Although a positive relationship between atmospheric loadings of inorganic mercury (Hg(II)) to watersheds and concentrations of methyl mercury (MeHg) in fish has now been established, net wet and dry deposition of Hg(II) and MeHg to watersheds remains challenging to quantify. In this study, concentrations and loadings of total mercury (THg; all forms of Hg in a sample) and MeHg in open area wet deposition, throughfall, and litterfall were quantified atthe remote Experimental Lakes Area in the boreal ecoregion, NW Ontario, Canada. Between 1992 and 2006, mean annual THg and MeHg loadings in the open were 36 +/- 17 and 0.5 +/- 0.2 mg ha(-1), respectively. Throughfall THg and MeHg loadings were generally 2-4 times and 0.8-2 times higher, respectively, than loadings in the open. Loadings of both THg and MeHg were highest under an old growth spruce/fir canopy and lowest under a deciduous maple canopy, whereas loadings under young jack pine and wetland spruce/pine/alder canopies were intermediate. Litterfall generally represented the largest input of THg (86-105 mg ha(-1)) and MeHg (0.7-0.8 mg ha(-1)) to the landscape on an annual basis. Using the "direct" method of estimating dry deposition (thoughfall + litterfall - open loadings), we calculated that annual dry deposition of THg and MeHg under forest canopies ranged from 105 to 201 mg ha(-1), whereas dry deposition of MeHg ranged from 0.7 to 1.2 mg ha(-1). Photoreduction and emission of wet-deposited Hg(ll) from canopy foliage were accounted for, resulting in 3-5% (5-6 mg ha(-1)) higher annual estimates of dry deposition than via the direct method alone. NetTHg and MeHg loadings to this remote landscape were lower than at any other previously studied forested site globally. This study shows that THg and MeHg loading can be extremely variable within a heterogeneous boreal landscape and that processes such as Hg photoreduction and emission from foliage should be considered when estimating dry deposition of Hg.
The forest canopy was an important contributor to fluxes of methyl mercury (MeHg) and total mercury (THg) to the forest floor of boreal uplands and wetlands and potentially to downstream lakes, at the Experimental Lakes Area (ELA), northwestern Ontario. The estimated fluxes of MeHg and THg in throughfall plus litterfall below the forest canopy were 2 and 3 times greater than annual fluxes by direct wet deposition of MeHg (0.9 mg of MeHg ha(-1)) and THg (71 mg of THg ha(-1)). Almost all of the increased flux of MeHg and THg under the forest canopy occurred as litterfall (0.14-1.3 mg of MeHg ha(-1) yr(-1) and 110-220 mg of THg ha(-1) yr(-1)). Throughfall added no MeHg and approximately 9 mg of THg ha(-1) yr(-1) to wet deposition at ELA, unlike in other regions of the world where atmospheric deposition was more heavily contaminated. These data suggest that dry deposition of Hg on foliage as an aerosol or reactive gaseous Hg (RGM) species is low at ELA, a finding supported by preliminary measurements of RGM there. Annual total deposition from throughfall and litterfall under a fire-regenerated 19-yr-old jack pine/birch forest was 1.7 mg of MeHg ha(-1) and 200 mg of THg ha(-1). We found that average annual accumulation of MeHg and THg in the surficial litter/fungal layer of soils since the last forest fire varied between 0.6 and 1.6 mg of MeHg ha(-1) and between 130 and 590 mg of THg ha(-1) among sites differing in drainage and soil moisture. When soil Hg accumulation sites were matched with similar sites where litterfall and throughfall were collected, measured fluxes of THg to the forest floor (sources) were similar to our estimates of longterm soil accumulation rates (sinks), suggesting that the Hg in litterfall and throughfall is a new and not a recycled input of Hg to forested ecosystems. However, further research is required to determine the proportion of Hg in litterfall that is being biogeochemically recycled within forest and wetland ecosystems and, thus, does not represent new inputs to the forest ecosystem.
The overall objectives of this study were to examine the effects of flooding on the decomposition and mercury (Hg) content of tissues from plants common to boreal upland forests at the Experimental Lakes Area in northwestern Ontario. We used litterbags to study changes in total Hg (THg), methyl Hg (MeHg), carbon (C), and nitrogen (N) in 12 different plant tissues (birch, alder, blueberry, and Labrador tea leaves, bunchberry plants, jack pine needles, Sphagnum spp., Polytrichum spp., and Pleurozium spp. bryophytes, lichen, and fresh and extensively decomposed wood) placed on unflooded boreal forest soils and in experimentally created reservoirs over an approximately 800 day period. Rates of decomposition (as indicated by differences in the percentage of C and N mass left in the tissues over time) were slower in plant tissues placed on unflooded soils compared to the same tissues that were inundated in reservoirs. Depending on tissue type and initial THg concentrations, decomposing litter on both unflooded and flooded soils was either a source or a sink for THg. Tissues where initial THg concentrations were greater than 30 ng g(-1) represented a source of THg to the surrounding environment, whereas tissues that had initial concentrations of less than 30 ng g(-1) gained THg mass. Initial rates of change in THg were more rapid in plant tissues placed in reservoirs compared to the same plant tissue placed on unflooded soils, but there were no differences in final THg masses after approximately 800 days. Plant tissues placed in reservoirs exhibited large increases in MeHg mass, whereas MeHg mass decreased in the same plants placed on unflooded soils. This is the first study examining THg and MeHg cycling in decomposing plants in upland boreal forests and reservoirs.
Mercury speciation, controls on methylmercury (MeHg) production, and bed sediment-pore water partitioning of total Hg (THg) and MeHg were examined in bed sediment from eight geochemically diverse streams where atmospheric deposition was the predominant Hg input. Across all streams, sediment THg concentrations were best described as a combined function of sediment percent fines (%fines; particles < 63 µm) and organic content. MeHg concentrations were best described as a combined function of organic content and the activity of the Hg(II)-methylating microbial community and were comparable to MeHg concentrations in streams with Hg inputs from industrial and mining sources. Whole sediment tin-reducible inorganic reactive Hg (Hg(II) R ) was used as a proxy measure for the Hg(II) pool available for microbial methylation. In conjunction with radiotracer-derived rate constants of 203 Hg(II) methylation, Hg(II) R was used to calculate MeHg production potential rates and to explain the spatial variability in MeHg concentration. The %Hg(II) R (of THg) was low (2.1 ( 5.7%) and was inversely related to both microbial sulfate reduction rates and sediment total reduced sulfur concentration. While sediment THg concentrations were higher in urban streams, %MeHg and %Hg(II) R were higher in nonurban streams. Sediment pore water distribution coefficients (log K d 's) for both THg and MeHg were inversely related to the log-transformed ratio of pore water dissolved organic carbon (DOC) to bed sediment %fines. The stream with the highest drainage basin wetland density also had the highest pore water DOC concentration and the lowest log K d 's for both THg and MeHg. No significant relationship existed between overlying water MeHg concentrations and those in bed sediment or pore water, suggesting upstream sources of MeHg production may be more important than local streambed production as a driver of water column MeHg concentration in drainage basins that receive Hg inputs primarily from atmospheric sources.
With increasing input of neurotoxic mercury to environments as a result of anthropogenic activity, it has become imperative to examine how mercury may enter biotic systems through its methylation to bioavailable forms in aquatic environments. Recent development of stable isotope-based methods in methylation studies has enabled a better understanding of the factors controlling methylation in aquatic systems. In addition, the identification and tracking of the hgcAB gene cluster, which is necessary for methylation, has broadened the range of known methylators and methylation-conducive environments. Study of abiotic factors in methylation with new molecular methods (the use of stable isotopes and genomic methods) has helped elucidate the confounding influences of many environmental factors, as these methods enable the examination of their direct effects instead of merely correlative observations. Such developments will be helpful in the finer characterization of mercury biogeochemical cycles, which will enable better predictions of the potential effects of climate change on mercury methylation in aquatic systems and, by extension, the threat this may pose to biota.
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