Metabolic Microenvironmental Control by Photosynthetic Biofilms under Changing Macroenvironmental Temperature and pH Conditions

Ex situ microelectrode experiments, using cyanobacterial biofilmsfrom karst water creeks, were conducted under various pH, temperature,and constant-alkalinity conditions to investigate the effectsof changing environmental parameters on cyanobacterial photosynthesis-inducedcalcification. Microenvironmental chemical conditions aroundcalcifying sites were controlled by metabolic activity overa wide range of photosynthesis and respiration rates, with littleinfluence from overlying water conditions. Regardless of overlyingwater pH levels (from 7.8 to 8.9), pH at the biofilm surfacewas approximately 9.4 in the light and 7.8 in the dark. Thesame trend was observed at various temperatures (4°C and17°C). Biological processes control the calcium carbonatesaturation state ( ${Omega}$ ) in these and similar systems and are ableto maintain ${Omega}$ at approximately constant levels over relativelywide environmental fluctuations. Temperature did, however, havean effect on calcification rate. Calcium flux in this systemis limited by its diffusion coefficient, resulting in a highercalcium flux (calcification and dissolution) at higher temperatures,despite the constant, biologically mediated pH. The abilityof biological systems to mitigate the effects of environmentalperturbation is an important factor that must be consideredwhen attempting to predict the effects of increased atmosphericpartial CO₂ pressure on processes such as calcification andin interpreting microfossils in the fossil record.

INTRODUCTION

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INTRODUCTION

Calcifying biofilms have contributed significantly to the formationof carbonate sediments throughout earth history (8, 24, 27).These sediments are known as microbialites and, if macroscopicallylaminated, stromatolites. Their temporal and geographic distributionshave been used to infer the impacts of metazoan evolution (4,33) and changes in ocean chemistry (2, 13, 26). Many stromatolitesare formed in the photic zone of shallow-water environmentsby thin cyanobacterial biofilms, rather than by thick microbialmats, which tend to produce more irregular fabrics.

The principal mechanisms involved in stromatolite formationare (i) heterogeneous crystal nucleation at acidic extracellularpolymeric substances (1, 19, 22, 32) and (ii) increases in theCa²⁺ x CO₃^2– ion activity product (IAP), which may beinduced by microbial activity (e.g., photosynthesis, sulfatereduction) and/or external physicochemical factors (e.g., evaporation,CO₂ degassing) (5, 21, 25, 31). Lamination of microbialite depositsmay result from a number of factors, including seasonally inducedchanges to calcification processes caused by changes in biofilmcomposition and calcium carbonate mineral supersaturation. Somecalcifying biofilms exhibit fabrics containing cyanobacterialCaCO₃ tubes which can be preserved as microfossils known asGirvanella or Cayeuxia (25, 34). These cyanobacterial tubeshave been attributed to photosynthesis-induced pH microgradientsunder conditions of low dissolved-inorganic-carbon (DIC) levelsand, consequently, low bulk-phase pH buffering (2). Specifically,the impact of a given amount of DIC removal on changes in CaCO₃supersaturation should, theoretically, increase with decreasingDIC concentrations and initial pHs at a given IAP. Other factorsthat have been discussed in this context are temperature andCaCO₃ mineral supersaturation (14, 26).

Changing environmental conditions (e.g., temperature and pH)may affect biological activity and calcification. Precipitationand dissolution may be affected by warming-induced changes,as brought about by global climate change, and/or by changesto overlying water pH, brought about by changes to atmosphericpartial CO₂ pressure (pCO₂), in rainfall patterns or trophicstate. Understanding the effects of changing environmental conditionson calcification and dissolution processes is important, bothto the prediction of the effects of global climate change andto the interpretation of the paleo record.

The influence of diurnal temperature changes on hydrochemistryin karst water creeks has been investigated previously (12),and from these changes, inferences regarding precipitation processeswere made. Drysdale et al. (12) reported a strong diurnal patternto hydrochemistry and calcite saturation in what they consideredto be a karst system with solely inorganic precipitation. Theyreported that diurnal fluctuations in temperature significantlyaltered the creek's carbonate chemistry and led to changes inrates and reach of precipitation. Changing environmental factorssuch as temperature also influence biotic processes such asphotosynthesis and respiration. In karst systems such as thoseinvestigated here, in which biofilms play a significant rolein controlling the chemical conditions at the sites of mineralnucleation (6), fluctuations in abiotic conditions may alsoaffect stromatolite formation processes. These effects may bemanifested as changes to rates of precipitation/dissolutionor as mitigating effects of the biofilm against bulk water changes.

Despite the importance of understanding these processes to bothprojections of biological response to climate change and topaleoenvironmental interpretations, experimental studies oncalcification in cyanobacterial communities are rare (e.g. (11,18), and the specific relationship between various environmentalfactors, such as temperature and pH conditions, on photosynthesis-inducedcalcification of cyanobacterial biofilms have not, thus far,been investigated. Temperature changes may alter the rate ofabiotic degassing and the rate of biological processes and,hence, precipitation. Changes to bulk water pH will alter thebulk water CaCO₃ saturation state but may not have such a greateffect at the stromatolite surface, if biological processesare maintained. In this study, the results of ex situ microelectrodeexperimental studies using cyanobacterial biofilms from karstwater creeks under various bulk water conditions are presentedand discussed with respect to their implications for predictionof climate-induced changes to calcification and to interpretationof the paleoenvironmental record.

MATERIALS AND METHODS

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MATERIALS AND METHODS

Samples and sample collection.
Samples were collected from the Deinschwanger Bach, as describedin reference 6. The Deinschwanger Bach is located near Nuremberg(49°23'N, 11°28'E) in southern Germany and has beenused for previous studies on cyanobacterial biofilm calcification.It is described in more detail in reference 3 and shows activelaminar stromatolite formation up to 1.8 mm/year.

Samples were collected from two distinct, active tufa-formingsites for pH manipulation experiments. Site 1 comprised a smallstromatolite cascade 65 m downstream from a minor spring, whichentered the creek's main flow approximately 40 m after the cascade.At this site, the water was approximately 1- to 5-cm deep andexhibited a fast flow rate (approximately 40 cm s^–1) and,consequently, a small diffusive boundary layer (DBL; approximately200 to 300 µm). Stromatolite at site 1 was laminated andseveral centimeters thick. Site 2 was a well-illuminated sectionof the lower creek, approximately 20-cm deep, and had a slowerflow rate (approximately 10 cm s^–1) than, but similarDBL (approximately 200 µm) to, site 1. Site 2 exhibitedthin (up to 1 mm) fragile carbonate crusts. Samples from site2 only were used for temperature manipulation experiments. Sampleswere removed from the creek with a motorized core-drilling device(modified Stihl chainsaw) and stored in ambient creek waterin coolers until they were returned to the laboratory, within24 h. Creek water samples for the experiments were collectedwithout air bubbles in 20-liter plastic containers and storedat 4°C in the dark until use.

Laboratory setup.
Once in the laboratory, samples were stored in temperature-controlled,aerated, recirculating aquariums (total volume, approximately30 liters) containing creek water. Phototrophic community compositiondid not change during transport and incubation (6). Sampleswere removed to flow cells connected to the same recirculatingwater supply for measurements during experiments run at ambienttemperature and experimentally altered temperatures. Experimentalflow rates were approximately 0.03 liter s^–1. A reservoirof creek water separate from the main holding aquarium's supplywas used for pH-manipulated experiments. pH was manipulatedby the addition of CO_2, in bottled Vilsa (Germany) mineral water,to lower pH or by aerating the reservoir with CO₂-free air (airscrubbed in NaOH) to raise it. Vilsa water (http://www.pmgeiser.ch/mineral/index.php?func=dispes&parval=54)contains only trace mineral components. Amounts added to 30-literexperimental setups were <20 ml and were deemed to have hadno effect on overall water chemistry. During pH adjustments,pH was monitored continuously with an MA130 ion detector (MettlerToledo, Columbus, OH). Rates of CO₂ addition or removal wereadjusted to maintain the desired pH.

Microelectrode measurements comprised three sets. The firstconsisted of measurements of O₂, pH, and Ca²⁺ concentrationprofiles on samples held at ambient creek conditions (temperature,10°C; pH 8.4). The second comprised measurements of concentrationgradients of the same ions in the sample at a pH raised to 8.9and at a pH lowered to lowered 7.8. The final set of measurements,involving the same ions as those in the previous experiments,were on temperature-adjusted samples from the DeinschwangerBach collected 12 months later. In this set of measurements,temperature was raised from the ambient 10°C to 17°Cand lowered to 4°C.

Microelectrode measurements and calculations.
Liquid membrane Ca²⁺ and pH sensors were prepared and calibratedas described previously (9, 10). Fast-responding O₂ microsensorswere also prepared as described previously (23). All electrodeswere placed manually at the stromatolite surface while viewingthe sample through a dissection microscope. The stromatolitesurface was then set at 0 cm. All measurements were made atmeasured distances above the stromatolite. Negative distances,therefore, indicate that the sensor is above the stromatolite/waterinterface. Profiling was automated after electrodes were positionedat the stromatolite surface. Sensors were connected to a micromanipulator,which was fixed to a motorized stage (VT-150; Micos, Eschbach,Germany) and allowed reproducible positioning of the sensortip with 1-µm precision. The microelectrodes were connectedto a picoammeter (O₂ electrode) or a millivoltmeter, and themeter output was collected by a data acquisition device (NIDaqPad-6015; National Instruments, Austin, TX). After positioningat the surface, profiling was performed automatically. Motorcontrol and data acquisition were performed with a computerand custom-written software (µ-Profiler; provided by LubosPolerecky). All profiles were corrected for offset to ion levelsin the bulk liquid; oxygen concentrations in the bulk liquidwere determined from literature values at experimental temperatures(salinity = 0 ppt), pH as described above, Ca²⁺ by inductivelycoupled plasma-optical emission spectroscopy (Perkin Elmer Optima3300 DV) and DIC by CO₂ coulometer (UIC Coulometrics, Joliet,IL).

Interfacial fluxes (J) were calculated from the concentrationprofiles by using Fick's first law: J = D x (dc/dx), where Dis the diffusion coefficient and dc/dx is the interfacial concentrationgradient, i.e., the concentration gradient in the mass boundarylayer directly adjacent to the stromatolite surface.

Calcite saturation is given by the saturation state omega ( ${Omega}$ ): ${Omega}$ = Ca²⁺ x CO₃^2–/K_c_alcite, where the numerator is the IAPand the denominator the solubility product K_calcite as givenby reference 20. Carbonate concentrations were determined frombulk water DIC and pH microprofiles. For the calculation of ${Omega}$ _calcite, activities were estimated by applying the activitycoefficients of water used in experiments as delivered fromthe PHREEQC program (0.686 for Ca²⁺ and CO₃^2–).

Diffusion coefficients.
The diffusion coefficients of O₂ and Ca²⁺ are literature-derivedvalues corrected for temperature and type of counter ion (7,16). Diffusion coefficients for oxygen that we used were asfollows: at 4°C, 1.28 x 10^–9 m² s^–1; at 10°C,1.57 x 10^–9 m² s^–1; and at 17°C, 1.934 x 10^–9m² s^–1. Diffusion coefficients that we used for Ca²⁺ withHCO₃^– as counter ion were as follows: at 4°C, 0.546x 10^–9 m² s^–1; at 10°C, 0.67 x 10^–9 m²s^–1; and at 17°C, 0.827 x 10^–9 m² s^–1.

Statistical analyses.
Analysis of variance was used to test for the effects of treatmenton chemical flux rates. Tests were conducted separately foreach chemical flux (Ca²⁺, O₂) and at each light phase (lightor dark) for each pH and temperature treatment. Homogeneityof variances was checked visually by examining residual plots.Data that did not meet this assumption of analysis of variancewere log transformed. Significant factors were compared usingTukey's honestly significant difference post hoc tests. Allstatistical tests were performed at an ${alpha}$ of 0.05, with F_2,5,using the statistical software SPSS version 10.

RESULTS

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RESULTS

Steady-state microsensor profiles were obtained for all treatmentsand displayed typical variation (see Fig. S1 in the supplementalmaterial). The steady state was reached very quickly (<10min) both after switching on and turning off the lights. Calciumfluxes have been shown previously to represent CaCO₃ dissolutionand precipitation in these stromatolites (6, 29). Biofilms wereable to control microenvironmental conditions under all experimentalconditions. Changing overlying water pH and temperature hadlittle effect on biofilm ${Omega}$ state. Temperature did, however, affectcalcium fluxes by influencing calcium ion diffusion coefficients.

pH manipulations.
Concentration profiles of O₂, pH, and Ca²⁺ were measured onall samples (Fig. 1) at experimentally manipulated pHs. It shouldbe noted that slight discrepancies in the observed height ofthe DBL and bulk water concentrations of chemical species measuredare evident in the results presented. The profiles presentedare averages of two positions on each sample, and these variationsindicate both the heterogeneity within the samples and the difficultyin aligning the various sensors to exactly the same positionon each sample. The profiles do, however, show consistent results.

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FIG. 1. pH, O₂, and Ca²⁺ profiles in the light and dark at the three experimental pHs for site 1 and site 2.

In all samples, photosynthesis increased O₂ concentration atthe stromatolite surface in the light, causing a concomitantincrease in pH and a decrease in Ca²⁺ ion concentration. Inthe dark, respiration resulted in a decrease in O₂ concentrationand often a small decrease in pH and increase in Ca²⁺ concentration.In the high-pH (8.9) treatment, however, a decrease in calciumion concentration was seen in both light and dark incubations.

Flux rates of O₂ and Ca²⁺ and pH changes ( ${Delta}$ pH) observed are presentedin Table 1. In all treatments, pHs approached the same values(9.2 to 9.5) in light incubations, although there were somesmall differences, largely between sites. The fact that similarmaximum pH values were reached in all treatments leads to different ${Delta}$ pH values. Higher ${Delta}$ pH values occurred in the low-pH (7.8) treatmentthan in the high-pH (8.9) treatment in the light. In the dark,the opposite trend was observed because pHs were always around7.8, regardless of the overlying water pH. The highest fluxesof O₂ from the biofilm were seen in the samples at ambient pH(8.4) at both sites (statistically significant only at site2; P < 0.05), as were the highest O₂ fluxes to the biofilmsurface during dark incubations, although these were not significantlydifferent (P > 0.05).

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TABLE 1. Fluxes of oxygen and calcium (mean ± standard error; n = 2) and pH changes at biofilm surfaces measured in samples from the Deinschwanger Bach^a

Calcium fluxes were very similar under all treatments at bothsites but did display some minor variations (Table 1). At site1, the light flux was highest at pH 8.9 but was not significantlydifferent from that at 8.4 or 7.8 (P > 0.05). In the dark,there was a significant difference between the fluxes (P <0.05). The lowest absolute flux was seen at pH 7.8, while theflux at pH 8.9 was actually toward the biofilm, indicating precipitation.At site 2, a different pattern was seen. Dark fluxes were stillmuch lower than light fluxes and, except in the high-pH (8.9)treatment, were all away from the biofilm surface. In the light,the highest flux (P < 0.05) was observed in the lowest-pH(7.8) treatment. The data clearly show a biologically controlled,diurnal pattern of calcium precipitation.

Calcite saturation state microprofiles (Fig. 2), calculatedfrom bulk water DIC, pH, and Ca²⁺ microprofiles, demonstratethe degree to which ${Omega}$ _calcite is controlled by the carbonate system. ${Omega}$ _calcite profiles mirrored pH profiles and indicated that thewater was supersaturated with respect to calcite under all experimentalconditions. At both sites, illumination caused a photosyntheticallyinduced increase in ${Omega}$ _calcite. In turn, a clear decrease in ${Omega}$ _calcitewas evident at both sites without illumination. Despite thesemetabolically induced changes in ${Omega}$ _calcite, no relationship existedbetween the rate of calcification (derived from Ca²⁺ fluxes)and the degree of supersaturation.

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FIG. 2. Omega value profiles, calculated from Ca²⁺ profiles and alkalinity levels, for sites 1 and 2 at each experimental pH.

Temperature manipulations.
The second experiment comprised manipulations of temperature,in order to investigate its effects on calcification. In lightof the heterogeneity in each sample indicated by the pH experiment,concentration profiles in the temperature experiments were measuredat the same location on each sample, and only samples from site2 were used for the experiments. Temperatures tested were 4°C,10°C (ambient), and 17°C. Measured profiles are presentedin Fig. 3.

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FIG. 3. pH, O₂, and Ca²⁺profiles at each experimental temperature.

In all treatments, pHs approached the same values in both lightand dark incubations, although there were some small differences(Table 2). The pH increased markedly under light conditions,from 8.4 to approximately 9.5 (maximum, 9.7). Under dark conditions,the pH decreased slightly, from 8.4 to approximately 8.1 at10°C and 17°C, respectively, while no pH decrease wasobserved at 4°C.

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TABLE 2. Fluxes of oxygen and calcium (mean ± standard error; n = 2) and pH changes at biofilm surfaces measured in samples from Deinschwanger Bach at different temperatures^a

Oxygen fluxes both away from and toward the sediment increasedwith the temperature in the light and dark, respectively (Table2). Calcium flux was always toward the stromatolite biofilmsurface under light conditions and increased with increasingtemperature, although this increase was not statistically significant(P > 0.05). Dark fluxes were much lower than those seen underthe light conditions, were always away from the stromatolitebiofilm surface, and also increased with increasing temperature.Under dark conditions, no calcium flux was observed from ortoward the stromatolite surface at 4°C (Table 2). Fluxesat 10°C and 17°C were significantly different from this.

DISCUSSION

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DISCUSSION

The investigated biofilm community, rich in filamentous cyanobacteria,flourishes in its natural setting (hard-water creeks) undera wide range of pH and temperature conditions; the pH rangesfrom 7.6 (a short distance downstream from the spring) to 8.5(lower creek sections and end of the carbonate deposition zone),with maximum values up to 9.3 measured within the biofilm microenvironment(6). The biofilm composition is described in detail by Shiraishiet al. (29). Phototrophic members of the biofilm were dominatedby filamentous cyanobacteria (3- to 5-µm wide) of morphotype"Phormidium incrustatum" but also included Lyngbya-type andcoccoid cyanobacteria and filamentous green algae of the genusCladophora. Diatoms, such as Achnanthes, Gomphonema, Nitzschia,and Navicula, occurred in the upper biofilm. Nonphototrophiccommunity members included heterotrophic bacteria, includingsulfate-reducing bacteria and flavobacterial species. The cyanobacterialcommunity composition was reasonably constant over the investigatedzone, with only the immediate spring environment (pH 7.3 to7.4) exhibiting distinct communities (unpublished data). Insitu temperatures vary seasonally between 5°C and 13°C.

Experimental manipulations of pH and temperature conditionswere conducted under conditions of constant alkalinity (3.0mmol kg^–1) but various DIC (2.8 to 3.1 mmol kg^–1);pH conditions were manipulated by the addition of CO₂. Experimentalflow rates were lower than in situ, resulting in slightly higherDBLs. We have shown previously (6) that photosynthesis increaseswhen the DBL approaches 600 µm but that the in situ flowconditions used maintained a DBL of 400 µm or less andagreed well with in situ microsensor measurements, both in thedark and in the light.

Under illumination, photosynthesis consistently caused the pHat the biofilm surface to increase to approximately 9.4, regardlessof overlying water pCO₂ (2,200 to 150 ppm V).

Changes similar to those with respect to the pH were noted fortemperatures, except at 4°C, where biological activity wasreduced to such an extent that changes were negligible. Thisdifference in the ${Delta}$ pH values in the light was observed despitethe similar O₂ production rates. In the dark, the opposite wasseen, i.e., respiration caused the pH to drop to approximately7.8 regardless of pCO₂ or temperature. Again, this occurreddespite similar O₂ consumption rates in the pH manipulationexperiments. O₂ consumption rates were, however, lower at lowertemperatures. The direction of the ${Delta}$ pH value changes was as expected,i.e., photosynthesis increased pH, while in the dark, respirationled to its decrease. The differences in the magnitudes of ${Delta}$ pH,resulting from different initial pH values but very similarfinal pH values, were unexpected. Several explanations for thisphenomenon may be offered.

The first is that the observed ${Delta}$ pH values were related to thephysiological optima of the mat community. If this had beenthe case, the highest ${Delta}$ pH value should have correlated with thehighest O₂ fluxes, but this was not observed. O₂ fluxes at allpH treatments were reasonably similar, with the maximum fluxactually occurring at a pH of 8.4, which is the pH of the creeksection from which the samples were taken.

The second explanation for the ${Delta}$ pH values observed is the possibilityof different pH buffering capacities at the various initialpHs. In this model, the lowest ${Delta}$ pH values should correlate withthe highest buffering at pK_a = 6.34 and pK_b = 10.36. Our results,however, show that + ${Delta}$ pH and – ${Delta}$ pH have opposite trends forincreasing bulk water pH values (Fig. 1). Furthermore, withinthe experimental pH range (7.8 to 8.9), which is near the half-equivalencepoint of 8.1, changes in pH buffering are very minor.

Third, the availability of DIC for photosynthesis may limitthe extent of light-induced pH increases. As CO₂ is removedby photosynthesis and pH increases, less CO₂ is available. Inthe current system (alkalinity, 3 mmol kg^–1) at pH 7.8,approximately 4% (138 mmol m^–3) of DIC exists as CO₂,while at pH 8.9, this value is reduced to 0.3% (10 mmol m^–3).Several studies have shown that DIC may limit photosynthesis,and it was suggested by Larkum et al. (15) that when the pHexceeds the level at which DIC exists as CO₂, DIC must be consumedas HCO₃^–. In the biofilms investigated here, the pH neverexceeds this level, although CO₂ does drop to a very low value(approximately 1 mmol m^–3 at pH 9.5). Cyanobacteria mayovercome CO₂ limitation via carbon-concentrating mechanisms,which effectively uncouple photosynthesis from CO₂ concentration.While these may have an effect on DIC chemistry at a cellularlevel, their effect on community level chemistry will be minimal.In essence, carbon-concentrating mechanisms do not change thestoichiometry of the processes and, thus, the local effectson pH. The fact that O₂ concentrations (the product of photosynthesis)remain well below overlying water DIC concentrations suggeststhat DIC is not limiting in this system. Even if DIC supplywere limiting photosynthesis, the nature of + ${Delta}$ pH and – ${Delta}$ pHtrends observed here would not be explained. There may indeedbe some physiological limitation to the extent of physiologicallyinduced + ${Delta}$ pH value changes, but these should also be reflectedin the O₂ production rates, which remain similar under all treatments.It is also possible that the calcification process limits theextent of pH changes and supports photosynthesis (17). For thisto explain the observed ${Delta}$ pH and O₂ production trends, we shouldsee calcification rates increase with increasing pH. This isnot the case. The explanation of DIC limitations also does notexplain the observed – ${Delta}$ pH value changes.

The final explanation for the observed results is a contributionfrom other unassessed processes (e.g., nitrate/ammonia assimilation),which may affect pH levels (30). The most probable explanationis some combination of all of the above, and further modelingand experimental work is required to address these issues.

Temperature manipulations were all conducted at pH 8.4, whichwas the in situ pH at the time of sampling. Temperature wasclearly shown to affect biological activity, with O₂ fluxesincreasing with increasing temperatures, both in the light andin the dark. Ca²⁺ fluxes (indicating, in this system, calciumcarbonate precipitation and dissolution) (6) also increasedwith increasing temperatures (Table 2 and Fig. 3). Althoughthese increases were not statistically significant in the experimentsconducted, this may be explained by the small degrees of freedomused. The flux differences may be biologically important, andgiven that little change was observed in the biofilm surfacepH and ${Omega}$ values under all experimental conditions, it appearsthat the effects of temperature changes on the diffusion coefficientsof Ca²⁺ and HCO₃^2– are important in determining flux rates.The diffusion coefficients increase with temperatures and, inthese experiments, explain the magnitudes of increasing Ca²⁺flux rates we observed.

Temperature, therefore, affects the possible transport limitationsof precipitating chemicals, which in turn affects possible ratesof calcite deposition and dissolution. Although temperatureincrease leads to an increase in biological activity, ion diffusionvelocity, and calcification in the light, the concomitant increasein dark parameters also increases dissolution, thereby maintainingsimilar net diel precipitation rates at all temperatures. Forthe interpretation of the fossil record of calcifying cyanobacteria,this implies that the abundance of cyanobacterial microfossilsand related stromatolites appears not to be significantly affectedby marine surface temperature variations, contrary to previoussuggestions (21). This is true at least for the investigatedrange between 4°C and 17°C.

The ability of biological systems to control their microenvironment,and therefore create an environment very different from thatof their wider surroundings, also leads to interesting implicationsfor both the prediction of the effects of increasing atmosphericpCO₂ and the paleogeological interpretation of calcified microfossils.It appears that under high pCO₂ conditions, cyanobacterial calcificationmay be maintained by high CO₂ availability and proceed at low"apparent" pH (i.e., low pH in the overlying water). Therefore,as long as calcite saturation at the cell/biofilm surface remains>1, the formation of calcareous, tubular microfossils maystill occur at low overlying water pH conditions (certainlybetween 7.8 to 8.4, as investigated here). Indeed the magnitudeof ${Omega}$ does not appear to influence the rate of calcification,but rather, once some ${Omega}$ threshold (approximately 10) is reached,calcification may proceed. This is contradictory to the ideathat increasing pCO₂ should reduce the potential of photosynthesis-inducedcalcification in cyanobacterial biofilms by lowering bulk phasepH and hence CaCO₃ mineral supersaturation (14, 28).

ACKNOWLEDGMENTS

We thank the microsensor technicians at the MPI, Bremen, Germany,for assistance with microsensor construction and Lubos Polereckyfor the microprofiling software. We thank Hakhyun Nam (KwangwoonUniversity, South Korea) for supplying the carbonate ionophore.

This project is part of the Research Unit "Geobiology of organo-and biofilms," funded by the German Research Foundation (DFG-FOR571, publication no. 23).

FOOTNOTES

* Corresponding author. Present address: CSIRO, Plant Industry, P. O. Box 1600, Canberra, ACT 2601, Australia. Phone: 61 (0)2 6246 4820. Fax: 61 (0)2 6246 5000. E-mail: Andrew.Bissett{at}csiro.au

Published ahead of print on 8 August 2008.

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

REFERENCES

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