., C. C. Cerri, C. Neill, and J. F. L. De Moraes. 1998. The use of stable carbon isotopes for estimating soil organic matter turnover rates. Geoderma 82:43-58 [CrossRef] .
6.	Bisson, L., and D. M. Coons. 1993. Yeast sugar transporters. Crit. Rev. Biochem. Mol. Biol. 28:259-308 [Medline] .
7.	Blair, N., A. Leu, E. Munoz, J. Olsen, E. Kwong, and D. Des Marais. 1985. Carbon isotopic fractionation in heterotrophic microbial metabolism. Appl. Environ. Microbiol. 50:996-1001 [Medline] .
8.	den Hollander, J. A., T. R. Brown, K. Ugurbil, and R. G. Shulman. 1979. ¹³C nuclear magnetic resonance studies of anaerobic glycolysis in suspensions of yeast cells. Proc. Natl. Acad. Sci. USA 76:6096-6100 [Medline] .
9.	Desjardins, T., F. Andreux, B. Volkoff, and C. C. Cerri. 1994. Organic carbon and ¹³C contents in soils and soil size-fractions, and their changes due to deforestation and pasture installation in eastern Amazonia. Geoderma. 61:103-118 .
10.	Ehleringer, J. R. 1991. Carbon-13-carbon-12 fractionation and its utility in terrestrial plant studies, p. 187-200. In D. C. Coleman, and B. Fry (ed.), Isotopic techniques in plant, soil, and aquatic biology: carbon isotope techniques. Academic Press, San Diego, Calif.
11.	Farquhar, G. D., J. R. Ehleringer, and K. T. Hubick. 1989. Carbon isotope discrimination and photosynthesis. Annu. Rev. Plant Physiol. Plant Mol. Biol. 40:503-537 .
12.	Flanagan, L. B., and J. R. Ehleringer. 1998. Ecosystem-atmosphere CO₂ exchange: interpreting signals of change using stable isotope ratios. Trends Ecol. Evol. 13:10-14 .
13.	Flanagan, L. B., D. S. Kubien, and J. R. Ehleringer. 1999. Spatial and temporal variation in the carbon and oxygen stable isotope ratio of respired CO₂ in a boreal forest ecosystem. Tellus Ser. B Chem. Phys. Meteorol. 51:367-384 .
14.	Foster, J. W. 1949. Chemical activities of fungi. Academic Press, New York, N.Y.
15.	Frey, S. D., E. T. Elliott, and K. Paustian. 1999. Bacterial and fungal abundance and biomass in conventional and no-tillage agroecosystems along two climatic gradients. Soil Biol. Biochem. 31:573-585 .
16.	Galimov, E. M. 1985. The biological fractionation of isotopes. Academic Press, Orlando, Fla.
17.	Gannes, L. Z., C. Martinez Del Rio, and P. Koch. 1998. Natural abundance variations in stable isotopes and their potential uses in animal physiological ecology. Comp. Biochem. and Physiol. A Comp. Physiol. 119:725-737 .
18.	Gannes, L. Z., D. M. O'Brien, and C. M. Del Rio. 1997. Stable isotopes in animal ecology: assumptions, caveats, and a call for more laboratory experiments. Ecology 78:1271-1276 .
19.	Gardes, M., and T. D. Bruns. 1996. ITS-RFLP matching for identification of fungi. Methods Mol. Biol. 50:177-186 [Medline] .
20.	Gleixner, G., H. J. Danier, R. A. Werner, and H. L. Schmidt. 1993. Correlations between the carbon-13 content of primary and secondary plant products in different cell compartments and that in decomposing basidiomycetes. Plant Physiol. 102:1287-1290 .
21.	Griffiths, H. (ed.). 1998. Stable isotopes: integration of biological, ecological, and geochemical processes. Bios Scientific Publishers Ltd., Oxford, United Kingdom.
22.	Hobbie, E. A., S. A. Macko, and H. H. Shugart. 1999. Insights into nitrogen and carbon dynamics of ectomycorrhizal and saprotrophic fungi from isotopic evidence Oecologia (Berlin) 118:353-360 .
23.	Hobbie, E. A., S. A. Macko, and H. H. Shugart. 1999. Interpretation of nitrogen isotope signatures using the NIFTE model. Oecologia (Berlin) 120:405-415 .
24.	Hogberg, P., M. N. Hogberg, M. E. Quist, A. Ekblad, and T. Nasholm. 1999. Nitrogen isotope fractionation during nitrogen uptake by ectomycorrhizal and non-mycorrhizal Pinus sylvestris. New Phytol. 142:569-576 .
25.	Hogberg, P., A. H. Plamboeck, A. F. S. Taylor, and P. M. A. Fransson. 1999. Natural ¹³C abundance reveals trophic status of fungi and host-origin of carbon in mycorrhizal fungi in mixed forests. Proc. Natl. Acad. Sci. USA 96:8534-8539 [Abstract/Full Text] .
26.	Jennings, D. H. 1995. The physiology of fungal nutrition. Cambridge University Press, Cambridge, United Kingdom.
27.	Kohzu, A., T. Yoshioka, T. Ando, M. Takahashi, K. Koba, and E. Wada. 1999. Natural ¹³C and ¹⁵N abundance of field-collected fungi and their ecological implications New Phytol. 144:323-330 .
28.	Lajtha, K., and R. H. Michener (ed.). 1994. Stable isotopes in ecology and environmental science. Blackwell Scientific Publications, Oxford, United Kingdom.
29.	Lajtha, K., and R. H. Michener. 1994. Introduction, p. xi-xix. In K. Lajtha, and R. H. Michener (ed.), Stable isotopes in ecology and environmental science. Blackwell Scientific Publications, Oxford, United Kingdom.
30.	Marx, D. H. 1969. The influence of ectotrophic mycorrhizal fungi on the resistance of pine roots to pathogenic infections. I. Antagonism of mycorrhizal fungi to root pathogenic fungi and soil bacteria. Phytopathology 59:153-163 .
31.	Monson, K. D., and J. M. Hayes. 1982. Biosynthetic control of the natural abundance of carbon 13 at specific positions within fatty acids in Saccharomyces cerevisiae. J. Biol. Chem. 257:5568-5575 [Abstract] .
32.	Monson, K. D., and J. M. Hayes. 1982. Carbon isotopic fractionation in the biosynthesis of bacterial fatty acids. Ozonolysis of unsaturated fatty acids as a means of determining the intramolecular distribution of carbon isotopes. Geochim. Cosmochim. Acta 46:139-149 .
33.	Morrison, S. C., D. A. Wood, and P. M. Wood. 1999. Characterization of a glucose 3-dehydrogenase from the cultivated mushroom (Agaricus bisporus). Appl. Microbiol. Biotechnol. 51:58-64 [CrossRef] .
34.	Natelhoffer, K. J., and B. Fry. 1988. Controls on natural nitrogen-15 and carbon-13 abundances in forest soil organic matter. Soil Sci. Soc. Am. J. 52:1633-1640 .
35.	Newell, S. Y. 1992. Estimating fungal biomass and productivity in decomposing litter, p. 521-561. In G. C. Carrol, and D. T. Wicklow (ed.), The fungal community: its organization and role in the ecosystem, 2nd ed. Marcel Dekker, Basel, Switzerland.
36.	O'Brien, B. J., and J. D. Stout. 1978. Movement and turnover of soil organic matter as indicated by carbon isotope measurements. Soil Biol. Biochem. 10:309-317 .
37.	O'Leary, M. H. 1988. Carbon isotopes in photosynthesis. BioScience 38:328-336 .
38.	Rossman, A., M. Butzenlechner, and H.-L. Schmidt. 1991. Evidence for a nonstatistical carbon isotope distribution in natural glucose. Plant Physiol. 96:609-614 .
39.	Schweizer, M., J. Fear, and G. Cadisch. 1999. Isotopic (¹³C) fractionation during plant residue decomposition and its implications for soil organic matter studies. Rapid Commun. Mass Spectrom. 13:1284-1290 [CrossRef][Medline] .
40.	Smith, M. L., J. N. Bruhn, and J. B. Anderson. 1992. The fungus Armillaria bulbosa is among the largest and oldest living organisms. Nature 356:428-431 .
41.	Stapp, P., G. A. Polis, and F. S. Pinero. 1999. Stable isotopes reveal strong marine and El Niño effects on island food webs. Nature 401:467-469 [CrossRef] .
42.	Vander Zanden, M. J., J. M. Casselman, and J. B. Rasmussen. 1999. Stable isotope evidence for the food web consequences of species invasions in lakes. Nature (London) 401:464-467 [CrossRef] .
43.	Wedin, D. A., L. L. Tieszen, B. Dewey, and J. Pastor. 1995. Carbon isotope dynamics during grass decomposition and soil organic matter formation. Ecology 76:1383-1392 .
44.	Will, O. H., III, L. L. Tieszen, T. Gerlach, and M. Kellen. 1989. Alteration of carbon isotope ratios by eight Ustilago species on defined media. Bot. Gaz. 150:152-157 .
45.	Will, O. H., III, L. L. Tieszen, M. Kellen, and T. Gerlach. 1986. Stable carbon isotope discrimination in the smut fungus Ustilago violacea. Exp. Mycol. 10:83-88 .

Differential C Isotope Discrimination by Fungi during Decomposition of C3- and C4-Derived Sucrose

Differential C Isotope Discrimination by Fungi during Decomposition of C₃- and C₄-Derived Sucrose