Hostname: page-component-78c5997874-94fs2 Total loading time: 0 Render date: 2024-11-02T19:25:05.528Z Has data issue: false hasContentIssue false
  • English
  • Français

Measuring rates of gross photosynthesis and net community production in cryoconite holes: a comparison of field methods

Published online by Cambridge University Press:  14 September 2017

J. Telling ,
A.M. Anesio ,
J. Hawkings ,
M. Tranter ,
J.L. Wadham ,
A.J. Hodson ,
T. Irvine-Fynn  and
M.L. Yallop
J. Telling
Affiliation:
Bristol Glaciology Centre, School of Geographical Sciences, University of Bristol, University Road, Bristol BS8 1SS, UK E-mail: [email protected]
A.M. Anesio
Affiliation:
Bristol Glaciology Centre, School of Geographical Sciences, University of Bristol, University Road, Bristol BS8 1SS, UK E-mail: [email protected]
J. Hawkings
Affiliation:
Bristol Glaciology Centre, School of Geographical Sciences, University of Bristol, University Road, Bristol BS8 1SS, UK E-mail: [email protected]
M. Tranter
Affiliation:
Bristol Glaciology Centre, School of Geographical Sciences, University of Bristol, University Road, Bristol BS8 1SS, UK E-mail: [email protected]
J.L. Wadham
Affiliation:
Bristol Glaciology Centre, School of Geographical Sciences, University of Bristol, University Road, Bristol BS8 1SS, UK E-mail: [email protected]
A.J. Hodson
Affiliation:
Department of Geography, University of Sheffield, Winter Street, Sheffield S10 2TN, UK
T. Irvine-Fynn
Affiliation:
Department of Geography, University of Sheffield, Winter Street, Sheffield S10 2TN, UK
M.L. Yallop
Affiliation:
School of Biological Sciences, University of Bristol, Woodland Road, Bristol BS8 1UG, UK
Rights & Permissions [Opens in a new window]

Abstract

Photosynthesis by microbes on the surfaces of glaciers and ice sheets has the potential to fix carbon, alter the albedo of ice surfaces via the production of organic matter and so enhance ice melt. It could also be important for supplying labile organic matter and nutrients to in situ and downstream ecosystems. This study compares in situ 24 hour incubation methods for measuring rates of gross photosynthesis, respiration and net community production (NCP) in cryoconite holes on three Svalbard valley glaciers. Rates of gross photosynthesis and respiration measured by the ΔCO2 method were closely balanced, resulting in rates of NCP close to the detection limit (mean of –1.3 μg C g−1 d–1) consistent with previous measurements in Arctic cryoconite holes. This suggests that organic matter within cryoconite holes may be derived largely from allochthonous sources. The molar ratio of ΔO2 to ΔCO2 in incubations gave mean respiratory and photosynthetic quotients of 0.80 ± 0.17 (1 × SD) and 1.24 ± 0.20 (1 × SD), respectively. The 14C method typically underestimated rates of gross photosynthesis (ΔCO2 method) by more than one order of magnitude and measured a rate closer to NCP.

Type
Research Article
Information
Annals of Glaciology , Volume 51 , Issue 56 , 2010 , pp. 153 - 162
Copyright
Copyright © the Author(s) [year] 2010

Introduction

The surfaces of glaciers and ice sheets are known to harbour a diverse range of prokaryotic and eukaryotic microorganisms (Reference Mueller, Vincent, Pollard, Fritsen, Elster, Seckbach, Vincent and LhotskýMueller and others, 2001; Reference Christner, Kvito and ReeveChristner and others, 2003; Reference Porazinska, Fountain, Nylen, Tranter, Virginia and WallPorazinska and others, 2004). The abundance and activity of the microorganisms is typically focused within thin sediment layers (cryoconite) found within shallow (<50cm) water-filled depressions known as cryoconite holes (Reference Säwström, Mumford, Marshall, Hodson and Laybourn-ParrySawstrom and others, 2002; Reference HodsonHodson and others, 2007, Reference Hodson2008).

While rates of respiration and gross photosynthesis have been measured within cryoconite (Reference Säwström, Mumford, Marshall, Hodson and Laybourn-ParrySawstrom and others, 2002; Reference HodsonHodson and others, 2007, Reference Hodson2010a,Reference Hodsonb; Reference Stibal, Tranter, Benning and RehákStibal and others, 2008a; Reference Anesio, Hodson, Fritz, Psenner and SattlerAnesio and others, 2009), there is current debate in the literature as to the balance between them. If respiration dominates and cryoconite holes are net heterotrophic, then the dominant source of organic carbon within cryoconite sediments must be allochthonous in origin (Reference Stibal, Tranter, Benning and RehákStibal and others, 2008a; Reference HodsonHodson and others, 2010b). However, if rates of gross photosynthesis dominate, then the resultant net production of autochthonous organic matter could provide an important source of labile carbon and nutrients to in situ and downstream ecosystems (Reference Anesio, Hodson, Fritz, Psenner and SattlerAnesio and others, 2009). Furthermore, the formation of autochthonous organic matter could potentially promote ice melting, either directly through the production of pigmented organic matter (Reference Takeuchi, Kohshima and SekoTakeuchi and others, 2001; Reference Mueller and VincentMueller and Vincent, 2006) or indirectly by the entrapment of dark inorganic sediment by extracellular polymeric substances (Reference Yallop, de Winder, Paterson and StalYallop and others, 1994; Reference StalStal, 2003; Reference Mueller and VincentMueller and Vincent, 2006).

To date, all studies that have measured in situ rates of photosynthesis in cryoconite holes have used closed-bottle incubations over either 12 or 24 hours (Reference Säwström, Mumford, Marshall, Hodson and Laybourn-ParrySawstrom and others, 2002; Reference Stibal, Tranter, Benning and RehákStibal and others, 2008a; Reference Anesio, Hodson, Fritz, Psenner and SattlerAnesio and others, 2009; Reference HodsonHodson and others, 2010a,Reference Hodsonb). Only two studies have directly measured changes in O2 (ΔO2) and CO2 (ΔCO2) in the bottles (Reference HodsonHodson and others, 2010a,Reference Hodsonb), while the remainder have used the 14C method originally developed by Reference Steemann-NielsenSteemann-Nielsen (1952). The 14C method involves the addition of a small amount of NaH1 4CO3 as a tracer in closed-bottle incubations to measure rates of total C (i.e. 12C) uptake. Crucially, the 14C method may underestimate the rate of gross photosynthesis due to recycling of 14CO2 via cycles of photosynthesis and respiration (Reference PetersonPeterson, 1980). Checking for these effects requires cross calibration with other methods (Reference BenderBender and others, 1987).

This study uses in situ closed-bottle incubations in cryoconite holes on three Svalbard glaciers to cross calibrate the 14C method against direct measurements of ΔCO2 and ΔO2.

Methods

Site location and descriptions

Incubation experiments were conducted in 11 cryoconite holes on three valley glaciers, Midtre Lovenbreen (ML), Vestre Brøggerbreen (VB) and Austre Brøggerbreen (AB), situated in the northwest of the Svalbard archipelago, close to the scientific base at Ny-Alesund (78°55’48’’ N, 11°56’59’’E; Fig. 1). All incubations took place in July 2009. All the cryoconite holes studied were open, i.e. did not have ice lids. Owing to the relatively late start of the melt season on the glaciers in 2009, six of the 11 cryoconite holes were still covered in slush.

Fig. 1. Location of cryoconite holes where in situ rates of photosynthesis and respiration were measured. AB = Austre Brøggerbreen, ML=Midtre Lovénbreen, VB=Vestre Brøggerbreen. Note that x and y labels are in Universal Tranverse Mercator (UTM) coordinates.

Cryoconite hole diameters, heights, water depths, slush depths and sediment depths were measured using a 30 cm ruler, to allow estimates of relative sediment-to-water volumes.

O2 , temperature and dissolved inorganic carbon (DIC) measurements of water

Oxygen and temperature measurements were taken with a Hach HQ30d meter with luminescent dissolved oxygen probe following the method of Reference HodsonHodson and others (2010b). The relative standard deviation (RSD) of the luminescent oxygen probe was 1.5%. The precision of the temperature sensor is quoted by the manufacturer as ±0.1 °C. Measurements of DIC were made using a PP systems EGM-4 infrared CO2 meter, following the method of Reference HodsonHodson and others (2010b). The RSD was 0.98%.

Total organic carbon (TOC) content of cryoconite sediment

Cryoconite was first dried at 70°C for 2 days then analysed for total carbon (TC) on a Eurovector EA3000 Elemental analyser. Inorganic carbon (IC) was determined using a Coulomat 720 analyser. TOC was defined as the difference between TC and IC. The detection limit was 100| μgCg−1 dry sediment.

Batch incubations for estimating rates of photosynthesis and respiration

The ΔO2 and ΔCO2 methods

At each site, sediment was collected from the hole and added to six glass bottles with tapered glass stoppers (60 mL BOD bottles, Wheaton) to give a sediment depth of ∼2–4mm. All bottles were filled completely with in situ supraglacial water to give approximate sediment/water ratios of 1 :60. At each site, three of the bottles were chosen randomly and covered with aluminium foil (dark bottles). The remaining three bottles (light bottles) were illuminated by the natural levels found in situ. At three sites (one on each glacier), an additional two bottles (one light, one dark) were filled completely with supraglacial water only. All bottles were submerged completely in water within cryoconite holes and incubated for 24 ± 2 hours. If present, slush was scooped back over the bottles in the holes to give the same approximate depth of slush as was present initially.

Starting oxygen concentrations and temperature were measured on each individual bottle prior to incubation. Starting values for DIC were established by filling three identical BOD bottles with supraglacial water and measuring immediately for DIC, as described above. Oxygen, temperature and DIC were also measured in the bottles at the end of the incubation period. All measurements were made in situ on the glaciers immediately after removing the bottles from the cryoconite holes. Corrections for sulphide oxidation (for oxygen measurements, Equation (1)) and carbonate dissolution (for DIC measurements, Equation (2)) during incubation were made following the procedure of Reference HodsonHodson and others (2010b).

(1)

(2)

Start and end incubation concentrations for Ca2+, Mg2 + and SO42– were measured on a Dionex 4000i Ion Chromatography System at the University of Bristol. The acidified samples were stored refrigerated for up to 4 months prior to analysis. The RSD for Ca2+, Mg2 + and SO4 2– determinations was 8.7%, 5.6% and 7.3%, with corresponding detection limits of 2.0, 0.93 and 3.6 μM, respectively (based on mean + (3 × SD) of eight blanks).

Total respiration and net community production (NCP) were determined from the O2 and DIC measurements in dark and light bottles, respectively. NCP is defined here as the net balance of gross photosynthesis and respiration for the entire microbial community. Gross photosynthesis rates were calculated by subtracting the O2 and DIC concentrations of dark bottles from light bottles. In all cases, rates were normalized for the different dry weights of sediment in the bottles, determined by drying and weighing the sediment.

The detection limits for the ΔCO2 method were 18 μgC L−1 d−1 (1.2 μgCg−1 d−1) for rates of NCP and respiration, and 26 μgC L−1 d−1 (1.7μgCg−1 d−1) for gross photosynthesis. The detection limits for the ΔO2 method were 96 μgCL−1 d−1 (6.2μgCg−1 d−1) for rates of NCP and respiration and 136 μgCL−1 d−1 (8.8μgCg−1 d−1) for gross photosynthesis. The sediment weight normalized detection limits assume 1 g of dry sediment, which was typical for the incubations of the present study.

The 14C method

In parallel to the ΔO2 and ΔCO2 method incubations, sediment was added to six 7 mL transparent polystyrene vials with screw-cap lids to give sediment/volume ratios of approximately 1 :50. All vials were glued horizontally to glass slides so they sank to the bottom of cryoconite holes, so that they received the same ambient light levels as the glass BOD bottle incubations used for the ΔCO2 and ΔO2 methods. Supraglacial water was then added to fill the vials completely, leaving no headspace. At three sites (one on each glacier), an additional two vials (one light, one dark) were filled completely with supraglacial water only. Aliquots (7 μL) of a 37MBq stock of 14C-NaHCO3 (Perkin-Elmer) were added via an automatic pipette below the level of the water and the vials capped immediately. At each site, three of the six vials were covered with foil (dark controls) and the tubes left to incubate for 24 ± 2 hours. After incubation, samples were filtered immediately onto 0.2 μm Nuclepore polycarbonate filters, the filtrates collected into 20 mL scintillation vials and 300 μL of 3 M HCl added to acidify the samples and remove DIC. The filters were then transported back to the laboratory within 4 hours and left under an upturned beaker in a fume cupboard for 1 hour with small open beakers of 25% glutaraldehyde and concentrated hydrochloric acid to kill microbial activity and remove DIC. The filters were next placed in pre-weighed scintillation vials, allowed to dry overnight at 70°C and reweighed. The acidified filtrates were shaken and left to degas overnight in the fume cupboard. Samples were transported in 20 mL scintillation vials back to the UK, then 5 mL aliquots of scintillation cocktail (Ultima GoldTM, PerkinElmer) were added to 1 mL aliquots of filtrates, and 10 mL of scintillation cocktail added to filters. The vials were then left in the dark for 24 hours prior to counting on a PerkinElmer Tri-Carb 2810 TR scintillation counter, using external standards to correct for quenching.

DPM values were converted to carbon uptake values by:

(3)

where 12C uptake is the amount of carbon taken up into cells (μg C L−1 d−1), 14C sample is the activity of the sample (sum of filtrate and filter DPMs), C is the concentration of DIC in the incubation water (μg C L−1), 1.06 is the isotope constant effect between 12C and 1 C, 4C added is the activity of NaH14CO3 added to each vial (DPM) and t is the duration of incubation (days).

Rates of photosynthesis were calculated by subtracting dark control from light bottle incubations. The percentage of 14C incorporated into extracellular dissolved organic material (14C-DOC), rather than into microbial cells or particulate matter, was defined as the percentage of the 14C measured in the filtrates compared with that on the filters.

Statistical analysis

Preliminary statistical tests (for normality and variance) were carried out using the SPSS statistical software package. These tests demonstrated that the 14C, ΔCO2 and ΔO2 datasets had approximately normal distributions; however, there were differences in variance between methods. Consequently, comparisons between methods were carried out using two-tailed t tests (p<0.05) assuming non-equal variances. Correlations were carried out using Pearson’s product-moment correlation method.

Results

Temperature, O2 saturation and DIC of in situ cryoconite water

The temperature of the water in all 11 cryoconite holes used for incubation experiments was 0.1 ±0.1°C. O2 saturation levels were 100 ± 4 . 6% and DIC concentrations ranged from 29.8 to 44.9 μM (Table 1).

Table 1. Physical and chemical characteristics of cryoconite holes

Temperature, calcium, magnesium and sulphate changes in incubation water

There was no systematic difference in temperature between light and dark incubations of the ΔO2 and ΔCO2 methods, with a mean difference of 0.0±0.7°C (1 × SD). The mean temperatures measured at the start and end of incubations were 2.1°C ( ± 1.1°C, 1 × SD) and 1.3°C (± 0.7°C, 1 × SD), respectively, slightly higher than the mean in situ temperature of 0.1°C. However, temperatures in incubations were measured after bottles had been removed from the cryoconite holes and oxygen measurements taken. The warmer temperatures could therefore be an artefact of short-term surface warming during measurements rather than representative of incubation temperatures.

The maximum changes in Ca2+ and Mg2 + during incubations were <6 and <2 μM, respectively, with the exception of AB1 incubations where the Ca2+ and Mg2 + changes measured were up to 31 and 18μM, respectively. No changes in SO4 2 - concentration during incubations were detected.

TOC content of cryoconite

The TOC content of cryoconite ranged from 14 to 32 mg Cg−1 dry sediment, with an average of 23 mgCg−1 dry sediment d−1 (Table 1).

Comparison of A O2 and ΔCO2 methods for respiration and gross photosynthesis and NCP

Rates of gross photosynthesis and respiration determined by the ΔCO2 method in cryoconite-amended incubations were of similar magnitude (6.5–32.2 μgCg−1 d−1 for gross photosynthesis, 4.3–37.1 μgCg- 1 d−1 for respiration; Table 2), resulting in relatively small changes in NCP (–11.9 to 8.0 μgCg−1 d−1; Table 2). A comparison of paired ΔO2 and ΔCO2 rates of gross photosynthesis, respiration and NCP is shown in Figure 2. For all paired measurements above the detection limit (Fig. 2), the mean photosynthetic quotient (PQ, the molar ratio of O2 produced to CO2 consumed) was 1.24 ± 0.20 (1 × SD). The mean respiratory quotient (RQ, the molar ratio of CO2 produced to O2 consumed) was 0.80 ± 0 . 1 7 (1 × SD). The mean NCP quotient (defined here as the molar ratio of O2 produced to CO2 consumed) was 2.34 ± 1 . 9 0 (1 × SD). There were significant differences between paired ΔO2 and ΔCO2 measurements for photosynthesis (p<0.05, two-tailed t test) and gross photosynthesis (p<0.05, two-tailed t test), but not for NCP (p = 0.27, two-tailed t test).

Table 2. Rates of gross photosynthesis, respiration, NCP (all from ΔCO2 method) and 14C photosynthesis in cryoconite sediment and water incubations. Mean rates are shown with minimum and maximum rates in parentheses. Negative numbers for NCP indicate net heterotrophy; positive numbers indicate net autotrophy

Fig. 2. Comparison of paired measurements of rates by CO2 and O2 methods. (a) Gross photosynthesis, (b) respiration and (c) NCP. Dotted lines show typical ranges of photosynthetic and respiratory quotients (PQ and RQ) from other environments: PQ range of 1.0–1.4 (Reference Williams and RobertsonWilliams and Robertson, 1991); RQ range of 0.7–1.0 (Gnaiger, 1983). Shaded areas are below the detection limit.

Rates of gross photosynthesis and respiration were substantially lower in the water-only incubations compared with cryoconite-amended incubations (Table 2). Mean rates of respiration and gross photosynthesis in water-only incubations were 7.39 and 85.6 μgCL−1 d−1, respectively (ΔCO2 method) (Table 2). In situ ratios of cryoconite:water in the cryoconite holes (mean 1 :34, range from 1 :6 to 1 : 75; Table 1) were generally similar to, or lower than, that of the incubation bottles (1 :60). Rates of gross photosynthesis and respiration measured in bottle incubations should therefore approximate in situ rates of cryoconite holes.

The daily rates of gross photosynthesis were sufficient to utilize 41–291% (mean 146%) of the starting DIC pool in incubation bottles (Table 2). Since rates of NCP demonstrate only relatively small changes in DIC over the course of the incubations (Table 2; Fig. 3), this indicates that the DIC pool in incubation bottles is typically recycled completely in 24 hours. In contrast, daily rates of gross photosynthesis in water-only incubations were only capable of utilizing 0.5–1.9% (mean 1.2%) of the starting DIC pool (Table 2).

Fig. 3. Comparison of rates of photosynthesis by 14C method with (a) rates of gross photosynthesis by the ΔO2 and ΔCO2 methods and (b) rates of NCP by the ΔO2 and ΔCO2 methods. Error bars are 1 SD. Note the logarithmic scale in (a).

Comparison of the 1 4C method with estimates of NCP and gross photosynthesis by the ΔCO2 method

Measurements of photosynthesis by the 14C method ranged from 0.3 to 3.9 μgCg−1 d−1 (Table 2). These are closer to rates of NCP rather than gross photosynthesis as determined by the ΔCO2 method (Fig. 3). There were significant differences between mean rates of 14C photosynthesis and gross photosynthesis (p<0.05, two-tailed t test), but not between 14C photosynthesis and NCP (p = 0.186, two-tailed t test). Paired rates of 14C photosynthesis with NCP and paired rates of 14C photosynthesis with gross photosynthesis were poorly positively correlated (R=0.57 and 0.53, respectively), with neither correlation significantly different from zero (p<0.05) (Fig. 4).

Fig. 4. Scatter plots of rates of photosynthesis measured by the 14C method vs (a) gross photosynthesis (ΔCO2 method) and (b) NCP (ΔCO2 method). Errors bars are 1 SD of triplicate measurements. Pearson’s product-moment correlation indicated no significant relationships (p<0.05) in either (a) or (b).

Dark bottle uptake of 14C and percentage of 14C released as dissolved organic matter

There was a significant uptake of 14C in dark bottles, with higher rates in water-only incubations (11–33%, mean 22%; Table 2) compared with sediment-amended incubations (2.6–16.0%, mean 8.0%; Table 2). The percentage of 14C released as 14C-DOC into the filtrate fraction of sediment-amended incubations was low (0.2–1.4%; Table 2). A larger percentage of 14C-DOC was measured in the filtrate fraction of water-only incubations (13.0–37.3%).

Discussion

Respiratory and photosynthetic quotients (RQ and PQ) in Arctic cryoconite holes

The sediment fraction of cryoconite holes in the present study dominates both rates of gross photosynthesis and respiration (Table 2). This is consistent with previous studies on Arctic cryoconite holes (Reference Säwström, Mumford, Marshall, Hodson and Laybourn-ParrySawstrom and others, 2002; Reference Anesio, Hodson, Fritz, Psenner and SattlerAnesio and others, 2009; Reference HodsonHodson and others, 2010b). Previous studies have also assumed a 1 :1 stoichiometry between ΔO2 and ΔCO2 in Arctic cryoconite holes (Reference HodsonHodson and others, 2007; Reference Anesio, Hodson, Fritz, Psenner and SattlerAnesio and others, 2009). However, the present study demonstrated that there were significant differences (p<0.05) between the ΔO2 and ΔCO2 methods for measuring rates of respiration and gross photosynthesis, resulting in a mean RQ of 0.88 ±0.17 (1 × SD) and a mean PQ of 1.24 ± 0.2 (1 × SD) (Fig. 2). The mean RQ is within the range of RQ values expected from variations in the composition of biological organic matter (0.7–1.0; Reference Gnaiger, Gnaiger and ForstnerGnaiger, 1983). Similarly, the mean PQ value of the present study is within the typical PQ range for algae (1.0–1.4; Reference Williams and RobertsonWilliams and Robertson, 1991), with PQ varying with the source of nitrogen (e.g. ammonia or nitrate) used by the photosynthetic cells (Reference Williams and RobertsonWilliams and Robertson, 1991).

Rates of gross photosynthesis in cryoconite holes

The rates of gross photosynthesis in cryoconite-amended incubations (mean of 17.3 μgCg−1 d−1 by the ΔCO2 method) are similar to previous estimates of gross photosynthesis in Arctic cryoconite holes in Svalbard and Greenland made using the same method (mean between 15.7 and 23 μg C g−1 d−1, respectively; Reference HodsonHodson and others 2010a,Reference Hodsonb; Table 3). The factors limiting rates of gross photosynthesis in cryoconite holes have yet to be established, although phosphorus has been suggested as a likely limiting factor on rates of overall microbial growth (Reference Säwström, Laybourn-Parry, Granéli and AnesioSäwström and others, 2007a; Reference Stibal, Tranter, Telling and BenningStibal and others, 2008b).

Table 3. Summary of published rates of gross photosynthesis, NCP and 14C photosynthesis in cryoconite holes

The average rates of gross photosynthesis from the only available data of Antarctic cryoconite holes are an order of magnitude lower than Arctic cryoconite holes at 2.4 μg C g−1 d − 1 (Reference HodsonHodson and others, 2010b; Table 3). This could reflect the closed more hydrologically isolated nature of Antarctic cryoconite holes due to the thick ice lids that commonly form above them (Reference TranterTranter and others, 2004). Greater isolation both from the atmosphere and from hydrological flow would reduce the flux of both DIC and nutrients (Reference TranterTranter and others, 2004), while the thicker ice lids may lower the levels of light available to microorganisms.

The potential problem of bottle effects

This study assumes that rates of photosynthesis and respiration measured within incubation bottles accurately reflect those of the in situ cryoconite holes. However, there remains the possibility that nutrient concentrations in the bottles could change over 24 hours from in situ concentrations. This could potentially alter both rates of microbial processes and community structure in the bottles (i.e. ‘bottle effects’; Reference Li and DickieLi and Dickie, 1991). Ideally, future studies of cryoconite holes should compare shorter-term measurements of photosynthesis and respiration with 24 hour measurements to check for any bottle effects.

A further assumption of the light–dark bottle technique for estimating rates of gross photosynthesis is that rates of respiration are the same in the dark bottles as in the light bottles. Previous studies on other aquatic environments have shown that, while often true, this is not always the case and that respiration rates in the light can be higher than in the dark, leading to an underestimation of gross rates of photosynthesis (Reference YallopYallop, 1982; Reference BenderBender and others, 1987; Reference KanaKana, 1990). Processes that can cause increased respiration in light bottles include photorespiration and the Mehler reaction involving uptake of oxygen by photosystem 1 (Reference BurrisBurris, 1977; Reference YallopYallop, 1982; Reference Lancelot and MathotLancelot and Mathot, 1985). Conversely, respiration rates in the light could be lower than in the dark, either due to differences in temperature within dark and light bottles or inhibition of microorganisms by ultraviolet (UV) radiation (Reference Thomson, Dyke and WorrestThomson and others, 1980; Reference Herndl, Müller-Niklas and FrickHerndl and others, 1993). The former can be discounted, as there were no systematic temperature differences between paired light and dark bottles in the present study. Inhibition by UV radiation is also unlikely to reduce rates of respiration, since the glass walls of the incubation bottles used for the ΔCO2 and ΔO2 methods will cut out the majority of harmful UV-B radiation (Reference Ferreyra, Demers, del Giorgio and ChanutFerreyra and others, 1997).

However, it is possible that the elimination of UV-B radiation in glass bottle incubations may have artificially increased rates of photosynthesis and respiration in the ΔCO2 and ΔO2 methods relative to in situ rates (Reference Cullen, Neale and LesserCullen and others, 1992; Reference Herndl, Müller-Niklas and FrickHerndl and others, 1993). In contrast to the glass bottles, the polystyrene vials used in the 14C method will have transmitted a significant fraction of the UV-B spectrum (Reference Furgal and SmithFurgal and Smith, 1997).

Uncertainties in interpreting the 14C results

Importantly, this study has shown that 14C measurements do not accurately measure rates of either gross photosynthesis or NCP in cryoconite holes (Fig. 4). However, rates of 14C photosynthesis are closer to those of NCP than gross photosynthesis (Fig. 3). The majority of aqueous ecological studies that have used the 14C method over 24 hours have concluded that it measures a rate closer to net photosynthesis rather than gross photosynthesis (Reference PetersonPeterson, 1980; Reference Dring and JewsonDring and Jewson, 1982; Reference Behrenfeld and FalkowskiBehrenfeld and Falkowski, 1997). Net photosynthesis is defined here as gross photosynthesis minus photoautotrophic respiration, in contrast to NCP which subtracts total community respiration (Reference PetersonPeterson, 1980). The model most commonly used to explain why the 14C method can measure a rate closer to net photosynthesis is that of Reference Hobson, Morris and PirquetHobson and others (1976). In this model, photosynthetically fixed 14C-organic matter is respired back to 14CO2 and exuded outside the cell. The initial rate of photosynthesis will be closer to gross rates of photosynthesis because the initial organic matter within the cell will be low in 14C, so respiration will initially remove little 14C. As incubation time increases, the 14C content of the cell organic matter increases, so that the relative loss of 14C back to 14CO2 will also increase, until rates eventually approach that of net photosynthesis (Reference Hobson, Morris and PirquetHobson and others, 1976; Reference Williams and LefèvreWilliams and Lefèvre, 2008).

The model of Reference Hobson, Morris and PirquetHobson and others (1976) assumes that photoautotrophic respiration is responsible for all the respiration of photosynthetically fixed 14C-organic matter. However, if heterotrophic microorganisms respire a significant fraction of the fixed 14C-organic matter, then the 14C method can potentially measure a rate lower than net photosynthesis and approach NCP (Reference Gieskes, Kraay and BaarsGieskes and others, 1979). In net heterotrophic ecosystems, however, the 14C method can only approach zero rather than NCP, as an intrinsic drawback of the 14C method is that it can only measure positive (i.e. net autotrophic) values (Reference PetersonPeterson, 1980).

There was significant heterotrophic activity within the incubations of the present study. Indeed, many of the incubations were net heterotrophic (Fig. 3), although the proportion of heterotrophic to photoautotrophic respiration in the cryoconite is not known (Reference AnesioAnesio and others, 2010). Furthermore, the dark 14C uptake results of the present study were consistent with substantial heterotrophic activity. The mean dark 14C uptakes of 8.0% and 21.9% (for sediment-amended and water-only incubations, respectively; Table 2) were of a similar magnitude to those reported previously in Svalbard cryoconite (6.4–16.0%; Reference Stibal and TranterStibal and Tranter, 2007) and higher than the 1–2% typically found in surface ocean water (Reference Li, Irwin and DickieLi and others, 1993). Such relatively high dark uptake of 14C has previously been interpreted as the results of a high proportion of heterotrophic to photoautotrophic respiration (Reference Gieskes, Kraay and BaarsGieskes and others, 1979). However, other autotrophic bacteria (in particular, ammonia-oxidizing bacteria) could also be responsible for part of the dark 14C uptake (Reference BillenBillen, 1976).

Heterotrophic microorganisms need to gain access to, and respire, the photosynthetically fixed 14C-organic matter in order to directly affect the results of the 14C method. The principal mechanisms for this are cell lysis (and promotion of cell lysis by viral infection), grazing by predators (Reference Karl, Hebel, Björkman and LetelierKarl and others, 1998) and the release of organic matter from photosynthetic cells by passive or active exudation (Reference FoggFogg, 1983). While rates of cell lysis in cryoconite holes are unknown, the virus-induced lysis of cells in cryoconite holes may be an important source of organic carbon for heterotrophic microorganisms (Reference Anesio, Mindl, Laybourn-Parry, Hodson and SattlerAnesio and others, 2007; Reference Sä, wström, Granéli, Laybourn-Parry and AnesioSäwström and others, 2007b). A high incidence of microbial infection by phage cells has also been reported in cryoconite waters on ML (Reference Sä, wström, Granéli, Laybourn-Parry and AnesioSäwström and others, 2007b) and high ratios of viruses to bacteria have been documented in cryoconite sediments and waters on AB and ML (Reference Anesio, Mindl, Laybourn-Parry, Hodson and SattlerAnesio and others, 2007). In addition, eukaryotic predatory microorganisms, including tardigrades, rotifers and ciliates, have been documented in cryoconite holes (Reference De Smet and van RompuDe Smet and Van Rompu, 1994; Reference Porazinska, Fountain, Nylen, Tranter, Virginia and WallPorazinska and others, 2004), although the ecological importance of grazing in cryoconite holes has yet to be established. However, over the timescale of incubations in our study, the exudation of dissolved or colloidal organic matter by living photosynthetic algae and cyanobacteria is likely to be more important as a source of organic matter for heterotrophic microorganisms than cell lysis or grazing (Reference Karl, Hebel, Björkman and LetelierKarl and others, 1998).

The percentages of 14C exuded as DOC in water-only incubations of the present study (13.0–37.3%; Table 2) were similar to those in other aquatic environments (typically 5–40%; Reference FoggFogg, 1983; Reference Baines and PaceBaines and Pace, 1991; Reference Morán, Estrada, Gasol and Pedrόs-AliόMorán and others, 2002), whereas cryoconite-amended incubations had relatively low percentages of 14C-DOC (0.2–1.4%; Table 2). However, in microbial mats in some benthic environments, as much as 70% of total primary production may be exuded as colloidal organic matter in the form of extracellular polysaccharides (EPS) (Stal, 1993; Reference Goto, Kawamura, Mitamura and TeraiGoto and others, 1999). The relatively low percentages of 14C-DOC in sediment incubations of the present study could therefore be explained by the exudation of colloidal 14C-organic matter. Certainly, the production of colloidal EPS is consistent with a study indicating that cyanobacteria in cryoconite bind granules together with EPS (Reference HodsonHodson and others, 2010b). Alternatively, however, the relatively low 14C-DOC percentages could reflect either an overall low rate of organic matter exudation, or an efficient uptake of exuded 14C-DOC by heterotrophic bacteria in the cryoconite-amended incubations (Reference Karl, Hebel, Björkman and LetelierKarl and others, 1998). Further research is needed to distinguish between these hypotheses.

Interpreting the ecological significance of the 14C method in the present study is therefore problematic. If the bulk of photosynthetically fixed 14C-organic matter was respired by the photosynthetic microorganisms rather than heterotrophic microorganisms, then the 24 hour 14C method could have measured a rate close to that of net photosynthesis. If, however, heterotrophic recycling was substantial, then the 14C method may have measured a rate in between net photosynthesis and zero, and of potentially little value in ecological interpretation.

NCP in Arctic cryoconite holes

Measurements of NCP by the ΔCO2 method should be robust, as it relies simply on changes in the chemistry of one bottle (the light bottle). The relatively small rates of NCP (mean of –0.3 μgCg−1 d−1, with a range of –11.9 to 8.0 μg Cg−1 d−1, ΔCO2 method; Table 2) reflect the close balance between rates of respiration and gross photosynthesis within incubation bottles. Many of the NCP measurements were close to the detection limit (Fig. 2), probably accounting for part of the large variation in NCP quotients (1.98 ± 1.76).

Previous estimates of NCP in Arctic cryoconite holes have been similarly low to those of the present study (–0.6 to –1.8μgCg−1 d−1; Table 3). Previous mean measurements of photosynthesis using the 14C method have all been <1.3 μgCg−1 d−1 (Table 3). As discussed above, the ecological significance of the 24hour 14C data is uncertain; however, the low 14C rates are consistent with a closely balanced or net heterotrophic ecosystem. This study therefore supports the conclusion that photosynthesis in cryoconite holes has at most a small, and more likely a negligible, impact on the net creation of organic matter, suggesting instead that organic matter may be derived largely from allochthonous sources (Reference Stibal, Tranter, Benning and RehákStibal and others, 2008a; Reference HodsonHodson and others, 2010b). The major impact microbes can have in affecting the albedo of glaciers is then through the transformation and cementing together of allochthonous organic matter, rather than through the net creation of new dark organic matter (Reference HodsonHodson and others, 2010b).

Conclusions

This study compares different closed-bottle incubation methods of determining rates of gross photosynthesis, respiration and NCP in a range of cryoconite holes on three different valley glaciers in Svalbard. Rates of photosynthesis, respiration and NCP were determined by ΔO2 and ΔCO2 after 24 hour incubations. Rates of photosynthesis were also estimated using the 14C method in parallel 24 hour incubations.

Rates of gross photosynthesis and respiration measured by the ΔCO2 method were closely balanced (means of 17.3 and 20.1 μgCg−1 d−1, respectively). The molar ratio of ΔO2 :ΔCO2 in incubations gave mean respiratory and photosynthetic quotients of 0.80 ± 0 . 1 7 (1 × SD) and 1.24± 0.20 (1 × SD), respectively. The mean NCP (ΔCO2 method) was just –1.3 μgCg−1 d−1, close to the detection limit, and consistent with previous very low measurements of NCP in cryoconite holes in Svalbard and Greenland. This indicates that NCP has a negligible impact on the net creation of organic matter in cryoconite holes, and suggests instead that organic matter may be derived largely from allochthonous sources (Reference Stibal, Tranter, Benning and RehákStibal and others, 2008a; Reference HodsonHodson and others, 2010b).

Rates of photosynthesis estimated by the 14C method were typically more than an order of magnitude lower than rates of gross photosynthesis estimated by the ΔCO2 method and closer to (although not the same as) rates of NCP.

Acknowledgements

This work was funded by grants awarded to A.A. and A.H. from the UK Natural Environmental Research Council (NERC) (NE/G00496X/1 and NE/G006253/1). We thank N. Cox for all his logistical support at the NERC Arctic Station, Ny-A lesund. We also thank both the anonymous reviewers whose comments greatly improved the quality of this paper.

References

Anesio, A.M., Mindl, B., Laybourn-Parry, J., Hodson, A.J. and Sattler, B.. 2007. Viral dynamics in cryoconite holes on a high Arctic glacier (Svalbard). J. Geophys. Res., 112(G4), G04S31. (10.1029/2006JG000350.)Google Scholar
Anesio, A.M., Hodson, A.J., Fritz, A., Psenner, R. and Sattler, B.. 2009. High microbial activity on glaciers: importance to the global carbon cycle. Global Change Biol., 15(4), 955960.Google Scholar
Anesio, A.M. and 6 others. 2010. Carbon fluxes through bacterial communities on glacier surfaces. Ann Glaciol., 51(56) (see paper in this issue).Google Scholar
Baines, S.B. and Pace, M.L.. 1991. The production of dissolved organic matter by phytoplankton and its importance to bacteria: patterns across marine and freshwater systems. Limnol. Oceanogr., 36(6), 10781090.Google Scholar
Behrenfeld, M.J. and Falkowski, P.G.. 1997. A consumer’s guide to phytoplankton primary productivity models. Limnol. Oceanogr., 42(7), 14791491.Google Scholar
Bender, M. and 12 others. 1987. A comparison of four methods for determining planktonic community production. Limnol. Oceanogr., 32(5), 10851098.Google Scholar
Billen, G. 1976. Evaluation of nitrifying activity in sediments by dark 14C-bicarbonate incorporation. Water Res., 10(1), 5157.Google Scholar
Burris, J.E. 1977. Photosynthesis, photorespiration, and dark respiration in eight species of algae. Mar. Biol., 39(4), 371379.Google Scholar
Christner, B.C., Kvito, B.H. and Reeve, J.N.. 2003. Molecular identification of bacteria and eukarya inhabiting an Antarctic cryoconite hole. Extremophiles, 7(3), 177183.Google Scholar
Cullen, J.J., Neale, P.J. and Lesser, M.P.. 1992. Biological weighting function for the inhibition of phytoplankton photosynthesis by ultraviolet radiation. Science, 258(5082), 646650.CrossRefGoogle ScholarPubMed
De Smet, W.H. and van Rompu, E.A.. 1994. Rotifera and Tardigrada from some cryoconite holes on a Spitsbergen (Svalbard) glacier. Belg. J. Zool., 124(1), 2737.Google Scholar
Dring, M.J. and Jewson, D.H.. 1982. What does 14C uptake by phytoplankton really measure? A theoretical modelling approach. Proc. R. Soc. London, Ser. B, 214(1196), 351368.Google Scholar
Ferreyra, G.A., Demers, S., del Giorgio, P.A. and Chanut, J.-P.. 1997. Physiological responses of natural plankton communities to ultraviolet-B radiation in Redberry Lake (Saskatchewan, Canada). Can. J. Fish. Aquat. Sci., 54(3), 705714.Google Scholar
Fogg, G.E. 1983. The ecological significance of extracellular products of phytoplankton photosynthesis. Bot. Mar., 26(1), 314.Google Scholar
Furgal, J.A. and Smith, R.E.H.. 1997. Ultraviolet radiation and photosynthesis by Georgian Bay phytoplankton of varying nutrient and photoadaptive status. Can. J. Fish. Aquat. Sci., 54(7), 16591667.Google Scholar
Gieskes, W.W.C., Kraay, G.W. and Baars, M.A.. 1979. Current 14C methods for measuring primary production: gross underestimates in oceanic waters. Neth. J. Sea Res., 13(1), 5878.Google Scholar
Gnaiger, E. 1983. Appendix C: calculation of energetic and biochemical equivalents of respiratory oxygen consumption. In Gnaiger, E. and Forstner, H., eds. Polargraphic oxygen sensors: aquatic and physiological applications. Berlin, etc., Springer-Verlag, 337345.Google Scholar
Goto, N., Kawamura, T., Mitamura, O. and Terai, H.. 1999. Importance of extracellular organic carbon production in the total primary production by tidal-flat diatoms in comparison to phytoplankton. Mar. Ecol. Progr. Ser., 190, 289295.Google Scholar
Herndl, G.J., Müller-Niklas, G. and Frick, J.. 1993. Major role of ultraviolet-B in controlling bacterioplankton growth in the surface layer of the ocean. Nature, 361(6414), 717719.Google Scholar
Hobson, L.A., Morris, W.J. and Pirquet, K.T.. 1976. Theoretical and experimental analysis of the 14C technique and its use in studies of primary production. J. Fish. Res. Board Can., 33(8), 17151721.Google Scholar
Hodson, A.J. and 10 others. 2007. A glacier respires: quantifying the distribution and respiration CO2 flux of cryoconite across an entire Arctic supraglacial ecosystem. J. Geophys. Res., 112(G4), G04S36. (10.1029/2007JG000452.)Google Scholar
Hodson, A. and 7 others. 2008. Glacial ecosystems. Ecol. Monogr., 78(1), 4167.Google Scholar
Hodson, A.J. and 6 others. 2010a. The cryoconite ecosystem upon the Greenland Ice Sheet. Ann. Glaciol., 51(56) (see paper in this issue).Google Scholar
Hodson, A. and 6 others. 2010b. The structure, biological activity and biogeochemistry of cryoconite aggregates upon an Arctic valley glacier: Longyearbreen, Svalbard. J. Glaciol., 56(196), 349362.Google Scholar
Kana, T.M. 1990. Light-dependent oxygen cycling measured by an oxygen-18 isotope dilution technique. Mar. Ecol. Progr. Ser., 64, 293300.Google Scholar
Karl, D.M., Hebel, D.V., Björkman, K. and Letelier, R.M.. 1998. The role of dissolved organic matter release in the productivity of the oligotrophic North Pacific Ocean. Limnol. Oceanogr., 43(6), 12701286.Google Scholar
Lancelot, C. and Mathot, S.. 1985. Biochemical fractionation of primary production by phytoplankton in Belgian coastal waters during short- and long-term incubations with 14C-bicarbonate. Mar. Biol., 86(3), 227232.Google Scholar
Li, W.K.W. and Dickie, P.M.. 1991. Light and dark 14C uptake in dimly-lit oligotrophic waters: relation to bacterial activity. J. Plankton Res., 13, Suppl., s29s44.Google Scholar
Li, W.K.W., Irwin, B.D. and Dickie, P.M.. 1993. Dark fixation of 14C: variations related to biomass and productivity of phytoplankton and bacteria. Limnol. Oceanogr., 38(3), 483494.Google Scholar
Morán, X.A.G., Estrada, M., Gasol, J.M. and Pedrόs-Aliό, C.. 2002. Dissolved primary production and the strength of phytoplankton–bacterioplankton coupling in contrasting marine region. Microbial Ecol., 44(3), 217223.Google Scholar
Mueller, D.R. and Vincent, W.F.. 2006. Microbial habitat dynamics and ablation control on the Ward Hunt Ice Shelf. Hydrol. Process., 20(4), 857876.Google Scholar
Mueller, D.R., Vincent, W.F., Pollard, W.H. and Fritsen, C.H.. 2001. Glacial cryoconite ecosystems: a bipolar comparison of algal communities and habitats. In Elster, J., Seckbach, J., Vincent, W.F. and Lhotský, O., eds. Proceedings of the International Conference on Algae and Extreme Environments: Ecology and Physiology, 1116 September 2000, Téeboñ, Czech Republic . Berlin, J. Cramer/Stuttgart, Gebr. Borntraeger, 173197. (Nova Hedwigia Beiheft 123.)Google Scholar
Peterson, B.J. 1980. Aquatic primary productivity and the 14C–CO2 method: a history of the productivity problem. Annu. Rev. Ecol. Syst., 11 , 359385.Google Scholar
Porazinska, D.L., Fountain, A.G., Nylen, T.H., Tranter, M., Virginia, R.A. and Wall, D.H.. 2004. The biodiversity and biogeochemistry of cryoconite holes from McMurdo Dry Valley glaciers, Antarctica. Arct. Antarct. Alp. Res., 36(1), 8491.Google Scholar
Säwström, C., Mumford, P., Marshall, W., Hodson, A. and Laybourn-Parry, J.. 2002. The microbial communities and primary productivity of cryconite holes in an Arctic glacier (Svalbard 798N). Polar Biol., 25(8), 591596.Google Scholar
Säwström, C., Laybourn-Parry, J., Granéli, W. and Anesio, A.M.. 2007a. Heterotrophic bacterial and viral dynamics in Arctic freshwaters: results from a field study and nutrient-temperature manipulation experiments. Polar Biol., 30(11), 14071415.Google Scholar
, wström, C., Granéli, W., Laybourn-Parry, J. and Anesio, A.M.. 2007b. High viral infection rates in Antarctic and Arctic bacterioplankton. Environ. Microbiol., 9(1), 250255.Google Scholar
Stal, L.J. 2003. Microphytobenthos, their extracellular polymeric substances, and the morphogenesis of intertidal sediments. Geomicrobiol. J., 20(5), 463478.Google Scholar
Steemann-Nielsen, E. 1952. The use of radioactive carbon (14C) for measuring organic carbon production in the sea. J. Conseil Perm. Int. Explor. Mer, 18, 117140.Google Scholar
Stibal, M. and Tranter, M.. 2007. Laboratory investigation of inorganic carbon uptake by cryoconite debris from Weren-skioldbreen, Svalbard. J. Geophys. Res., 112(G4), G04S33. (10.1029/2007JG000429.)Google Scholar
Stibal, M., Tranter, M., Benning, L.G. and Rehák, J.. 2008a. Microbial primary production on an Arctic glacier is insignificant in comparison with allochthonous organic carbon input. Environ. Microbiol., 10(8), 21722178.Google Scholar
Stibal, M., Tranter, M., Telling, J. and Benning, L.G.. 2008b. Speciation, phase association and potential bioavailability of phosphorus on a Svalbard glacier. Biogeochemistry, 90(1), 113.Google Scholar
Takeuchi, N., Kohshima, S. and Seko, K.. 2001. Structure, formation, and darkening process of albedo-reducing material (cryoconite) on a Himalayan glacier: a granular algal mat growing on the glacier. Arct. Antarct. Alp. Res., 33(2), 115122.Google Scholar
Thomson, B.E., Dyke, H. and Worrest, R.C.. 1980. Impact of UV-B radiation (290–320 nm) upon estuarine bacteria. Oecologia, 47(1), 5660.Google Scholar
Tranter, M. and 6 others. 2004. Extreme hydrochemical conditions in natural microcosms entombed within Antarctic ice. Hydrol. Process., 18(2), 379387.CrossRefGoogle Scholar
Williams, P.J.LeB. and Lefèvre, D.. 2008. An assessment of the measurement of phytoplankton respiration rates from dark 14C incubation. Limnol. Oceanogr. Meth., 6(1), 111.Google Scholar
Williams, P.J.LeB. and Robertson, J.E.. 1991. Overall planktonic oxygen and carbon dioxide metabolisms: the problem of reconciling observations and calculations of photosynthetic quotients. J. Plankton Res., 13, Suppl., 153169.Google Scholar
Yallop, M.L. 1982. Some effects of light on algal respiration and the validity of the light and dark bottle technique for measuring primary productivity. Freshwater Biol., 12(5), 427433.Google Scholar
Yallop, M.L., de Winder, B., Paterson, D.M. and Stal, L.J.. 1994. Comparative structure, primary production and biogenic stabilization of cohesive and non-cohesive marine sediments inhabited by microphytobenthos. Estuar. Coast. Shelf Sci., 39(6), 565582.Google Scholar
Figure 0

Fig. 1. Location of cryoconite holes where in situ rates of photosynthesis and respiration were measured. AB = Austre Brøggerbreen, ML=Midtre Lovénbreen, VB=Vestre Brøggerbreen. Note that x and y labels are in Universal Tranverse Mercator (UTM) coordinates.

Figure 1

Table 1. Physical and chemical characteristics of cryoconite holes

Figure 2

Table 2. Rates of gross photosynthesis, respiration, NCP (all from ΔCO2 method) and 14C photosynthesis in cryoconite sediment and water incubations. Mean rates are shown with minimum and maximum rates in parentheses. Negative numbers for NCP indicate net heterotrophy; positive numbers indicate net autotrophy

Figure 3

Fig. 2. Comparison of paired measurements of rates by CO2 and O2 methods. (a) Gross photosynthesis, (b) respiration and (c) NCP. Dotted lines show typical ranges of photosynthetic and respiratory quotients (PQ and RQ) from other environments: PQ range of 1.0–1.4 (Williams and Robertson, 1991); RQ range of 0.7–1.0 (Gnaiger, 1983). Shaded areas are below the detection limit.

Figure 4

Fig. 3. Comparison of rates of photosynthesis by 14C method with (a) rates of gross photosynthesis by the ΔO2 and ΔCO2 methods and (b) rates of NCP by the ΔO2 and ΔCO2 methods. Error bars are 1 SD. Note the logarithmic scale in (a).

Figure 5

Fig. 4. Scatter plots of rates of photosynthesis measured by the 14C method vs (a) gross photosynthesis (ΔCO2 method) and (b) NCP (ΔCO2 method). Errors bars are 1 SD of triplicate measurements. Pearson’s product-moment correlation indicated no significant relationships (p<0.05) in either (a) or (b).

Figure 6

Table 3. Summary of published rates of gross photosynthesis, NCP and 14C photosynthesis in cryoconite holes