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Mercury isotope signatures of methylmercury in rice samples from the Wanshan mercury mining area, China: environmental implications Ping Li, Buyun Du, Laurence Maurice, Laure Laffont, Christelle Lagane, David Point, Jeroen E. Sonke, Runsheng Yin, Che-Jen Lin, and Xinbin Feng Environ. Sci. Technol., Just Accepted Manuscript • DOI: 10.1021/acs.est.7b03510 • Publication Date (Web): 29 Sep 2017 Downloaded from http://pubs.acs.org on September 29, 2017

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Mercury isotope signatures of methylmercury in rice samples from

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the

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implications

Wanshan

mercury

mining

area,

China:

environmental

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Ping Li†, Buyun Du†,‡, Laurence Maurice§, Laure Laffont§, Christelle Lagane§, David

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Point§, Jeroen E. Sonke§, Runsheng Yinǁ, Che-Jen Lin†,



Xinbin Feng†,*

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9

Chinese Academy of Sciences, Guiyang, 550081, China

State Key Laboratory of Environmental Geochemistry, Institute of Geochemistry,

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University of Chinese Academy of Sciences, Beijing 100049, China

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§

Observatory Midi-Pyrénées, Geosciences Environment Toulouse Laboratory,

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Research Institute for the Development (IRD), University of Toulouse and CNRS,

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31400 Toulouse, France

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ǁ

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Chinese Academy of Sciences, Guiyang, 550081, China

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State Key Laboratory of Ore Deposit Geochemistry, Institute of Geochemistry,



Center for Advances in Water and Air Quality, Lamar University, Beaumont, Texas

77710, USA

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*, Corresponding author: Feng X. ([email protected])

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ABSTRACT: Rice consumption is the primary pathway of methylmercury (MeHg)

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exposure for residents in mercury mining areas of Guizhou Province, China. In this

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study, compound-specific stable isotope analysis (CSIA) of MeHg was performed on

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rice samples collected in the Wanshan mercury mining area. An enrichment of 2.25‰

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in total Hg (THg) δ202Hg was observed between rice and human hair, and THg ∆199Hg

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in hair was 0.12‰ higher than the value in rice. Rice and human hair samples in this

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study show distinct Hg isotope signatures compared to those of fish and human hair of

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fish consumers collected in China and other areas. Distinct Hg isotope signatures were

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observed between IHg and MeHg in rice samples (in mean±standard deviation:

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δ202HgIHg at −2.30‰±0.49‰, ∆199HgIHg at −0.08‰±0.04‰, n=7; δ202HgMeHg at

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−0.80‰±0.25‰, ∆199HgMeHg at 0.08‰±0.04‰, n=7). Using a binary mixing model, it

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is estimated that atmospheric Hg contributed 31%±16% of IHg and 17%±11% of THg

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in the rice samples and the IHg in soil caused by past mining activities contributed to

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the remaining Hg. This study demonstrated that Hg stable isotopes are good tracers of

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human MeHg exposure to fish and rice consumption, and the isotope data can be used

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for identifying the sources of IHg and MeHg in rice.

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INTRODUCTION

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Mercury (Hg) and its compounds are highly toxic pollutants that can adversely

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affect human health. The toxicity of Hg depends on its chemical form. Humans are

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exposed to organic mercury through diet, and to inorganic Hg in air containing

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elevated Hg vapor caused by industrial emissions such as, coal combustion and

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artisanal gold mining or by Hg released by amalgam dental fillings. Exposure to

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dietary methylmercury (MeHg) has caused greater health concern because MeHg is

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much more toxic than inorganic Hg (IHg) and bioaccumulates more strongly than IHg

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in aquatic organisms.1,2 IHg can be readily methylated in aquatic ecosystems, and then

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accumulated as MeHg in the food chains, leading to elevated MeHg concentrations in

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fish and human exposure to MeHg through fish consumption.1

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Rice grown in contaminated soils, such as those near the closed Hg mining

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industries in Guizhou Province, China, can also contain high MeHg concentrations.3,4

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It has been found that rice paddies are hotspots of Hg methylation.5,6 MeHg in paddy

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soils are absorbed by the roots of rice plants and translocated to the leaves, stalks, and

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seeds.3 In contrast, IHg in rice plants originates from Hg uptake from soil or the

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atmosphere (mainly Hg0 uptake via foliage).7,8 Rice (rather than fish) has been

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identified as the main source of human exposure to MeHg in Guizhou Province4,9 and

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the inland area of South China.10 Health risks through co-exposure to IHg and MeHg

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are particularly of concern in Hg mining areas4 and other Hg contaminated areas of

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China. Understanding the source of Hg contamination and the pathways of human

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exposure to MeHg and IHg in these areas is critical to assess the health risks and

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implementing effective pollution control measures. 4

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Mercury stable isotope techniques are research tools to understand the sources

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and environmental processes of Hg.11,12 Mass dependent fractionation (MDF,

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quantified as δ202Hg) occurs in most physical, chemical and biological processes, such

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as

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photoreduction.17,18 The processes exhibit distinct δ202Hg signatures in IHg species

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(Hg2+ and Hg0) and MeHg. Mass independent fractionation (MIF, quantified as

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∆199Hg, ∆200Hg, and ∆201Hg) of both even and odd Hg stable isotopes can also affect

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Hg isotopic signatures of IHg and MeHg. MIF data provide useful information on the

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sources of Hg in the environment, human exposure pathways, as well as

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environmental processes (such as photochemistry) contributing to the biogeochemical

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cycle of Hg.17,19,20

microbiological

reduction,13,14

methylation,15

demethylation,16

and

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Signatures of stable Hg isotopes in environmental and biological samples have

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led to specific insights on the trophic transfer of Hg through aquatic food chains to

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fish consumers, such as humans, birds, and whales.21-28 Significant MDF does not

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occur during the trophic transfer of Hg to fish,26 but a δ202Hg increase of ~+2‰ has

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been found between fish and human hair/mammals/birds, indicating that MDF may

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occur through metabolic processes.27,

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observed in human hair and fish, which was explained by the photodegradation of

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MeHg in aquatic ecosystems before biomagnification.29-32 The absence of MIF during

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trophic transfer enables the use of MIF data for tracing Hg sources in food webs.26

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The correlations between δ202Hg (or ∆199Hg) and the MeHg fraction in total Hg (THg)

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found in aquatic food webs suggest that MeHg and IHg species may have distinct

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Positive MIF signatures have been

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isotopic signatures.33,34 This was also supported by the isotopic signature of MeHg

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found in marine biological samples using a compound-specific stable isotope analysis

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(CSIA) method.35

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The selective extraction method (SEM) for CSIA has been applied for fish

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tissues. Because fish has relatively high MeHg concentration and Hg in fish is present

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primarily as MeHg.35 However, rice samples contain relatively low MeHg

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concentrations and low fraction of MeHg3,4. In this study, a modified CSIA method

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was developed for determining the isotopic signatures of MeHg in rice samples

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collected from the Wanshan mercury mining area (WMMA), which had the largest Hg

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mining operation in China. Hg isotopes in hair samples of the residents in WMMA

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were also determined to understand the Hg exposure pathways.

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MATERIALS AND METHODS

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Samples collection. Rice and human hair samples were collected in the WMMA in

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December 2012. The study area and sampling procedure have been described

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previously.36 The Dashuixi village with a population of 100 people and 25 households

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was selected as the study site. Seven rice samples of relatively high MeHg

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concentrations and seven hair samples of large range of Hg concentrations were

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analyzed. Three male and four female subjects (with an average of 42.7 years old)

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were selected in this study. One rice sample and one hair sample were collected from

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each participating household and therefore each rice and hair samples were paired.

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Hair samples (50-100 mg) were cut with stainless steel scissors from the occipital 6

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region of the scalp. Each sample was bundled together in polyethylene bags, and then

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transferred to the laboratory for analysis. The portion of hair within 0-3 cm from the

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scalp was selected for Hg analysis to reveal the past 3 months' exposure. Uncooked

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rice samples (100 g) were collected from each participating household. The food

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consumption information for each participant (g/day) was estimated through

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face-to-face interview. The rice consumed by local residents was cultivated from their

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own land.

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Mercury concentrations and speciation. Each rice sample was air-dried, crushed,

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and passed through a 150 mesh sieve. Each hair sample was washed with nonionic

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detergent, distilled water, acetone, then dried in an oven at 60 °C overnight.37

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THg concentrations in hair and rice samples were determined using a DMA-80

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analyzer (Milestone, Italy) at the Geosciences Environment Toulouse laboratory

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(France).30 MeHg concentrations were determined by extracting the organic phase

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with tetramethylammonium hydroxide, followed by species-specific isotope-dilution

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analysis and gas chromatography inductively coupled plasma mass spectrometry.38

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Mercury isotope analysis. Between 0.1 and 0.8 g of a rice sample or between 0.01

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and 0.02 g of a hair sample (depending on the THg concentration) was digested in 5

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mL HNO3 at 120 °C for 6 h. The digest was then diluted with Milli-Q water to 15-25

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vol% acid, and adjusted to yield a reverse aqua regia solution (3:1 v/v HNO3 and HCl)

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with a THg concentration of 1 ng/g for Hg isotope analysis. The Hg stable isotope 7

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composition was determined using continuous cold vapor - multiple collector

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inductively coupled plasma mass spectrometer (CV-MC-ICPMS, Neptune, Thermo

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Fisher Scientific, USA) at the Geosciences Environment Toulouse laboratory

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following a previously published method.30 Hg MDF and MIF signatures were

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expressed relative to NIST SRM 3133 following recommended nomenclature.17

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Procedure of SEM was adapted from the method described by Masbou et al.35 An

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appropriate amount of a rice sample (0.25–0.5 g) was extracted with 5 mL acidic

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sodium bromide (30% w/w NaBr in 4 mol/L H2SO4), 10 mL aqueous cupric sulfate

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(2.5% w/w CuSO4), and 10 mL toluene in a 50mL centrifuge tube. The tube was

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shaken at 420 rpm for 1 h to transfer MeHgBr from the matrix to the toluene phase.

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The toluene phase was then removed and back-extracted with aqueous sodium

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thiosulfate solution (0.005 mol/L) to convert the MeHgBr into a stable

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MeHg-thiosulfate complex. An aliquot of the aqueous phase (containing the

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MeHg-thiosulfate complex) was transferred to a 5 mL tube and kept at 4 °C until

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analysis. For rice samples with low MeHg concentrations, the sample was extracted

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several times and the extracts were combined to obtain enough Hg in solution (1 ng/g)

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for Hg isotope analysis. Fish CRM TORT-2 (National Research Council Canada) was

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used to investigate the accuracy and precision of the SEM method.

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The THg concentration in each purified solution was determined by cold vapor

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atomic fluorescence spectroscopy (Brooks Rand Model III) at the Geosciences

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Environment Toulouse laboratory. The MeHg recoveries were calculated from the

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ratio of THg in purified solution to the initial MeHg concentrations in the rice samples. 8

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The MeHg concentration in each prepared extract was determined after aqueous

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ethylation, purging, trapping, and gas chromatography cold vapor atomic fluorescence

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spectroscopy (using a MERX instrument; Brooks Rand Instruments, USA) analysis in

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the State Key Laboratory of Environmental Geochemistry. The purity of MeHg in the

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extract was calculated from the percentage of MeHg to the THg concentration in each

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solution, and was used to determine the relative amounts of IHg impurities and to

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determine the efficiency of the extraction process.

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Each purified MeHg-thiosulfate solution was diluted with a 3:1 v/v mixture of

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HNO3 and HCl to give a final Hg concentration of 1 ng/g, MeHg CSIA was

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performed on the solution using continuous CV-MC-ICPMS.

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The stable isotopic compositions of IHg compounds were calculated from the

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isotopic mass balance differences using the THg and MeHg fractions isotopic

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compositions using equations 1 and 2:

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δ202HgTHg = δ202HgMeHg × R + δ202HgIHg × (1−R)

(1)

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∆199HgTHg = ∆199HgMeHg × R +∆199HgIHg × (1−R),

(2)

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where R is the percentage of MeHg to the THg concentration in a rice sample.

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Quality control. The quality control procedures applied to the Hg speciation analyses

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involved analyzing method blanks, spiked blanks, spiked matrix samples, certified

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reference materials (CRM), and blind duplicates. The limits of determination (LOD)

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for THg and MeHg were 0.02 and 0.003 ng/g, respectively. The mean THg

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concentration of lichen CRM (BCR482) was 475±15 ng/g (n=5), consistent with the 9

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certified concentration of 480±20 ng/g; the mean THg concentration of human hair

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CRM (NIES-13) was 4.3±0.09 µg/g (n=4), also consistent with the certified

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concentration of 4.4±0.2 µg/g. A mean MeHg concentration of 154±3.3 ng/g (n=5)

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was obtained for fish CRM TORT-2 having a certified value of 152±13 ng/g; a mean

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MeHg concentration of 3.74±0.24 µg/g (n=5) was obtained for NIES-13 having a

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certified value of 3.8±0.4 µg/g. The relative percentage differences for duplicate

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analysis of both rice and hair samples were