Elemental Sulfur and Thiosulfate Disproportionation by Desulfocapsa sulfoexigens sp. nov., a New Anaerobic Bacterium Isolated from Marine Surface Sediment

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Appl Environ Microbiol, January 1998, p. 119-125, Vol. 64, No. 1
0099-2240/98/$04.00+0
Copyright © 1998, American Society for Microbiology. All rights reserved.

Elemental Sulfur and Thiosulfate Disproportionation by Desulfocapsa sulfoexigens sp. nov., a New Anaerobic Bacterium Isolated from Marine Surface Sediment

Kai Finster,¹^,^* Werner Liesack,² and Bo Thamdrup³

Department of Microbial Ecology, Institute of Biological Sciences, University of Aarhus, DK-8000 Aarhus C, Denmark,¹ and Max-Planck-Institut für terrestrische Mikrobiologie, D-35043 Marburg,² and Max-Planck-Institut für marine Mikrobiologie, D-28359 Bremen,³ Germany

Received 25 June 1997/Accepted 10 October 1997

	ABSTRACT

Top Abstract Introduction Materials & Methods Results Discussion References

A mesophilic, anaerobic, gram-negative bacterium, strain SB164P1, was enriched and isolated from oxidized marine surface sedimentwith elemental sulfur as the sole energy substrate in the presenceof ferrihydrite. Elemental sulfur was disproportionated to hydrogensulfide and sulfate. Growth was observed exclusively in the presenceof a hydrogen sulfide scavenger, e.g., ferrihydrite. In the absenceof a scavenger, sulfide and sulfate production were observed butno growth occurred. Strain SB164P1 grew also by disproportionationof thiosulfate and sulfite. With thiosulfate, the growth efficiencywas higher in ferrihydrite-supplemented media than in media withoutferrihydrite. Growth coupled to sulfate reduction was not observed.However, a slight sulfide production occurred in cultures incubatedwith formate and sulfate. Strain SB164P1 is the first bacteriumdescribed that grows chemolithoautotrophically exclusively bythe disproportionation of inorganic sulfur compounds. Comparative16S rDNA sequencing analysis placed strain SB164P1 into the deltasubclass of the class Proteobacteria. Its closest relative isDesulfocapsa thiozymogenes, and slightly more distantly relatedare Desulfofustis glycolicus and Desulforhopalus vacuolatus. Thisphylogenetic cluster of organisms, together with members of thegenus Desulfobulbus, forms one of the main lines of descent withinthe delta subclass of the Proteobacteria. Due to the common phenotypiccharacteristics and the phylogenetic relatedness to Desulfocapsathiozymogenes, we propose that strain SB164P1 be designated thetype strain of Desulfocapsa sulfoexigens sp. nov.

	INTRODUCTION

Top Abstract Introduction Materials & Methods Results Discussion References

Since Bak and Cypionka (2) first described an energy metabolism based on the disproportionation of the inorganic sulfurcompounds thiosulfate and sulfite into sulfide and sulfate bya sulfate reducer designated Desulfovibrio sulfodismutans (3),this type of process has been recognized in numerous genera ofsulfate-reducing bacteria (15). However, most of the sulfatereducers tested were unable to couple the disproportionation ofinorganic sulfur compounds to growth. Disproportionation can bedescribed as an inorganic fermentation in which sulfur compoundswith an intermediate oxidation state serve as both electron donorsand electron acceptors in an energy-generating redox process (27).In recent years, it was demonstrated that thiosulfate disproportionationis an important metabolism in sulfur transformations in aquaticsystems (13) and that microorganisms which are able to carryout this type of metabolism are numerically abundant (3, 14).

Recently, Thamdrup et al. (32) discovered that enrichment cultures with elemental sulfur and iron or manganese oxides wereable to grow by disproportionation of elemental sulfur. This observationwas surprising, because under standard conditions the reactionis endergonic with $Delta$ G'° = 40.9 kJ reaction¹ (2). The authors stressed that the use of oxidized metalsas sulfide scavengers makes the process energetically favorable.Disproportionation of elemental sulfur in pure cultures was firstreported by Bak (1). The organism, later named Desulfocapsathiozymogenes, is a freshwater sulfate reducer that grows eitherheterotrophically by incomplete oxidation of different alcoholsor chemolithoautotrophically by disproportionation of thiosulfate,sulfite, or elemental sulfur (12). Apart from the recently describedspecies Desulforhopalus vacuolatus (11) and Desulfofustis glycolicus(9; see below), Desulfocapsa thiozymogenes is most closelyrelated to Desulfobulbus spp. Recently, Lovley and Phillips (18)have demonstrated that Desulfobulbus propionicus 1pr3 is alsoable to disproportionate elemental sulfur. However, this metabolismwas observed only when ferric iron was present in the medium asa sulfide scavenger, and growth was very slow.

In this communication, we report on the enrichment, isolation, and phylogenetic affiliation of a marine microorganism thatgrows exclusively chemolithoautotrophically by elemental sulfur,thiosulfate, and sulfite disproportionation.

	MATERIALS AND METHODS

Top Abstract Introduction Materials & Methods Results Discussion References

Sources of inoculum, media, enrichment, and isolation. Oxidized surface sediment from an eelgrass (Zostera noltii)-covered mud flat in the basin of Arcachon (France) served as theinoculum for a dilution series. Aliquots (9 ml) of carbonate-bufferedmarine minimal medium supplemented with trace metals and vitamins(for details, see reference 32; the only modification was theuse of 20 g of NaCl liter¹ instead of 15 g liter¹) were dispensed into sterile 16-ml glass test tubes. The testtubes had been supplied in advance with 1 ml of a 300 mM heat-sterilizedsuspension of ferrihydrite [Fe(OH)₃] and 200 to 300 mg of sterilesulfur flowers. A 1-cm³ portion of oxidized surface mud was added via a tip-cut plasticsyringe to the first test-tube in a series of seven. The mediumand the sediment was thoroughly mixed, and 1 ml of the homogenizedslurry was transferred to the next test tube. The procedure wasrepeated until all the tubes had been inoculated. The gas phaseof each tube was exchanged for a gas mixture of 90% N₂-10% CO₂,and the tubes were sealed with black rubber stoppers. The inoculatedtest tubes were incubated in the dark at 22°C for up to 12 weeks.Positive enrichments were identified by the formation of ironsulfides produced during the disproportionation of elemental sulfur(32). Sulfur-disproportionating bacteria were isolated by deepagar dilutions (23) prepared as described by Finster et al.(7). The isolation tubes contained two separated agar layers,one consisting of 1 ml of ferrihydrite suspension in 3 ml of 3%agar and the second containing inoculum and elemental sulfur in6 ml of 1% agar. Colonies were withdrawn from the agar deeps withdrawn Pasteur pipettes and transferred to liquid medium containingferrihydrite and elemental sulfur. Tubes containing sulfur-disproportionatingbacteria were identified by iron sulfide formation.

The purification procedure was repeated by deep agar dilutions in basal marine medium supplemented with ferrous iron (0.52g of FeCl₂ · 4H₂O liter¹) instead of the iron agar layer and thiosulfate (10 mM) insteadof elemental sulfur. Growing colonies were directly identifiableas black spots in the agar as a result of iron sulfide precipitation.The colonies were transferred to liquid medium containing thiosulfatein ferrous iron medium, and grown cultures were examined microscopicallyto compare the morphology with that of the original isolate fromelemental sulfur-containing medium. Also, the capability of elementalsulfur disporportionation was tested. Cultures were routinelygrown with elemental sulfur in the presence of ferrihydrite.

Purity was tested in medium supplemented with fumarate (5 mM), pyruvate (5 mM), glucose (10 mM), and yeast extract (0.1%)and by regular microscopic checks.

Stoichiometry of the disproportionations. The transformations of thiosulfate and elemental sulfur were quantified in 250-ml batch cultures in medium with and withoutferrihydrite. Cultures were inoculated with 2% (vol/vol) of apregrown culture, incubated at 28°C in the dark, and sampled regularlyfor 11 days when thiosulfate was the substrate and for 24 dayswhen elemental sulfur was the substrate. Aliquots for sulfate,dissolved sulfide, and thiosulfate determination were filteredunder N₂ and preserved in zinc acetate (final concentration, 0.2%),while aliquots for iron sulfides were preserved unfiltered inzinc acetate (final concentration, 5%). Aliquots for cell countswere fixed in glutaraldehyde (final concentration, 2.5%). Aliquotsof 100 µl for Fe(II) measurements were extracted in 5 ml of 0.5N HCl. Immediately after each sampling, the headspace of the incubationbottles was flushed with a gas mixture consisting of 90% N₂-10%CO₂, and the bottles were sealed with rubber stoppers.

Substrate tests. The spectrum of electron donors and electron acceptors used by the isolate was determined by using 20-ml screw-cap test tubesfilled to the rim. The tubes were filled with only 10 ml of mediumwhen oxygen was supplied as the electron acceptor. The bacteriawere precultivated with elemental sulfur and ferrihydrite. Theinoculum was 1% (vol/vol) of a pregrown culture. In electron donortests, either sulfur, thiosulfate (10 mM), sulfate (10 mM), dimethylsulfoxide (10 mM), nitrate (5 mM), or oxygen (0.02 atm) servedas the electron acceptor. Test medium containing elemental sulfuror thiosulfate and ferrihydrite served as positive controls. Inelectron donor tests when sulfate served as electron acceptor,ferrihydrite was added to visualize the production of hydrogensulfide. The sulfate-reducing capacity of strain SB164P1 was alsoassayed in ferric iron-free incubations with sulfate (10 mM),formate (10 mM), acetate, propionate, pyruvate, lactate, fumarate,or hydrogen (90%) as the electron donor (concentrations, 5 mMif not otherwise indicated). The test tubes were incubated at26°C in the dark. All tests were carried out in duplicate, andthe tubes were incubated for 4 weeks and periodically examinedfor sulfide production and/or growth.

The capacity of dissimilatory sulfate reduction was measured as the amount of radiolabeled hydrogen sulfide produced afteran incubation period of 7 days with radiolabeled sulfate. Thefollowing substrates were tested, based on our knowledge aboutcompounds metabolized by the different genera of sulfate-reducingbacteria (36) (concentrations in parentheses, 5 mM if not indicated):formate (10 mM), acetate, propionate, butyrate, valerate, pyruvate,lactate, succinate, malate, fumarate, glucose, benzoate (1 mM),nicotinate (1 mM), betaine, choline chloride, methanol (10 mM),ethanol, n-propanol, n-butanol, alanine, glutamate, $alpha$ -ketoglutarate,oxaloacetate, and citrate. The following incubations served ascontrols: (i) unsupplemented cultures to determine the backgroundsulfate transformation, and (ii) sulfur- or thiosulfate-supplementedcultures to determine sulfate transformation during sulfur orthiosulfate disproportionation.

The experiment was conducted as follows. Aliquots (2.5 ml) of an outgrown thiosulfate-ferrihydrite culture were transferredto evacuated sterile 5-ml rubber-septum-sealed glass vials witha sterile plastic syringe and needle. The cultures were supplementedwith the electron donor and sulfate from sterile stock solutionsto give a sulfate concentration of approximately 10 mM and a finalvolume of approximately 3 ml. Finally, 5 µl of carrier-free radiolabeledsulfate was added, resulting in an activity of 4.5 kBq µM¹ (sulfate). In total, 56 vials were prepared. Two incubationswere stopped immediately after addition of radiolabeled sulfateby injection of 0.5 ml of a 20% zinc acetate solution. They wereused to check if labeled sulfate is reduced chemically. The otherincubations were stopped after 7 days by an injection of zincacetate. Reduced radiolabeled sulfur was released from the mediumby the single-step chromium-reduction method (8) and countedwith a liquid scintillation counter.

Growth parameters. The vitamin requirements, as well as the pH, salt, and temperature tolerance of the isolate, were studied by incubating theisolate in 20-ml screw-cap test tubes with elemental sulfur andferrihydrite. Activity was monitored by microscopic examinationand by observing the formation of iron sulfide.

The temperature range for growth was determined by incubating inoculated test tubes in an insulated aluminum temperature gradientblock with a minimum temperature of 0°C and a maximum temperatureof 50°C in 5°C steps. All experiments were carried out in duplicateand stopped after a maximum of 6 weeks.

Growth conditions were evaluated by comparing the time passed until iron sulfide formation was observed. The fastest ironsulfide formation was interpreted as optimal conditions.

Molybdate addition. Thiosulfate-ferrihydrite-grown cultures of strain SB164P1 were inoculated into marine medium with thiosulfate plus ferrihydriteor elemental sulfur plus ferrihydrite and increasing concentrationsof molybdate (0, 0.5, 5, 50, 500, or 5,000 µM), a specific inhibitorof sulfate-reducing bacteria. This experiment was stimulated bythe recent publication by Krämer and Cypionka (15), proposingthat the reversal of sulfate reduction serves as the energy generatingpathway in thiosulfate-disproportionating sulfate reducers.

Analytical procedures. Sulfide was determined spectrophotometrically by the methylene blue method (5). Sulfate and thiosulfate were quantifiedby nonsuppressed anion-exchange chromatography (pump model 510,IC-Pak anion column, conductivity detector model 430 [Waters]).HCl-extracted Fe²⁺ was measured spectrophotometrically by monitoring its reactionwith Ferrozine without reducing agents (28) (0.1% in 50 mM HEPES[pH 7]), and total HCl-extractable Fe was measured similarly withreducing Ferrozine (Ferrozine with 1% hydroxylamine hydrochloride).

Acid-volatile and chromium-reducible sulfur compounds were separated by a two-step distillation procedure (8). Before distillation,zinc acetate-fixed samples were filtered through fiberglass filtersthat retained the sulfides. Elemental sulfur, present in excessin elemental sulfur-grown cultures, was removed by giving thefilters a wash with acetone, followed by three consecutive washeswith CS₂ and a final acetone wash. Thus, chromium reducible sulfuronly represents pyrite.

Cell counts. Cell counts were performed on glutaraldehyde-preserved aliquots. Before being counted, iron precipitates were dissolved ina dithionite solution (50 g of sodium dithionite liter¹ in 0.2 M sodium citrate and 0.35 M acetic acid) (17). Then50 to 200 µl of the preserved sample was added to 2 ml of theextractants. After 5 min, the mixture was filtered through a black0.2-µm-pore-size polycarbonate filter, which was subsequentlystained with 0.01% acridine orange for 1 min. The staining solutionwas filtered off, and the filter was washed with 90% methanolto remove nonspecifically bound acridine orange. All the solutionswere sterilized by filtration (0.2-µm-pore-size filter). The cellswere counted by epifluorescence microscopy.

G+C content of DNA. The G+C content of the DNA was determined by high-pressure liquid chromatography separation and UV detection (30). Calibrationand G+C determination were performed as described by Mesbah etal. (20).

Comparative 16S rDNA sequence analysis. DNA isolation, PCR-mediated amplification of the 16S rRNA gene from positions 28 to 1491 (numbering according to the InternationalUnion of Biochemistry nomenclature for Escherichia coli 16S rRNA),and sequencing analysis were done as previously described by Liesackand Finster (16) but with one modification: instead of purificationon Centricon 100 columns (Amicon, Witten, Germany), the 16S rDNAPCR products were purified with the Prep-A-Gene kit (Bio-Rad,Munich, Germany) as specified by the manufacturer. The 16S rDNAsequence of strain SB164P1 was added to a database of about 6,000publicly available bacterial 16S rRNA sequences (19, 25, 33).The database is part of the ARB (from "arbor", Latin: tree) programpackage (29). The 16S rDNA sequence from strain SB164P1 wasintegrated into this database with the automatic alignment toolof the ARB program package (29). This procedure revealed strainSB164P1 as a true member of the delta subclass of the class Proteobacteria.The phylogenetic position of strain SB164P1 was determined inmore detail by comparing its 16S rDNA sequence with 69 referencesequences comprising the main lines of descent within the deltasubclass of the Proteobacteria. The overall tree topology wasevaluated by distance matrix analyses. Evolutionary distancesbetween pairs of microorganisms were calculated for a sequencestretch ranging from positions 28 through 1435 (E. coli 16S rRNAnumbering) including only positions present in both sequencesof the respective sequence pairs (ARB and PHYLIP [6]). Sincethe inclusion of highly variable regions of the 16S rRNA geneinto the analysis may blur the reconstructed tree due to the highmutational rate of these nucleotide sequence positions and possiblealignment errors, these regions were excluded from the phylogeneticanalysis. To do that, two different approaches were used (i) manualremoval of regions that are known to be highly variable (34)and could not be aligned unambiguously (i.e., positions 69 to100, 182 to 218, 451 to 479, 833 to 853, 998 to 1042, and 1133to 1141 in the E. coli 16S rRNA numbering), and (ii) use of onlythe alignment positions for the phylogenetic analysis which containedidentical nucleotides in at least 50% of the 16S rRNA sequencesunder comparison. The usefulness of this invariance criterionapplied in the second approach for the inclusion and exclusion,respectively, of individual alignment positions was shown previously(9). The base frequency of the alignment positions was determinedby using the respective tool of the ARB program package. The treeswere constructed with the neighbor-joining algorithm (26) (ARBand PHYLIP). In addition, different subsets of about 30 16S rRNAsequences were reanalyzed by maximum-likelihood methods (fastDNAml[19] and ARB) to examine the significance of the phylogeneticposition of strain SB164P1 as it has been determined by usingthe larger data set of 69 reference 16S rRNA sequences in conjunctionwith the neighbor-joining algorithm.

Nucleotide sequence accession number. The 16S rDNA sequence of strain SB164P1 has been deposited in the EMBL, GenBank, and DDBJ nucleotide sequence databases underaccession no. Y13672.

	RESULTS

Top Abstract Introduction Materials & Methods Results Discussion References

Enrichment cultures. Black spots in the reddish brown ferrihydrite, indicating the formation of iron sulfide, were observed in the first dilutionstep after 4 days and occurred up to the fifth dilution step.Sulfate accumulated concomittantly with iron sulfide. Culturesfrom the highest dilution with growth (10⁵) were used for further isolation. Microscopic examination revealedtwo major bacterial morphotypes. The predominant type was rodshaped and slender, and some cells were motile. The other typewas coccoid and nonmotile. Both types grew in close proximityto the particle phase, and an increased numbers of cells wereseen after particle disruption. Bacteria were seldom observedin supernatant aliquots. In addition to the dominating cell types,small, highly motile vibrioid cells were observed. The cultureused for isolation was purified by repeated application of deepagar dilution series.

Isolation. In low agar dilutions (up to tube 3), large amounts of black iron sulfide developed within 3 weeks of incubation and obscuredthe bacterial colonies. In the higher dilutions, only a littleiron sulfide was produced, allowing the identification of bacterialcolonies under the dissection microscope. The colonies were roundand whitish and developed in close proximity to sulfur particles.A microscopic examination of an isolated colony revealed onlyslender rod-shaped cells. After a transfer to liquid medium, fivemorphologically identical cultures were obtained. The cultureswere able to grow with thiosulfate as a substitute for elementalsulfur. An additional purification was conducted with thiosulfateand Fe²⁺, leaving out the iron agar layer. Thiosulfate-disproportionatingcolonies were black due to iron precipitates. Well-separated coloniesfrom the highest dilution were transferred to liquid thiosulfate-containingmedium. Microscopic examination of the colonies revealed the samestructure and cell type as described for the sulfur-ferrihydriteagar shakes. The six isolates were able to grow by elemental sulfurdisproportionation. One isolate, designated SB164P1, was chosenfor detailed physiological and phylogenetic characterization.

Morphology. Strain SB164P1 cells were 2 to 4 µm long and 0.5 µm wide with slightly pointed ends (Fig. 1). Motile cells were observed.Cells from outgrown cultures stained gram negative.

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FIG. 1. Phase-contrast photomicrograph of D. sulfoexigens SB164P1 grown with elemental sulfur and ferrihydrite. Most ferrihydrite and iron sulfide precipitates were dissolved by dithionite-citrate-acetic acid extraction. Residual precipitates are seen as highly refractive aggregates. Bar, 10 µm.

Growth and temperature requirements. Strain SB164P1 did not require organic carbon or vitamins for growth, but NaCl and MgCl₂ were necessary for growth. Growthwas inhibited below 25 mM NaCl and 2 mM MgCl₂ · 6H₂O. The culturesdeveloped equally well within concentration ranges of 170 to 330mM NaCl and 7 to 15 mM MgCl₂ · 6H₂O, respectively. Higher concentrationswere not tested. The pH range for growth was from 6.0 to 8.2 withan optimum between 6.7 and 7.3. In growing cultures, the pH coulddrop below 6.0 when elemental sulfur served as the substrate.The pH tests were carried out in bicarbonate-buffered medium only.Strain SB164P1 grew within a temperature range from 5 to 35°C.The optimum growth temperature was 30°C.

Metabolic properties. Apart from sulfur, thiosulfate, and sulfite disproportionation, strain SB164P1 reduced small amounts of sulfate in the presenceof formate and hydrogen. Within a period of 6 weeks, 0.09 and0.11 mM sulfide were produced in the presence of formate and hydrogen,respectively. Sulfate reduction did not sustain growth. No sulfidewas detectable (detection limit, 1 µM) in the other incubations.Sulfate reduction with formate was also demonstrated in incubationswith radiolabeled sulfate. Radiolabeled sulfide accumulated exclusivelywith formate as the electron donor. A fermentative type of metabolismwith pyruvate, lactate, or glucose was not observed. Neither nitrate,dimethyl sulfoxide, nor oxygen (2%) was used as the electron acceptor.

Disproportionation of sulfur compounds. Elemental sulfur and thiosulfate were disproportionated by strain SB164P1 with or without ferric iron present in the growthmedium (Fig. 2 and 3). The rate of thiosulfate consumption wassimilar in the presence and absence of ferrihydrite. In ferriciron-free medium (Fig. 2, top), the ratio of sulfate producedto thiosulfate consumed was 1:1, in agreement with thiosulfatedisproportionation:

<UP>S2O</UP><UP>3</UP><UP>2−</UP><UP> + H2O → SO</UP><UP>4</UP><UP>2−</UP><UP> + HS− + H+</UP>

Sulfide production was somewhat lower than predicted, which can be explained by degassing of H₂S. When ferrihydrite was presentas a sulfide scavenger during thiosulfate disproportionation (Fig.2, middle), the amount of sulfate plus sulfide produced closelymatched the amount of thiosulfate consumed. Under these conditions,sulfide accumulated as FeS and dissolved sulfide was not detectable,so that loss through degassing was excluded. Ferrihydrite reactsrapidly with hydrogen sulfide, producing Fe²⁺. Ferrous iron may further precipitate sulfide as FeS (24),and elemental sulfur formed may be further disproportionated.This results in a sulfide to sulfate accumulation ratio smallerthan 1.0.

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FIG. 2. Thiosulfate metabolism of strain SB164P1. (Top) Incubation without ferrihydrite. Results are means of two incubations. (Middle) Incubation with ferrihydrite. Results are means of two incubations. (Bottom) Cell counts from two parallel incubations with and without ferrihydrite. Note the logarithmic scale.

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FIG. 3. Elemental sulfur metabolism of strain SB164P1. Sulfur was added in excess. (Top) Incubation without ferrihydrite. Results are means of two incubations. (Middle) Incubation with ferrihydrite. Results are means of two incubations. FeS₂ represents pyrite sulfur. Note the different scales in the top and middle panels. (Bottom) Cell counts from two parallel incubations with and without ferrihydrite. Note the logarithmic scale.

With elemental sulfur, strain SB164P1 produced sulfide and sulfate at a ratio close to 3:1 at the beginning of the incubation(Fig. 3, top), in agreement with sulfur disproportionation:

<UP>4S<SUP>0</SUP> + 4H<SUB>2</SUB>O → SO</UP><SUB><UP>4</UP></SUB><SUP><UP>2−</UP></SUP><UP> + 3HS<SUP>−</SUP> + 5H<SUP>+</SUP></UP>

After 10 days, the ratio shifted to lower values. Removal of sulfide by degassing during sampling is again the most likelyexplanation. About 10 times as much sulfate was produced in thepresence of ferrihydrite (Fig. 3, middle). Free sulfide was notdetected. Sulfide accumulated as both FeS and pyrite, FeS₂. Pyritemay form through the following reaction (4):

<UP>FeS + S<SUP>0</SUP> → FeS<SUB>2</SUB></UP>

The final ratio of Fe(III) consumed to sulfate produced was 2:1, as expected for disproportionation in the presence of ferrihydrite(32).

Strain SB164P1 also grew by sulfite disproportionation in the absence of ferrihydrite (data not shown).

Growth by sulfur and thiosulfate disproportionation. Strain SB164P1 grew exponentially at the beginning of the incubation period except with elemental sulfur in ferrihydrite-freemedium (Fig. 2 and 3, bottom). With elemental sulfur and ferrihydrite,growth ceased after 7 days while sulfur disproportionation continuedthroughout the entire incubation period. However, the rate ofsulfur disproportionation decreased from day 7 until the end ofthe incubation. Growth cessation coincided with the depletionof Fe(III). The doubling times were 1 and 1.5 days with thiosulfatein the presence and absence of Fe(III), respectively, and 2 dayswith elemental sulfur and ferrihydrite in the medium. Culturesgrew without a lag phase when iron was present in the medium,while the iron-free thiosulfate cultures were delayed by 1 day.In the latter culture, growth ceased after 4 days, when 1.2 mMthiosulfate were consumed. The disproportionation of the remaining3 mM was not accompanied by growth. Thiosulfate-ferrihydrite culturesgrew exponentially at the beginning of the incubation. Afterwards,growth was linear with a slow increase throughout the rest ofthe incubation. The shift in the growth pattern was paralleledby the time courses of thiosulfate degradation and sulfate andferrous iron production.

Molybdate addition. Thiosulfate and elemental sulfur disproportionation were affected by the presence of molybdate. Both thiosulfate and elementalsulfur disproportionation were inhibited completely by 5 mM molybdate.At lower concentrations, the isolate responded differently whengrown with thiosulfate and with elemental sulfur. With thiosulfate,the inhibition was relieved at molybdate concentrations below500 µM. The lag phase in the presence of 500 µM molybdate wassignificantly longer (8 days) than in molybdate-free incubations(0 to 1 day). At molybdate concentrations lower than 50 µM, nodifference was observed compared with the lag phase in molybdate-freecultures. Cultures with elemental sulfur were more sensitive tomolybdate. Complete relief of the inhibition was observed onlyat molybdate concentrations below 5 µM.

G+C content of the DNA. The average G+C content of strain SB164P1 was 47.2 ± 0.2 mol%.

Phylogeny. Strain SB164P1 is a member of the delta subclass of the Proteobacteria. It belongs to a coherent group of microorganisms whichconsists of the recently described species Desulfocapsa thiozymogenes(12), Desulforhopalus vacuolatus (11), and Desulfofustis glycolicus(9) (Fig. 4). Within this phylogenetic cluster, strain SB164P1is more closely related to Desulfocapsa thiozymogenes than tothe other two organisms. This is indicated by the overall similarityvalues of 91.5, 90.7, and 89.8%, respectively, between the respective16S rRNA sequence pairs. This group forms a common line of descentwith members of the genus Desulfobulbus, with overall similarityvalues between strain SB164P1 and the four Desulfobulbus speciesranging from 86.6 to 88.7% while the corresponding values forall other representatives of the delta subclass of the Proteobacteriaare lower, i.e., between 80.2 and 84.6%. The monophyletic characterof the Desulfocapsa/Desulfobulbus group was supported in all treeinganalyses independent of the algorithms used for tree reconstructionand the procedure applied to exclude highly variable alignmentpositions. However, except for Desulfovibrio and related organisms,the relative branching order of the major subgroups within thedelta subclass of the Proteobacteria could not be determined unambiguously,resulting in a multifurcation of the respective branches in thetree (Fig. 4).

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FIG. 4. Phylogenetic tree based on 16S rRNA sequences showing the relationship between strain SB164P1 and its closest relatives as well as 62 other reference organisms of the delta subclass of the Proteobacteria. The triangles indicate groups of phylogenetically related species or genera: 1, Desulfobacter spp. plus Desulfobacterium, Desulfobacula, and Desulfosarcina spp.; 2, Syntrophobacter spp. plus Desulfoacinum and Desulforhabdus spp.; 3, Geobacter spp. plus Desulfuromonas, Desulfuromusa, and Pelobacter spp.; 4, Desulfovibrio spp. plus Desulfohalobium and Desulfomicrobium spp. The 16S rRNA sequence of E. coli was used as an outgroup reference. The scale bar represents the estimated number of base changes per nucleotide sequence position.

	DISCUSSION

Top Abstract Introduction Materials & Methods Results Discussion References

Strain SB164P1 was routinely cultured in marine medium containing elemental sulfur as a source of energy and reduction equivalentsand ferric iron as a sulfide scavenger. It grew exclusively bydisproportionation of elemental sulfur, thiosulfate, or sulfite.With thiosulfate and sulfite, a sulfide scavenger was not required,although growth with thiosulfate was stimulated by the presenceof ferrihydrite. Growth by elemental sulfur disproportionationhas recently been described for marine enrichment cultures (32)and the freshwater isolates Desulfocapsa thiozymogenes (12)and Desulfobulbus propionicus 1pr3 (18). Strain SB164P1, incontrast to Desulfocapsa thiozymogenes and Desulfobulbus propionicus,did not grow by sulfate reduction. It is thus the first obligatedisproportionator of sulfur compounds to be described. Like Desulfocapsathiozymogenes (12) and marine enrichment cultures (32), strainSB164P1 did not require organic carbon for growth. However, carbonfixation has not been directly demonstrated.

Growth yields and growth efficiencies with elemental sulfur and thiosulfate. Based on a ratio of cell dry weight to cell volume of 0.305 g/cm³ as reported for E. coli (21), an average dry weight of 1.8× 10¹³ g for individual cells of strain SB164P1 was calculated. Withelemental sulfur, approximately 0.24 g of dry cell mass was producedper mol of elemental sulfur disproportionated compared to the0.1 g reported by Janssen et al. (12) for Desulfocapsa thiozymogenes.With thiosulfate alone, the growth yield at the end of the exponentialgrowth phase was 0.94 g (dry weight) mol of thiosulfate¹. This is less than half the growth yield reported for Desulfocapsathiozymogenes (12) and Desulfovibrio sulfodismutans (2),which, however, were both grown with acetate as the carbon source.In the presence of ferric iron, the growth yield was 1.3 g (dryweight) mol of thiosulfate¹. Based on the growth yields given above, we can estimate thegrowth efficiency of strain SB164P1 with thiosulfate or elementalsulfur. Assuming that (i) strain SB164P1 grew autotrophicallyand CO₂ assimilation produced glucose or organic carbon with thesame chemical composition and formation energy as those of glucoseand that (ii) thiosulfate or elemental sulfur was the only energyand electron source, we calculate a carbon yield of 3.5 g of Cmol of thiosulfate¹. The isolate produced 0.94 g (dry weight) mol of thiosulfate¹, corresponding to 0.38 g of C (using a 40% [by weight] C contentof glucose), or 10.7% of the theoretically possible amount ofcarbon. In the presence of elemental sulfur, a growth efficiencyof approximately 3% can be determined. These values are in therange of thermodynamic efficiency values of chemolithoautotrophicsulfide-oxidizing bacteria compiled by Nelson and Hagen (22).

Effect of molybdate. The inhibitory effect of molybdate on sulfate reduction is well understood (31). By formation of adenosine-5-phosphomolybdate,molybdate depletes the internal ATP pool of the cell. Interestingly,molybdate also inhibited elemental sulfur and thiosulfate disproportionation.Recently, Krämer and Cypionka (15) and Fuseler and Cypionka(10) proposed that ATP synthesis by disproportionation resultsfrom the inversion of the initial steps of sulfate reduction,including the formation of adenosine-5-phosphosulfate throughsubstrate-level phosphorylation. Molybdate may interfere withthe formation of APS and consequently may inhibit disproportionationreactions. We have no explanation why sulfur disproportionationwas more sensitive to molybdate than was thiosulfate disproportionation.

Ecological considerations. Strain SB164P1 is the first marine bacterium found to be able to thrive by disproportionation of intermediately oxidized inorganicsulfur compounds alone. Since it was isolated from the fifth stepin a series of 10-fold dilutions, it appears to be abundant inthe sediment. Up to 10⁶ cells per cm³ of sulfur-disproportionating bacteria have previously been countedin marine sediments with a medium similar to that used in thepresent study (32). Most-probable-number counts of sulfate reducersin sediments from Arcachon Bay range from 10⁶ to 10⁷ cells per cm³ (35). The occurrence of obligate sulfur disproportionatorsin numbers comparable to those of sulfate reducers is a strongindication that disproportionation is a common way of living inthese environments. This is further accentuated when the relativelylow growth yield of the process is considered. Jørgensen and Bak(13) argued on the basis of most-probable-number counts thatthiosulfate disproportionation in marine environments is mainlya cometabolism executed by sulfate reducers but not a major typeof metabolism. These authors, however, did not include a sulfidescavenger in their medium. In natural sediments, the scavengingof hydrogen sulfide by iron oxides is a very important process,which often maintains sulfide concentrations at low levels inspite of intense sulfide production through sulfate reduction.We conclude from the results of our studies that the presenceof a sulfide scavenger is essential for counting, enrichment,and isolation of SB164P1-like bacteria and, consequently, thatlife by disproportionation is more common than has so far beenassumed.

Phylogenetic position. The closest relative of strain SB164P1 is Desulfocapsa thiozymogenes. Desulforhopalus vacuolatus and Desulfofustis glycolicusare slightly more distantly related (Fig. 4). From the phylogeneticpoint of view, the dissimilarity value of 8.5% between the 16SrRNA sequences of Desulfocapsa thiozymogenes and strain SB164P1would allow us to propose the taxonomic rank of a new genus forthe latter organism. However, considering the very similar phenotypicand genotypic properties, including the G+C content of the genomicDNA (47.2% versus 50.7%), we favour the inclusion of strain SB164P1into the genus Desulfocapsa and suggest the species name D. sulfoexigens.

Description of Desulfocapsa sulfoexigens sp. nov. Desulfocapsa sulfoexigens (sul.fo.ex'i.gens. L. n. sulfurum, sulfur; L. v. exigo, to demand; M. L. part. adj. sulfoexigens,demanding sulfur for growth). Gram-negative cells that are elongatedwith slightly pointed ends, 0.5 µm wide and 2 to 4 µm long. Multiplicationoccurs by binary fission. Under most conditions, only a few cellsare motile. Spores are not produced. Growth occurs in mineralmedium without vitamins or organic carbon sources with bicarbonateas the sole carbon source. Disproportionation of elemental sulfur,sulfite, and thiosulfate to sulfide and sulfate occurs. Growthby sulfur disproportionation occurs only in the presence of ahydrogen sulfide-scavenging agent, like ferric iron. Growth bydisproportionation of thiosulfate occurs with and without iron.No growth occurs by sulfate reduction. The pH range is from 6.0to 8.2 with an optimum of 6.7 to 7.3. The temperature range is4 to 35°C with an optimum of 30°C. The habitat is oxidized marinesurface sediment. The type strain was isolated from marine sedimentcovered by the eelgrass, Zostera noltii, in the basin of Arcachon,France.

The G+C content of the genomic DNA is 47.2 ± 0.2 mol%.

The type strain is strain SB164P1, DSM 10523, deposited with the Deutsche Sammlung von Mikroorganismen und Zellkulturen, Braunschweig,Germany.

	ACKNOWLEDGMENTS

K.F. is indebted to Niels Peter Revsbech for support. Sonja Fleissner and Swantje Fleischer are acknowledged for technicalassistance. We thank three anonymous reviewers for constructivecriticism of the manuscript.

The study was financed by a European Union project on Coastal Lagoon Eutrophication and Anaerobic Processes (C.L.AE.N) (contractEV5V-CT92-008), by the Danish Committee on Biotechnology, by theBundesministerium für Bildung, Wissenschaft, Forschung und Technologie(contract 21/03111221), and by the Max Planck Society.

	FOOTNOTES

^* Corresponding author. Mailing address: Department of Microbial Ecology, Institute of Biological Sciences, University of Aarhus,Ny Munkegade, DK-8000 Aarhus, Denmark. Phone: 45 89 423241. Fax:45 86 129171. E-mail: Kai{at}bio.aau.dk.

REFERENCES

Top
Abstract
Introduction
Materials & Methods
Results
Discussion
References

1. Bak, F. 1993. Fermentation of inorganic sulfur compounds by sulfate-reducing bacteria, p. 75-78. In R. Guerrero, and C. Pedrós-Alió (ed.), Trends in microbial ecology. Spanish Society for Microbiology, Barcelona.

2. Bak, F., and H. Cypionka. 1987. A novel type of energy metabolism involving fermentation of inorganic sulphur compounds. Nature 326:891-892.

3. Bak, F., and N. Pfennig. 1987. Chemolithotrophic growth of Desulfovibrio sulfodismutans sp. nov. by disproportionation of inorganic sulfur compounds. Arch. Microbiol. 147:184-189.

4. Berner, R. A. 1970. Sedimentary pyrite formation. Am. J. Sci. 268:1-23.

5. Cline, J. D. 1969. Spectrophotometric determination of hydrogen sulfide in natural waters. Limnol. Oceanogr. 14:454-458.

6. Felsenstein, J. 1993. . PHYLIP (Phylogeny Inference Package). University of Washington, Seattle.

7. Finster, K., W. Liesack, and B. J. Tindall. 1997. Desulfospira joergensenii, gen. nov., sp. nov., a new sulfate-reducing bacterium isolated from marine surface mud. Syst. Appl. Microbiol. 20:201-208.

8. Fossing, H., and B. B. Jørgensen. 1989. Measurements of bacterial sulfate reduction in sediments: evaluation of a single-step chromium reduction method. Biogeochemistry 8:205-222.

9. Friedrich, M., N. Springer, W. Ludwig, and B. Schink. 1996. Phylogenetic positions of Desulfofustis glycolicus gen. nov., sp. nov., and Syntrophobotulus glycolicus gen. nov., sp. nov., two new strict anaerobes growing with glycolic acid. Int. J. Syst. Bacteriol. 46:1065-1069[Abstract/Free Full Text].

10. Fueseler, K., and H. Cypionka. 1995. Elemental sulfur as an intermediate of sulfide oxidation with oxygen by Desulfobulbus propionicus. Arch. Microbiol. 164:104-109.

11. Isaksen, M. F., and A. Teske. 1996. Desulforhopalus vacuolatus gen. nov., sp. nov., a new moderately psychrophilic sulfate-reducing bacterium with gas vacuoles isolated from a temperate estuary. Arch. Microbiol. 166:160-168.

12. Janssen, P. H., A. Schuhmann, F. Bak, and W. Liesack. 1996. Disproportionation of inorganic sulfur compounds by the sulfate-reducing bacterium Desulfocapsa thiozymogenes gen. nov., sp. nov. Arch. Microbiol. 166:184-192.

13. Jørgensen, B. B. 1990. A thiosulfate shunt in the sulfur cycle of marine sediments. Science 249:152-154[Abstract/Free Full Text].

14. Jørgensen, B. B., and F. Bak. 1991. Pathways and microbiology of thiosulfate transformations, and sulfate reduction in a marine sediment (Kattegat, Denmark). Appl. Environ. Microbiol. 57:847-856[Abstract/Free Full Text].

15. Krämer, M., and H. Cypionka. 1989. Sulfate formation via ATP sulfurylase in thiosulfate- and sulfite-disproportionating bacteria. Arch. Microbiol. 151:232-237.

16. Liesack, W., and K. Finster. 1994. Phylogenetic analysis of five strains of gram-negative, obligately anaerobic, sulfur-reducing bacteria and description of Desulfuromusa gen. nov., including Desulfuromusa kysingii sp. nov., Desulfuromusa bakii sp. nov., and Desulfuromusa succinoxidans sp. nov. Int. J. Syst. Bacteriol. 44:753-758[Abstract/Free Full Text].

17. Lord, C. J., III. 1980. . The chemistry and cycling of iron, manganese, and sulfur in salt marsh sediments. Ph.D. dissertation. University of Delaware.

18. Lovley, D. R., and E. J. P. Phillips. 1994. Novel processes for anaerobic sulfate production from elemental sulfur by sulfate-reducing bacteria. Appl. Environ. Microbiol. 60:2394-2399[Abstract/Free Full Text].

19. Maidak, B. L., G. J. Olsen, N. Larsen, R. Overbeek, M. J. McCaughey, and C. R. Woese. 1996. The ribosomal database project (RDP). Nucleic Acids Res. 24:82-85[Abstract/Free Full Text].

20. Mesbah, M., U. Premachandran, and W. B. Whitman. 1989. Precise measurements of the G+C content of deoxyribonucleic acid by high-performance liquid chromatography. Int. J. Syst. Bacteriol. 39:159-167.

21. Neidhardt, F. C. 1987. Chemical composition of Escherichia coli, p. 3-6. In F. C. Neidhardt, J. L. Ingraham, K. B. Low, B. Magasanik, M. Schaechter, and H. E. Umbarger (ed.), Escherichia coli and Salmonella typhimurium: cellular and molecular biology, vol. 1. American Society for Microbiology, Washington, D.C.

22. Nelson, D., and K. D. Hagen. 1995. Physiology and biogeochemistry of symbiontic and free-living chemoautotrophic sulfur bacteria. Am. Zool. 35:91-101.

23. Pfennig, N. 1978. Rhodocyclus purpureus gen. nov. and sp. nov., a ring-shaped, vitamin B₁₂-requiring member of the family Rhodospirillaceae. Int. J. Syst. Bacteriol. 28:283-288[Abstract/Free Full Text].

24. Pyzik, A. J., and S. E. Sommer. 1981. Sedimentary iron monosulfides: kinetics and mechanism of formation. Geochim. Cosmochim. Acta 45:687-698.

25. Rodriguez-Tom, P., P. J. Stoehr, G. N. Cameron, and T. P. Flores. 1996. The European Bioinformatics Institute (EBI) databases. Nucleic Acids Res. 24:6-12[Abstract/Free Full Text].

26. Saitou, N., and M. Nei. 1987. The neighbor-joining method: a new method for reconstructing phylogenetic trees. Mol. Biol. Evol. 4:406-425[Abstract].

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28. Stookey, L. L. 1970. Ferrozine $---$ a new spectrophotometric reagent for iron. Anal. Chem. 42:779-781.

29. Strunk, O., and W. Ludwig. 1996. . ARB. Technische Universität München, Munich, Germany.

30. Tamaoka, J., and K. Komagato. 1984. Determination of DNA base composition by reverse-phase high performance liquid chromatography. FEMS Microbiol. Lett. 25:125-128.

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33. Van de Peer, Y., S. Nicolaï, P. De Rijk, and R. De Wachter. 1996. Database on the structure of small ribosomal subunit RNA. Nucleic Acids Res. 24:86-91[Abstract/Free Full Text].

34. Van de Peer, Y., S. Chapelle, and R. De Wachter. 1996. A quantitative map of nucleotide substitution rates in bacterial rRNA. Nucleic Acids Res. 24:3381-3391[Abstract/Free Full Text].

35. Welsh, D. T., S. Bourguès, R. De Wit, and R. A. Herbert. 1996. Seasonal variations in rates of heterotrophic nitrogen fixation (acetylene reduction) in Zostera noltii meadows and uncolonised sediments of the Bassin d'Arcachon, south-west France. Hydrobiologia 329:161-174.

36. Widdel, F., and T. A. Hansen. 1992. The dissimilatory sulfate- and sulfur-reducing bacteria, p. 583-624. In A. Balows, H. G. Trüper, M. Dworkin, W. Harder, and K.-H. Schleifer (ed.), The prokaryotes: a handbook on the biology of bacteria. Ecophysiology, isolation, identification applications, 2nd ed. Springer Verlag, New York, N.Y.

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1.	Bak, F. 1993. Fermentation of inorganic sulfur compounds by sulfate-reducing bacteria, p. 75-78. In R. Guerrero, and C. Pedrós-Alió (ed.), Trends in microbial ecology. Spanish Society for Microbiology, Barcelona.
2.	Bak, F., and H. Cypionka. 1987. A novel type of energy metabolism involving fermentation of inorganic sulphur compounds. Nature 326:891-892.
3.	Bak, F., and N. Pfennig. 1987. Chemolithotrophic growth of Desulfovibrio sulfodismutans sp. nov. by disproportionation of inorganic sulfur compounds. Arch. Microbiol. 147:184-189.
4.	Berner, R. A. 1970. Sedimentary pyrite formation. Am. J. Sci. 268:1-23.
5.	Cline, J. D. 1969. Spectrophotometric determination of hydrogen sulfide in natural waters. Limnol. Oceanogr. 14:454-458.
6.	Felsenstein, J. 1993. . PHYLIP (Phylogeny Inference Package). University of Washington, Seattle.
7.	Finster, K., W. Liesack, and B. J. Tindall. 1997. Desulfospira joergensenii, gen. nov., sp. nov., a new sulfate-reducing bacterium isolated from marine surface mud. Syst. Appl. Microbiol. 20:201-208.
8.	Fossing, H., and B. B. Jørgensen. 1989. Measurements of bacterial sulfate reduction in sediments: evaluation of a single-step chromium reduction method. Biogeochemistry 8:205-222.
9.	Friedrich, M., N. Springer, W. Ludwig, and B. Schink. 1996. Phylogenetic positions of Desulfofustis glycolicus gen. nov., sp. nov., and Syntrophobotulus glycolicus gen. nov., sp. nov., two new strict anaerobes growing with glycolic acid. Int. J. Syst. Bacteriol. 46:1065-1069[Abstract/Free Full Text].
10.	Fueseler, K., and H. Cypionka. 1995. Elemental sulfur as an intermediate of sulfide oxidation with oxygen by Desulfobulbus propionicus. Arch. Microbiol. 164:104-109.
11.	Isaksen, M. F., and A. Teske. 1996. Desulforhopalus vacuolatus gen. nov., sp. nov., a new moderately psychrophilic sulfate-reducing bacterium with gas vacuoles isolated from a temperate estuary. Arch. Microbiol. 166:160-168.
12.	Janssen, P. H., A. Schuhmann, F. Bak, and W. Liesack. 1996. Disproportionation of inorganic sulfur compounds by the sulfate-reducing bacterium Desulfocapsa thiozymogenes gen. nov., sp. nov. Arch. Microbiol. 166:184-192.
13.	Jørgensen, B. B. 1990. A thiosulfate shunt in the sulfur cycle of marine sediments. Science 249:152-154[Abstract/Free Full Text].
14.	Jørgensen, B. B., and F. Bak. 1991. Pathways and microbiology of thiosulfate transformations, and sulfate reduction in a marine sediment (Kattegat, Denmark). Appl. Environ. Microbiol. 57:847-856[Abstract/Free Full Text].
15.	Krämer, M., and H. Cypionka. 1989. Sulfate formation via ATP sulfurylase in thiosulfate- and sulfite-disproportionating bacteria. Arch. Microbiol. 151:232-237.
16.	Liesack, W., and K. Finster. 1994. Phylogenetic analysis of five strains of gram-negative, obligately anaerobic, sulfur-reducing bacteria and description of Desulfuromusa gen. nov., including Desulfuromusa kysingii sp. nov., Desulfuromusa bakii sp. nov., and Desulfuromusa succinoxidans sp. nov. Int. J. Syst. Bacteriol. 44:753-758[Abstract/Free Full Text].
17.	Lord, C. J., III. 1980. . The chemistry and cycling of iron, manganese, and sulfur in salt marsh sediments. Ph.D. dissertation. University of Delaware.
18.	Lovley, D. R., and E. J. P. Phillips. 1994. Novel processes for anaerobic sulfate production from elemental sulfur by sulfate-reducing bacteria. Appl. Environ. Microbiol. 60:2394-2399[Abstract/Free Full Text].
19.	Maidak, B. L., G. J. Olsen, N. Larsen, R. Overbeek, M. J. McCaughey, and C. R. Woese. 1996. The ribosomal database project (RDP). Nucleic Acids Res. 24:82-85[Abstract/Free Full Text].
20.	Mesbah, M., U. Premachandran, and W. B. Whitman. 1989. Precise measurements of the G+C content of deoxyribonucleic acid by high-performance liquid chromatography. Int. J. Syst. Bacteriol. 39:159-167.
21.	Neidhardt, F. C. 1987. Chemical composition of Escherichia coli, p. 3-6. In F. C. Neidhardt, J. L. Ingraham, K. B. Low, B. Magasanik, M. Schaechter, and H. E. Umbarger (ed.), Escherichia coli and Salmonella typhimurium: cellular and molecular biology, vol. 1. American Society for Microbiology, Washington, D.C.
22.	Nelson, D., and K. D. Hagen. 1995. Physiology and biogeochemistry of symbiontic and free-living chemoautotrophic sulfur bacteria. Am. Zool. 35:91-101.
23.	Pfennig, N. 1978. Rhodocyclus purpureus gen. nov. and sp. nov., a ring-shaped, vitamin B₁₂-requiring member of the family Rhodospirillaceae. Int. J. Syst. Bacteriol. 28:283-288[Abstract/Free Full Text].
24.	Pyzik, A. J., and S. E. Sommer. 1981. Sedimentary iron monosulfides: kinetics and mechanism of formation. Geochim. Cosmochim. Acta 45:687-698.
25.	Rodriguez-Tom, P., P. J. Stoehr, G. N. Cameron, and T. P. Flores. 1996. The European Bioinformatics Institute (EBI) databases. Nucleic Acids Res. 24:6-12[Abstract/Free Full Text].
26.	Saitou, N., and M. Nei. 1987. The neighbor-joining method: a new method for reconstructing phylogenetic trees. Mol. Biol. Evol. 4:406-425[Abstract].
27.	Singleton, R., Jr. 1993. The sulfate-reducing bacteria: an overview, p. 1-20. In J. M. Odom, and R. Sinleton, Jr. (ed.), The sulfate-reducing bacteria: contemporary perspectives. Springer Verlag, New York, N.Y.
28.	Stookey, L. L. 1970. Ferrozine $---$ a new spectrophotometric reagent for iron. Anal. Chem. 42:779-781.
29.	Strunk, O., and W. Ludwig. 1996. . ARB. Technische Universität München, Munich, Germany.
30.	Tamaoka, J., and K. Komagato. 1984. Determination of DNA base composition by reverse-phase high performance liquid chromatography. FEMS Microbiol. Lett. 25:125-128.
31.	Taylor, B. F., and R. S. Oremland. 1979. Depletion of adenosine triphosphate in Desulfovibrio by oxyanions of group VI elements. Curr. Microbiol. 3:101-103.
32.	Thamdrup, B., K. Finster, J. W. Hansen, and F. Bak. 1993. Bacterial disproportionation of elemental sulfur coupled to chemical reduction of iron or manganese. Appl. Environ. Microbiol. 59:101-108[Abstract/Free Full Text].
33.	Van de Peer, Y., S. Nicolaï, P. De Rijk, and R. De Wachter. 1996. Database on the structure of small ribosomal subunit RNA. Nucleic Acids Res. 24:86-91[Abstract/Free Full Text].
34.	Van de Peer, Y., S. Chapelle, and R. De Wachter. 1996. A quantitative map of nucleotide substitution rates in bacterial rRNA. Nucleic Acids Res. 24:3381-3391[Abstract/Free Full Text].
35.	Welsh, D. T., S. Bourguès, R. De Wit, and R. A. Herbert. 1996. Seasonal variations in rates of heterotrophic nitrogen fixation (acetylene reduction) in Zostera noltii meadows and uncolonised sediments of the Bassin d'Arcachon, south-west France. Hydrobiologia 329:161-174.
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