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Blueprint for Children?s Health and the Built Environment Presented by the Children's Environmental Health Institute

Green Chemistry & Environmental Health

Comparative Toxicogenomics Database (CTD)

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Environmental Health Perspectives Volume 115, Number S-1, December 2007 Open Access
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Fish as Biomonitors of Polybrominated Diphenyl Ethers and Hexabromocyclododecane in Czech Aquatic Ecosystems: Pollution of the Elbe River Basin

Jana Pulkrabová, Jana Hajslová, Jan Poustka, and Radek Kazda

Institute of Chemical Technology, Department of Food Chemistry and Analysis, Prague, Czech Republic

Abstract
Background: Brominated flame retardants (BFRs) —polybrominated diphenyl ethers (PBDEs) and hexabromocyclododecane (HBCD) —belong to the group of relatively "new" environmental contaminants. The occurrence of these compounds in the Czech aquatic ecosystem was for the first time documented within the 3-year monitoring study initiated in 2001.

In 2002–2003 HBCD and the major PBDE congeners (28, 47, 49, 66, 85, 99, 100, 153, 154, and 183) were found in 136 freshwater fish samples collected from several sampling sites located at three Czech rivers (Vltava, Elbe, Tichá Orlice) . Chub (Leuciscus cephalus) , barbel (Barbus barbus) , bream (Abramis brama) , perch (Perca fluviatilis) , and trout (Salmo trutta) , representing the most common fish species, were examined by gas chromatography coupled with negative chemical ionization mass spectrometry.

Results: The presence of PBDE congeners and HBCD was detected in all analyzed samples (limits of detection for target analyts ranged from 0.015 to 0.1 ng/g lipid weight) . Without exception the dominating congener was BDE-47. The most pronounced extent of fish contamination was found in the Vltava river at Klecany, downstream from the industrial agglomeration of Prague. As for fish species, the highest concentrations of PBDEs (sum of congeners) were measured in benthic species, represented by bream and barbel, up to 19.6 ng/g wet weight and 16.5 ng/g wet weight, respectively. The lowest accumulation occurred in predator fish (perch and trout) . The highest levels of HBCD were detected in barbel from Srnojedy on the Elbe River (15.6 ng/g wet weight) , downstream.

Key words: , , , , , . Environ Health Perspect 115(suppl 1) : 28–34 (2007) . doi:10.1289/ehp.9354 available via http://dx.doi.org/ [Online 8 June 2007]

Address correspondence to J. Hajslová, Institute of Chemical Technology, Department of Food Chemistry and Analysis, Technická 3, 166 28 Prague 6, Czech Republic. Telephone/fax: 420 220 443 185. E-mail: jana.hajslova@vscht.cz

Funding was provided by European Union project QLRT-2001-00596 FIRE (flame retardants interated risk assessment for endocrine disruption) and a project of the Ministry of Education, Youth and Sports of the Czech Republic (MSM 6046137505) . This financial support is gratefully acknowledged.

The authors declare they have no competing financial interests.

Received 22 May 2006 ; accepted 26 September 2006.

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Introduction

In the recent decade several monitoring studies have started to focus on not only "classic" persistent organic pollutants (POPs), such as polychlorinated biphenyls (PCBs), organochlorinated pesticides (OCPs), and/or polychlorinated dibenzodioxins/polychlorinated dibenzofurans (PCDDs/PCDFs) but also on other groups of halogenated xenobiotics such as brominated flame retardantds (BFRs). These chemicals are used mainly as additives in polymers to prevent them from catching fire (de Wit 2002; Hale et al. 2003). Generally, two types of BFRs can be distinguished: a) reactive compounds, for instance tetrabromobisphenol A (TBBPA), are incorporated by covalent binding into polymeric matrix and b) additive BFRs, represented by polybrominated diphenyl ethers (PBDEs), hexabromocyclododecane (HBCD), and/or polybrominated biphenyls (PBBs), are merely dissolved in polymeric material. Although TBBPA is used mainly in North America, the production of PBDEs prevails in Europe (de Wit 2002; Rahman et al. 2001).

Products based on penta-, octa-, and decabromodiphenyl ethers are currently the only commercially interesting PBDEs (de Boer et al. 2000a). They are used in the housing and electronic parts of television sets or personal computers and also in textiles [de Wit 2002; World Health Organization (WHO) 1994, 1997]. PentaBDEs are mainly applied in textiles and polyurethane foams, whereas decaBDEs are used in textile as well as in many other kinds of synthetic plastics such as polyester used for electronic circuit boards (de Wit 2002; Petterson and Karlsson 2001). HBCD is used in foams and expanded polystyrene and final products such as upholstered furniture, interior textiles, and packaging material (de Wit 2002).

The occurrence of BFRs in various environmental compartments is of great concern because of their high lipophility (log Kow is between 5 and 10) and/or high resistance to degradation processes (Haglund et al. 1997). Although the first reports on a presence of PBDEs in both abiotic and biotic matrices were published as early as the late 1970s [see Zweidinger et al. (1979) for early data on air particles] and the beginning of the 1980s [see Andersson and Blomkvist (1981) concerning fish from Swedish rivers], intensive investigation into their occurrence in the environment started a decade later. Various PBDE congeners were found in Dutch (de Boer et al. 2000b), Swedish (Haglund et al. 1997; Sellström et al. 1993, 1998), Japanese (Ohta et al. 2002; Watanabe et al. 1987), British (Allchin et al. 1999), and Canadian (Alaee et al. 1999) fish samples. Similarly, these brominated POPs were also detected in sediments, wastewaters, and air (Allchin et al. 1999; de Boer et al. 2003; Sellström et al. 1998). BFRs may be released into the environment from many sources such as a) landfills (additive types may leach out); b) emissions originated during incineration processes (brominated dioxins and furans may originate under these conditions) (de Wit 2002); and/or c) effluents from sewage treatment plants (STPs), and communal and industrial wastes.

Like other POPs, the BFR group is the subject of a wide range of toxicologic and ecotoxicologic studies. Some of these studies classified these chemicals as endocrine disruptors. These substances may exhibit adverse effects on the regulation of thyroid hormone and induce immunotoxicity. They also induce neurotoxicity, causing interferences at sensitive periods of brain development (de Boer et al. 2000a; Rahman et al. 2001).

The goal of the present study, which is the first conducted in the Czech Republic, was to recognize the extent of contamination by PBDEs and HBCD in aquatic ecosystems. Several fish species common to the Czech rivers Vltava, Elbe, and Tichá Orlice were used as biomonitors for this purpose.

Materials and Methods

Sample collection. Five fish species—chub, barbel, bream, perch, and trout—were caught at several sampling sites at three Czech rivers (Vltava, Elbe, and Tichá Orlice) during 2001–2003 and were delivered to the laboratory in edible form (fillets). Before storage at –18°C, fish samples were pooled according to fish weight and length (parameters correlating with age of the fish). Typically one pooled sample was prepared from three to five individual fish. Lipid content was determined in each composite sample using extraction by n-hexane: dichlormethane (1:1, vol/vol). The characteristics of examined samples are summarized in Tables 1 and 2; sampling sites are shown in Figure 1.

Characterization of fish used as biomonitors. The fish used as biomonitors in the present study represented a spectrum of freshwater species typically found in Czech aquatic ecosystems. Chub (Leuciscus cephalus) is a relatively abundant fish found in Czech rivers and is suitable as a bioindicator of contamination in aquatic ecosystems. This omnivorous species grows slowly, and its mean lipid content in muscle is about 2.5%. Barbel (Barbus barbus) and bream (Abramis brama) have high lipid content in muscle (up to 7%); for this reason they are able to bioaccumulate lipophilic organic pollutants to a large degree. These fish live in close contact with benthic sediments. Perch (Perca fluviatilis) and trout (Salmo trutta) belong to a group of predators, and their lipid content in fillet is relatively low (not more than 1%). The fish were treated humanely and with regard for alleviation of suffering.

Chemicals. Standard solutions containing PBDE congeners (concentration 50 µg/mL in nonane) are 2,4,4´-triBDE (BDE-28); 3,4,4´-BDE (BDE-37); 2,2´,4,4´-tetraBDE (BDE-47); 2,2´,4,5´-tetraBDE (BDE-49); 2,3´,4,4´-tetraBDE (BDE-66); 2,2´,3,4,4´-pentaBDE (BDE-85); 2,2´,4,4´,5-pentaBDE (BDE-99); 2,2´,4,4´,6-pentaBDE (BDE-100); 2,2´,4,4´,5,5´-hexaBDE (BDE-153); 2,2,4´,4,5´,6´-hexaBDE (BDE-154); 2,2´,4,4´,5´,6-BDE (BDE-183) and deca-BDE (BDE-209). All were obtained from Cambridge Isotope Laboratories (≥ 98% pure; CIL, Andover, MA, USA). Working standard solutions were prepared in isooctane and were stored in a refrigerator (5°C). The α-HBCD standard (50 µg/mL in toluene) with declared purity of 98% was supplied by CIL. A standard solution of PCB-112 (10 µg/mL in isooctane) was purchased from Gr. Ehrenstorfer GmBH (Augsburg, Germany).

The organic solvents (hexane, cyclohexane, isooctane) declared as organic trace analysis grade were supplied by Merck (Darmstadt, Germany). Ethylacetate and dichloromethane were obtained from Scharlau (Barcelona, Spain). Anhydrous sodium sulfate, supplied by Penta Chrudim (Chrudim, Czech Republic), was heated at 600°C for 5 hr, then stored in a desiccator before use. Styrene–divinylbenzene gel (Bio Beads S-X3, 200–400 mesh) was purchased from Biorad Laboratories (Hercules, CA, USA). Sulfuric acid (98%) was obtained from Merck.

Instruments. We used a homogenizer (model 2094; Foss Tecator, Hilleroed, Denmark) to homogenize fish samples. For the extraction step, we used the Soxhlet extractor Gerhart 173200 EV (Gerhart, Königswinter, Germany) with a cellulose extraction thimble (Whatman, Brentford, UK).

An automated gel permeation chromatography (GPC) system consisting of 350 MASTER pump, fraction collector, automatic regulator of loop XLI, microcomputer (software 731 PC via RS32C), dilutor 402 (GILSON, Villiers le Bel, France), and stainless steel column 500 x 8 mm inner diameter (i.d.) packed with Bio-Beads S-X3 (soft gel) was used for a cleanup of crude extracts.

A vacuum evaporator (Büchi Rotavapor R-114) and water bath (B-480) (Büchi, Postfach, Switzerland) were used for concentration of extracts.

We used an Agilent 6890 gas chromatograph equipped with electronic pressure control (EPC), split/splitless injector, and coupled to a mass selective detector Agilent 5973 (Agilent Technologies, CA, USA). Capillary columns used were the a) DB-XLB column (30 m x 0.25 mm i.d. x 0.1-µm film thickness), and b) BD-XLB (15 m x 0.25 mm i.d. x 0.1-µm film thickness (all from J&W Scientific, Folsom, CA, USA) were employed for separation of PBDEs and HBCD.

Extraction of fish samples. Thirty grams of homogenous fish muscle were mixed with 120 g anhydrous sodium sulfate to form a flowing powder. The sample was transferred into a cellulose extraction thimble and stored in a desiccator for 12 hr to complete the desiccation process, then inserted into a Soxhlet apparatus and extracted for 8 hr (seven cycles per hour) with 340 mL solvent mixture n-hexane:dichlormethane (1:1, vol/vol). The crude extract was carefully evaporated by rotary vacuum evaporator, and the residual solvents were removed by a gentle stream of nitrogen. The lipid content was determined gravimetrically using the analytical balance A&D MH–300 (A&D Co., Tokyo, Japan) with 0.001-g accuracy.

Cleanup. Extracted lipids were dissolved in 10 mL of cyclohexane:ethylacetate mixture (1:1, vol/vol) containing 5 ng/mL PCB-112 (this congener is not present in commercial mixtures or environmental samples); this was considered the recovery standard. Two milliliters of this solution (corresponding to 6 g wet sample) were loaded onto a GPC column. The mobile phase was cyclohexane: ethylacetate (1:1, vol/vol) with a flow rate of 0.6 mL/min. The fraction corresponding to the elution volume of 14–30 mL was collected. The eluate was evaporated by rotary vacuum evaporator, and the residual solvents were carefully eliminated by a gentle stream of nitrogen to dryness. The residue was then dissolved in 1 mL isooctane containing 1 ng/mL BDE-37 (3,4,4´-BDE) as syringe standard and treated with concentrated sulfuric acid (approximately three drops) to remove residual lipids. After 10 min of compete phase separation, an aliquot of the upper organic (isooctane) layer was taken and transferred into a glass vial for subsequent gas chromatography (GC )analysis.

GC analysis. We used a high-resolution GC (HRGC) unit resolution mass-selective detector (MSD) for analyses of the PBDEs and HBCD in purified extracts. The GC conditions (column 1) were as follows: column temperature program, from 105°C (hold 2 min) to 300°C at 20°C/min (hold 5 min); carrier gas, helium (Linde, Prague, Czech Republic) with a constant flow of 1.5 mL/min; injection temperature, 275°C; injection volume, 1 µL using pulsed splitless injection mode (splitless time, 2 min). An MSD with quadrupole analyzer was operated in a selective ion-monitoring (SIM) mode in a negative chemical ionization (NCI). Monitored ions (m/z) were 79, 81, 159, and 161 (PBDEs); 79, 81, 158, and 160 (HBCD); and 326 and 328 (PCB-112, internal standard). Ion m/z 79 was used to quantify all target analytes. Methane was used as a reagent gas (purity 99.995%, Linde) and was set at a pressure 2 x 10–4 mbar. Ion source temperature was 150°C and quadrupole temperature 105°C.

We monitored the presence of decaBDE using the same GC coupled with negative chemical ionization mass spectrometry (GC/MS-NCI) employing a shorter column (column 2). The temperature program was as follows: from 80°C (hold 2 min) to 280°C at 20°C/min and to 320°C at 5°C/min (hold 5 min); carrier gas, helium with constant flow 3 mL/min; injection temperature, 285°C; injection volume, 1 µL using pulsed splitless injection mode (splitless time, 2 min). Monitored ions were m/z 485 and 487; the ion at m/z 487 was used for quantification.

We identified the target analytes by comparing their retention times with retention times of standards and by MS confirmation. For quantification, a multilevel calibration curve was used (at least 5 points for each congener).

Quality assurance. For each extraction batch (consisting of five fish samples), one procedure blank was processed. The results were corrected for blank interferences and for recovery (PCB-112 was added as surrogate before GPC cleanup). Limit of detection (LOD) was calculated as quantity of analyte that generates a response 3 times greater than the noise level of the detection system. Limits of quantification (LOQs) were the minimum concentrations of analytes possible to quantify with acceptable accuracy and precision. Under these conditions, the LOQ was the lowest calibration level and corresponded for particular analyte to 3 x LOD.

LOD values (nanograms per gram lipid weight) for fish were BDE-28, 0.015; BDE-47, 0.015; BDE-49, 0.015; BDE-66, 0.015; BDE-85, 0.02; BDE-99, 0.015; BDE-100, 0.015; BDE-153, 0.02; BDE-154, 0.015; BDE-183, 0.015; BDE-209, 2.0; and HBCD, 0.1.

For recovery testing of the overall analytical method, chub muscle was spiked at level 2 ng/g (of each analyte) by 100 µL standard mixture (500 ng/mL) in acetone. Real-life samples were also analyzed to obtain background levels of analytes. PBDE recoveries ranged between 83–101%, and recovery of HBCD was 91%. Acceptable recovery rate was 80–110%. We also determined the precision of the analytical method (repeatability) by analyzing six spiked fish samples; repeatability ranged from 4 to 12% (expressed as relative SD). Recovery of BDE-209 was 78 ± 3% (n = 6). Chub muscle samples spiked at 20 ng/g wet weight and were analyzed within the validation process. The method we used is fully validated. The repeatability of our results is documented by our participation in certification study BROC (biological reference materials for organic contamination) (van Leeuwen et al. 2006).

Results and Discussion

As mentioned previously, fish is widely used as a biomonitor of bioavailable POPs that occur in aquatic environments. However, interpretation of obtained data is not simple. Both bioaccumulation and depuration processes may take place in aquatic biota simultaneously, and the ratio of their intensities may differ widely among the fish species. It should be noted that the concentration of POPs measured in their bodies is dependent on many factors such as age, sex, and/or feeding habits of particular resident species. In practice it is difficult to obtain homogenous sets of biomonitors from an entire river. Differences exist among sampling localities in terms of food availability, causes of variations of fat content, and hence varying accumulation potential in fish. Table 3 is a summary of fish characteristics and the results (based on wet weight) of target PBDEs and HBCD (sum of isomers) in collected samples. It should be noted that technical HBCD mixtures consist of three diastereomers—α, β, and γ—the last being the typically dominating component (up to 80%) of this primary polluting material. In other words, biotransformation of γ-HBCD may occur in biota, resulting in a changed contamination pattern, which may lead under certain circumstances (e.g., biomagnification) to α-HBCD becoming the dominant component in the diastereomers profile. One should be aware that under GC conditions (hot injection), thermal conversion of γ-HBCD yielding α-diastereomer also may occur. Therefore, in most studies using GC for quantification, α-diastereomer is used as the calibration standard representing HBCD groups. For determination of all individual HBCD diastereomers, LC/MS must be used (Morris et al. 2004).

Table 3 shows that in all examined fish samples, the major PBDE congener was BDE-47. Levels of this 2,2´4,4´-tetrabromodiphenyl ether were approximately one order of magnitude higher than those of other monitored congeners. This was not surprising, as BDE-47 was a main component in various kinds of technical mixtures (e.g., Bromkal 70-5DE) commonly used in industry. As in our samples, this congener typically makes the major contribution to the total PBDE content in the environmental samples collected in Europe. Pentabromodiphenyl ether congeners BDE-99 and BDE-100, and hexabromodiphenylether congeners BDE-153 and BDE-154 were also present in most samples. The levels of these congeners exceeded the LOD in 70% of fish, and at least one of these PBDEs was detected. The presence of BDE-49 was confirmed in only about 10% of the samples; BDE-66 and BDE-183 were not detected in any sample. In accordance with similar studies (de Boer et al. 2003; Eljarat et al. 2004, 2005), no detectable decabromodiphenyl ether (congener 209) was present in any examined fish sample. According to several authors (Geyer et al. 1999; Sellström et al. 1998), the superlipophilic nature of this chemical (log Kow ~ 10) might be responsible for the lack of detection. BDE-209 can be strongly bound to sediments, hence its actual dissolved concentration in water is very low, and thus only a negligible fraction of this BFR is expected to be bioavailable to fish. As discussed by Eljarat et al. (2005), the low bioaccumulation potential of this chemical is due to its large molecular size that hinders a passage over membranes (Andersson and Blomkvist 1981). The alternative explanation of minimal occurrence of the deca-BDE congener in aquatic organisms is its rapid excretion and/or biotransformation after entering their body (Eljarrat et al. 2005; Eriksson et al. 2004). Regardless, BDE-209 is a relatively labile substance that easily decomposes under environmental conditions in yielding a large range of lower brominated congeners in addition to other bromine-containing products when illuminated by sunlight (Eriksson at al. 2004; Söderström et al. 2004).

The presence of HBCD in fish collected in 2002 and 2003 was detected in more than 80% of tested samples, with the highest contamination found in fish species from Srnojedy (Elbe River). Figure 2A,B shows examples of concentrations of BDE-47, other ΣPBDEs (congeners 28, 49, 85, 99, 100, 153, and 154), and HBCD in chub from all sampling localities. The average concentration of BFRs in fish from Klecany at Vltava River (aggregated data obtained within the monitoring period) was almost 5 times that of samples obtained in Podolí upstream from Prague. The data obtained by analysis of chub from the Elbe River in 2001–2003 indicated that Srnojedy, located downstream from Pardubice (a large industrial area) was the most polluted locality along the Elbe River.

Figure 1

Figure 1. The sampling sites on the Czech rivers.

Figure 2

Figure 2. Concentration of BDE-47, other ΣPBDEs (BDE-28, -49, -66, -99, -100, -153, and -154), and HBCD in chub samples from sampling sites (ng/g wet weight). Error bars represent mean ± SD. (A) River Vltava and (B) River Elbe.

Figure 3

Figure 3. Comparison of BDE-47, other ΣPBDEs (BDE-28, -49, -66, -99, -100, -153, and -154), and HBCD levels in tested fish species in Hrensko on the Elbe river (ng/g wet weight) from 2001 to 2003. Error bars represent mean ± SD.

Figure 4

Figure 4. Pattern of PBDE congeners in various fish species in Elbe-Hrensko. Error bars represent mean ± SD.

Figure 5

Figure 5. Comparison of PBDE and PCB content in fish collected in six sampling localities (aggregated data).

Table 1.

Table 1

Table 2.

Table 2

Table 3.

Table 3

Table 4.

Table 4

In Hluboká n/V (Vltava River) and Hrensko (Elbe River), no significant variation among the monitoring years was found, whereas the concentrations of BFRs in the lower part of the Elbe River were largely variable (Figure 2B). In addition to being caused by increasing pollution, this trend might be attributed to differences of seasonal flows in this part of Elbe River for individual years. Extreme floods in 2002 were probably accompanied by the removal of contaminated sediments from monitored localities in the upper part of the Elbe River and the apparent drop of aquatic ecosystem pollution, hence reduction of fish exposure to bioaccumulatively chemicals. On the other hand, the total rainfall in the upper part of the Elbe River basin in 2003 were below the long-term average values (ELbe InformationsSystEm 2006) and the flow was low. Because of the existence of permanent emission sources (industrial wastes) of PBDEs and HBCD along the upper part of the Elbe River, the increases in pollution at monitoring localities occurred again in the following year.

Figure 3 shows large differences in the extent of PBDE and HBCD bioaccumulation among the examined fish species. It is important to note that regardless of the monitoring year and sampling place, the concentrations of these BFRs (based on wet weight) were found in the following order: barbel > bream > chub > perch. de Boer and Brinkman (1994) and Geyer et al. (1999) have shown that the contribution of persistent organohalogen compound buildup in the food chain becomes relevant when log Kow values are > 5–6.5. Because log Kow values of major PBDE congeners monitored in our study range from 5.5 to 7, biomagnification of these chemicals (i.e., their transfer within the trophic levels of examined fish species that leads to a stepwise increase in contamination) might be expected. Similarly, higher levels of PBDEs in lipids were, for example, found in bass, a predator fish (collected in Penobscot River in central Maine), compared with those in white sucker, a benthic feeder, from the same locality (Anderson and MacRae 2006). Conversely, the lowest extent of contamination (regardless of the expression of BFR content on wet weight or lipids) was found in perch, which represent the highest trophic level among the fish examined in our study. Similar trends were also reported in other studies (Table 4). For example, Covaci et al. (2006) showed that the concentration of PBDEs in benthic bream from the Danube delta in Romania was about 50% higher than that in predator perch from the same locality. This controversy could be attributed to differing fat content in these two species, which is in addition to other factors related to differences in their feeding habits. Another reason for the lower concentration of PBDEs in predator species such as perch might be the fish's higher growth rate (the ratio between weight and age), leading to "dilution" of accumulated pollutants because of a rapid increase of fish muscle tissue. Generally, slow-growing fish species are exposed to polluted environments for a longer time. Moreover, in the case of benthic species (represented in our study by barbel and bream), intensive contact with highly contaminated sediments is also considered a factor in the higher levels of their contamination (Covaci et al. 2006).

Substantial differences were observed between the contamination pattern of perch and other fish species. Figure 4 shows aggregated data obtained for four experimental biomonitors collected in Hrensko (Elbe River) in two monitoring years, 2001 (before floods) and 2003 (after floods, low rainfalls). As illustrated in the figure, the spectrum of PBDEs (regardless of their total concentrations, see Table 3) was almost identical to that found in omnivorous and benthic fish with distinctly dominating BDE-47 (40–75% of the total PBDE content). In perch the content of BDE-99 was equal to or even higher than that of BDE-47. Their contribution to the total PBDEs ranged between 30 and 40% and 25 and 45%, respectively. In most studies (Covaci et al. 2005; Luross et al. 2002; Sellström et al. 1998; de Boer et al. 2003), the dominanting congeners were also BDE-47, BDE-99, and BDE-100. On the other hand, in Spanish studies by Eljarat et al. (2004 and 2005), hexa-BDEs (BDE-153 and BDE-154) as well as hepta-BDE (183) were the most abundant BFRs occurring in fish (barbel and bream) samples. Probably less common PBDE technical mixtures were released into the aquatic environment.

In Figure 5 the mean values of PBDE content (aggregated data) are compared with PCB levels (ΣPCB, PCB-28, -52, -101, -118, -138, -153, and -180) determined in the same fish samples in a parallel study concerned with chlorine-containing POPs (Pulkrabová J, Suchan P, Kocourek V, Hajslová J, Pudil F. Unpublished data 2006). Typically, the content of PCBs in biomonitors was higher by one order of magnitude and generally did not correlate with the extent of contamination in by PBDEs in particular localities. Differences in pollution sources were documented by large variations in the PCB/PBDE ratios calculated for individual fish species. Barbel showed the tendency of fish species to accumulate more PCBs than PBDEs (in Klecany, this phenomenon was not pronounced, with the PCB/PBDE ratio of 59). The correlation coefficient characterizing the relationship between the 10 ΣPBDE congeners and the 7 indicator ΣPCB congeners in all examined fish species was 0.39 (p < 0.05). It is reasonable to believe that such low correlation clearly indicates the independence of PBDEs and organochlorine compounds as sources of pollution.

Disscusion

In North-East Atlantic coastal ecosystems, levels of BFR compounds generally decreased as a function of increasing latitude (Figures 2 and 3). The obvious reason for this is that the use and leakage of BFRs into the environment is higher in urbanized areas along the Norwegian coast than in the almost unpopulated Spitsbergen. High levels of BFRs have been reported in sewage [see review by Law et al. (2006a)], and the source of BFRs in the southern part of the study area is most likely local discharges from urban sewage and industrial activity. Because of their semivolatile properties, POPs are subject to long-range atmospheric transport (Wania and Mackay 1993, 1996), and this is thus most likely the origin of the BFRs detected in endemic Arctic biota.

The finding herein—that levels of BFRs are lower in marine Arctic ecosystems than in temperate marine ecosystems—is also in accordance with previous reports in marine mammals. Data compiled on PBDEs in marine mammals from temperate environments and from the Canadian Arctic showed that levels of PBDEs were about 1,000 times higher in marine mammals from temperate marine ecosystems than in ringed seals from the Arctic (Ikonomou et al. 2002). Furthermore, levels of Σ;PBDEs (BDE-17, BDE-47, BDE-49, BDE-99, BDE-100, BDE-119, BDE-140, BDE-153, BDE-154, BDE-183) in harbor porpoises also decreased as a function of increasing latitude along the Norwegian coast, and were lower in animals from Iceland than from Norway (Thron et al. 2004). Concentrations of polychlorinated biphenyls (PCBs) in seawater in the North-East Atlantic have been shown to decrease as function of increasing latitude (Sobek and Gustafsson 2004). This confirms that levels of POPs in marine biota generally decrease as a function of the distance from the release areas.

When we compare organisms that occupy similar trophic levels, the Arctic is still a pristine environment with respect to organohalogenated anthropogenic compounds. This is contrary to the beliefs of many politicians, governmental bureaucrats, and nongovernmental organizations, who, because of the particularly high levels of PCBs reported in polar bears (Ursus maritimus), seem to believe that the Arctic is heavily polluted by POPs. The high levels of PCBs in polar bears are attributed to the fact that this species is an apex predator that feeds almost exclusively on the blubber of seals (Derocher et al. 2002). Thus, because of biomagnification of the most persistent PCB congeners from seals to polar bears, levels of Σ;PCB in polar bears become very high (Bernhoft et al. 1997; Skaare et al. 2002). Levels of all BFR compounds analyzed herein (except for BDE-153) were lower in polar bears than in its main prey species, the ringed seal (Sørmo et al. 2006), most likely because the polar bear has a high ability to metabolize POPs (Letcher et al. 1996).

The clear latitudinal decrease in levels of BFRs was not that pronounced in the two tern species compared with the other species included in the study (Figures 2 and 3). This is most likely linked to the fact that the terns are migratory birds, whereas the other species are endemic to their regions. During their migration from Africa (common tern) and Antarctica (arctic tern), they feed along the highly urbanized and thus more polluted coasts of Europe. Therefore, even though the terns may metabolize and excrete some of the BFR compounds during their migration via urbanized and industrialized polluted areas, levels still seem to be relatively high when they reach their breeding areas. Because migration is energetically costly, the birds will have to build up lipid stores for egg laying when arriving at their breeding sites. Thus, because levels of POPs are lower in prey at more northern breeding sites, body burdens of POPs in female birds will be diluted, resulting in the latitudinal decrease of BFR compounds in their eggs reported herein. When the eggs are laid, the lipophilic BFRs are transferred from the female to her eggs.

The high levels of HBCD reported in common tern eggs from the Netherlands [330–7,100 ng/g lw (Morris et al. 2004)] occur most likely because specimens that breed here are exposed to higher concentrations for a longer period of time than specimens that only transiently pass the Netherlands en route to Norway and the Arctic.

In another study on kittiwakes (Rissa tridactyla), levels of the sum of 23 PCB congeners and the Σ;PBDEs (BDE-28, BDE-47, BDE-99, BDE-100, BDE-153, BDE-154) in newly hatched chicks did not differ between the west coast of Norway (Runde, 62° N) and Spitsbergen (Kongsfjorden, 79° N) (Murvoll et al. 2006b). The apparent lack of a latitudinal decrease in PBDE levels in kittiwakes may be because they winter in the North Atlantic, close to where these compounds are used and released.

In calanoid species, HBCD was detected only in the Oslofjord (Figure 3A). In Atlantic cod, levels of PBDEs (Figure 2B) and HBCD (Figure 3B) were somewhat higher in the Oslofjord than at Froan, and were lowest in polar cod from Spitsbergen. Levels of PBDEs in the Oslofjord were considerably lower than concentrations reported in cod from 16 different locations in the North Sea and Skagerrak (Boon et al. 2002).

Because food webs are complex, and because few species were studied, we acknowledge that it is difficult to estimate biomagnification rates in the different ecosystems included in this study. However, our crude approach, assuming a simple cod–harbor seal food chain, will still give some information on biomagnification processes of BFR compounds in the three coastal ecosystems.

In the Oslofjord, the biomagnification of BDE-99 from Atlantic cod to harbor seal was particularly high (Table 2), perhaps because BDE-99 constitutes a large part of the technical penta-BDE mixture, and the releases of this compound into the environment probably has been high. The high level of BDE-99 reported in the nearby Drammens fjord (Zegers et al. 2003) supports this. Furthermore, levels of BDE-99 were quite high in calanoids from the Oslofjord (Table 1). Much higher levels of BDE-99 than reported herein have been reported in more pelagic stocks of Atlantic cod in the Skagerrak and the North Sea (Boon et al. 2002). It is also possible that harbor seals in the Oslofjord prefer to prey on cod from the pelagic stocks. The Atlantic cod sampled in this study may have belonged to a more coastal bound stock which the harbor seal does not prefer to prey on, and this may have resulted in an overestimation of the BMF for BDE-99. It should also be noted that BDE-99 is meta-para-substituted and consequently not easily metabolized (Veltman et al. 2005). These factors may help explain the high BMF of BDE-99 from Atlantic cod to harbor seals in the Oslofjord.

The BMF of BDE-153 was also high in harbor seals from the Oslofjord, perhaps because BDE-153 has a substitution pattern similar to that of PCB-153, which is the most persistent PCB compound. It is therefore possible that the high BMF of BDE-153 in the Oslofjord is caused by its persistence.

In most species from all locations, BDE-47 was the most abundant congener (Table 1). This congener was also biomagnified throughout the three food chains (Table 2). BDE-47 constitutes approximately 25% of the technical penta-BDE mixture (Hites 2004) and has thus been released to the environment in relatively large volumes. Furthermore, there are indications that in fish, BDE-99 (which constitutes ~ 50% of the penta-BDE mixture) is debrominated to BDE-47 (Stapleton et al. 2004), and this may thus lead to a further biomagnification of BDE-47 in marine food chains.

Even though BDE-209 often is the predominating PBDE congener in marine sediments (de Boer et al. 2003), it has been reported to contribute very little to the total PBDE burden in organisms (Law et al. 2006a). This is believed to be caused by the large molecular size of the compound and the resultant low transfer over cells and uptake into the organisms (Stapleton et al. 2004). Recently, there has been a growing body of evidence that suggests that BDE-209 is bioaccumulated to a larger extent in terrestrial food chains than in marine food chains (Law et al. 2006a). However, BDE-209 has been reported to account for > 50% of total BDE burden in the detritus feeding ice-amphipod Gamarus wilkitzkii at Spitsbergen (Sørmo et al. 2006). Herein, BDE-209 was detected in animals from all the three ecosystems (Table 1). Because BDE-209 is almost ubiquitous, all possible efforts were made to avoid contamination of the samples during sampling, storage, and analysis. During the analyses, blank samples were run parallel to the samples to control for possible contamination in the laboratory, and no such contamination could be identified.

The highest BDE-209 levels were found in arctic tern eggs from Spitsbergen (Table 1). Further, it should be noted that the highest concentration of BDE-209 relative to Σ;PBDEs was found in polar cod from Spitsbergen (ca. 16% of Σ;PBDEs), harbor seals from Spitsbergen (~ 3%), and arctic terns from Spitsbergen (~ 2%).

BDE-209 has a strong affinity to particles. It is therefore possible that the detected levels in the calanoid species and in the two cod species are associated with the cuticle/skin or sediment particles and/or prey species in the intestines (Law et al. 2006a; Leonards et al. 2004). However, the detection of BDE-209 in tern eggs and seal blubber shows that it is accumulated also in marine food chains. This is consistent with reports that BDE-209 was bioaccumulated in grey seal given a supplement of this congener in their diet (Thomas et al. 2005). BDE-209 has recently also been reported in adipose tissue and plasma from polar bears and glaucous gulls (Larus hyperboreus) from Spitsbergen (Sørmo et al. 2006; Verreault et al. 2005). The relatively high contribution of BDE-209 to Σ;PBDEs in animals from Spitsbergen demonstrates that this congener is subject to long-range transport and dispersal.

Whereas the data herein indicate that BDE-209 may be biomagnified from polar cod to harbor seals (Table 2), this was not the case from Atlantic cod to seals at Froan. Thus, the potential of BDE-209 to be transferred in food webs is unclear. The technical deca-BDE-mixture, in which BDE-209 is the major congener, presently constitutes about 80% of the world market demand of PBDEs (de Boer et al. 2003). Thus, there is a clear need for more information on the ability of BDE-209 to biomagnify and/or be debrominated in marine ecosystems.

At Spitsbergen, levels of both PBDEs and HBCD were higher in ringed seals than in harbor seals (Table 1). The most obvious differences between these two seal species were related to the much higher levels of BDE-47, HBCD, and BDE-100 in ringed seals. These differences are most likely related to differences in species-specific differences in their ability to metabolize and biotransform the BFR compounds, and possibly also related to differences in prey preferences.

There are few reports concerning levels of HBCD in marine ecosystems (Morris et al. 2004; Stapleton et al. 2006; Wolkers et al. 2004; Zegers et al. 2005). Herein, HBCD were found in animals from all trophic levels, except in calanoids at Froan and at Spitsbergen. The commercial HBCD mixtures mainly consist of the three stereoisomers γ-HBCD (75–89%), α-HBCD (10–13%), and β-HBCD (1–12%) (Heeb et al. 2005). In biota, the HBCD isomer composition changes, and α-HBCD dominates (Law et al. 2006a). In the present study, we did not distinguish among the different isomers of HBCD. However, in aquatic invertebrates, marine fish, birds, and marine mammals HBCD is present predominantly as α-HBCD (Covaci et al. 2006).

In cod, seals, and terns, HBCD levels seemed to be similar in the Oslofjord and at Froan, whereas levels were much lower at Spitsbergen (Figure 3B–D), except in ringed seals (Table 1). The particular high levels of HBCD in the ringed seals indicate that the bioaccumulation potential of HBCD in this species may be particularly high (Sørmo et al. 2006). Previously, it has been reported that HBCD does not seem to biomagnify from ringed seals to polar bears (Sørmo et al. 2006) possibly because polar bears generally have a large capacity to metabolize organohalogenated compounds (Letcher et al. 1996).

In common dolphins (Delphinus delphis) from the Central and South Atlantic coast of Europe (Scotland, Ireland, the Netherlands, Spain), median concentrations of HBCD ranged from 200 to 900 ng/g lw, whereas median concentrations in harbor porpoises ranged from 100 to 5,100 ng/g lw (Zegers et al. 2005). Levels were highest in the Irish Sea and in North-East Scotland. In blubber of two harbor seals from the western Wadden Sea, concentrations of HBCD ranged from 63 to 2,055 ng/g lw (Morris et al. 2004). In stranded and by-caught harbor porpoises in the United Kingdom, HBCD levels ranged from 11 to 21,300 ng/g lw (Law et al. 2006b), and a time-trend analysis of the data strongly indicated a sharp increase in HBCD concentrations from about 2001 onward. The HBCD levels reported in cetaceans from the South- and Central-East Atlantic coast, and in the harbor seals from the Wadden Sea are much higher than those found in harbor seals from the Oslofjord, Froan, and Spitsbergen (Table 1).

Relatively high levels of HBCD have also been reported in hatchlings of kittiwakes from the Norwegian west coast (~ 260 ng/g lw; Runde, 62° N) and levels were somewhat lower in hatchlings from Spitsbergen (~ 120 ng/g lw; Kongsfjorden 79° N) (Murvoll et al. 2006b). Furthermore, even higher levels of HBCD were reported in hatchlings of European shags (Phalacrocorax aristotelis) from the western Norwegian coast (~ 420 ng/g lw; Sklinna 65° N) (Murvoll et al. 2006a). The much higher levels in the European shag and kittiwake hatchlings may be related to differences in the analytical matrix (whole egg herein vs. yolk sac in hatchlings). However, the differences may also be related to the fact that kittiwakes and European shags winter in the North Sea, the Norwegian Sea, and along the Canadian east coast, whereas common and arctic terns migrate to the more pristine areas in Africa and Antarctica, respectively. In North Sea estuaries (United Kingdom and the Netherlands), levels of HBCD in cormorant livers (Phalacrocorax carbo) and common tern eggs were 330–7,100 and 138–1,320 ng/g lw, respectively (Morris et al. 2004). These concentrations are higher than those reported in the tern eggs herein.

Because HBCD has been reported to have histopathologic and neurotoxic effects (Birnbaum and Staskal 2004; Darnerud 2003; Mariussen and Fonnum 2003), there is cause for concern about the spreading and uptake of this compound in biota. In Californian sea lions (Zalophus californianus) a significant temporal increase in HBCD was reported from 1994 to 2004 (Stapleton et al. 2006), and in harbor porpoises from the United Kingdom a sharp increase in HBCD concentrations was found from about 2001 onward (Law et al. 2006b). Because there currently are no restrictions on the use of HBCD (Stapleton et al. 2006), there are reasons to believe that the global spreading of the compound will continue and that levels in Arctic biota will increase with time.

Conclusion

As mentioned previously, this is the first report on the occurrence of PBDEs and HBCD in freshwater fish in Czech rivers. The results of the present study are summarized as follows:

• Fish is a suitable species for use as a bioindicator for monitoring BFRs in aquatic ecosystem; the greatest accumulation was measured in fatty benthic species represented by barbel and bream. Conversely, the potential of perch (predator fish) for bioaccumulation of these chemicals was lower.

• Contamination patterns and their extent in fish collected in the Elbe and Vltava rivers are comparable with those reported in other European studies conducted in rivers in industrial areas. Technical mixtures based on penta- congeners were probably the source of pollution. When the entire data set generated in our present study was compared with data sets in similar studies conducted abroad, no extremely contaminated locality was found in Czech rivers that we monitored; the extent of pollution was similar to that in other industrial regions, for example, in Canada, Sweden, and Spain.

• The levels of PBDEs were about 10–30 times lower than PCB levels determined in the same fish samples. In barbel from Hrensko (Elbe River), the level of PBDEs was 60 times lower compared with that of PCBs. The concentrations of HBCD in fish were of the same order of magnitude as those of the most abundant PBDE-47.
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References

Alaee M, Luross J, Sergeant DB, Muir DCG, Whittle DM, Solomon K. 1999. Distribution of polybrominated diphenyl ethers in the Canadian environment. Organohalogen Compounds 40:347–350.

Allchin CR, Law RJ, Morris S. 1999. Polybrominated diphenylethers in sediments and biota downstream of potential sources in the UK. Environ Pollut 105: 197–207.

Anderson T MacRae JD. 2006. Polybrominated diphenyl ethers in fish and wastewater samples from an area of the Penobscot River in Central Maine. Chemosphere 62: 1153–160.

Andersson Ö, Blomkvist G. 1981. Polybrominated aromatic pollutants found in fish in Sweden. Chemosphere 10:1051–1060.

Asplund L, Hornung M, Peterson RE, Turesson K, Bergman A. 1999. Levels of polybrominated diphenyl ethers (PBDEs) in fish from the Great Lakes and Baltic Sea. Organohalogen Compounds 40:351–354.

Covaci A, Bervoets L, Hoff P, Voorspoel S, Voets J, Van Campenhout K, et al. 2005. Polybrominated diphenyl ethers (PBDEs) in freshwater mussels and fish from Flanders, Belgium. J Environ Monit 7:132–136.

Covaci A, Gheorghe A, Hulea O, Schepens P. 2006. Levels and distribution of organochlorine pesticides, polychlorinated biphenyls and polybrominated diphenyl ethers in sediments and biota from the Danube Delta, Romania. Environ Pollut 140:136–149.

de Boer J, Brinkman UAT. 1994. The use of fish as biomonitor for the determination of contamination of the aquatic environment by persistent organochlorine compounds. Trac Trend Anal Chem 13:397–404.

de Boer J, de Boer K, Boom JP. 2000a. Polybrominated biphenyls and diphenyl ethers. In: The Handbook of Environmental Chemistry. Vol 3. Part K: New Types of Persistent Halogenated Compounds (Paassivirta J, ed). Berlin: Springer, 62–95.

de Boer J, van der Horst A, Wester PG. 2000b. PBDEs and PBBs in suspended particulate matter, sediments, sewage treatment plant in- and effluents and biota from the Netherlands. Organohalogen Compounds 47:85–88.

de Boer J, Wester PG, van der Horst A, Leonards PE. 2003. Polybrominated diphenyl ethers in influents, suspended particulate matter, sediments, sewage treatment plant and effluents and biota from the Netherlands. Environ Pollut 122:63–74.

de Wit CA. 2002. An overview of brominated flame retardants in the environment. Chemosphere 46: 583–624.

Eljarrat E, de la Cal A, Raldua D, Duran C, Barcelo D. 2004. Occurrence and bioavaiability of polybrominated diphenyl ethers and hexabromocyclododecane in sediment and fish from the Cinca river, a tributary of the Ebro river (Spain). Environ Sci Technol 38:2603–2608.

Eljarrat E, de la Cal A, Raldua D, Duran C, Barcelo D. 2005. Brominated flame retardants in Alburnus alburnus from Cinca River Basin (Spain). Environ Pollut 133:501–508.

ELbe InformationsSystEm. 2006. Home Page. Available: http://elise.bafg.de/servlet/is/7211/ [accessed 15 January 2006]

Eriksson J, Green N, Marsh G, Bergman A. 2004. Photochemical decomposition of 15 polybrominated diphenyl ether congeners in methanol/water. Environ Sci Technol 38: 3119–3125.

Geyer HJ, Rimkus GG, Scheunert I, Kaune A, Kettrup A, Zeeman M, et al. 1999. Bioaccumulation and occurrence of endrocrine-disrupting chemicals (ECDs), persistent organic pollutants (POPs), and other organic compounds in fish and other organism including humans. In: The Handbook of Environmental Chemistry, Vol 2 (Beek B, ed). Berlin: Springer, 1–166.

Haglund PL, Zook DR, Buser HR, Hu J. 1997. Identification and quantification of polybrominated diphenyl ethers and methoxy-polybrominated diphenyl ethers in Baltic biota. Environ Sci Technol 31: 3281–3287.

Hale RC, Alaee M, Manchester-Neesvig JB, Stapleton HM, Ikonomou MG. 2003. Polybrominated diphenyl ether flame retardants in the North American environment. Environ Int 29:771–779.

Kierkegaard A, Bignert A, Sellström U, Olsson M, Asplund L, Jansson B, et al. 2004. Polybrominated diphenyl ethers (PBDEs) and their methoxylated derivates in pike from Swedish waters with emphasis on temporal trends, 1967–2000. Environ Pollut 130:187–198.

Lacorte S, Raldúa D, Martínez E, Navarro A, Diez S, Bayona JM, et al. 2006. Pilot survey of a broad range of priority pollutants in sediment and fish from the Ebro river basin (NE Spain). Environ Pollut 140:471–482.

Luross JM, Alaee M, Sergeant DB, Cannon CM, Whittle DM, Solomon KR, et al. 2002. Spatial distribution of polybrominated diphenyl ethers and polybrominated biphenyls in lake trout from the Laurentian Great Lakes. Chemosphere 46: 665–672.

Morris S, Allchin CR, Zegers BN, Haftka JJH, Boon JP, Belpaire C, et al. 2004. Distribution and fate of HBCD and TBBPA brominated flame retardants in North Sea estuaries and aquatic food web. Environ Sci Technol 38: 5497–5504.

Ohta S, Ishizuka D, Nishimura H, Nakao T, Aozasa O, Shimidzu Y, et al. 2002. Comparison of polybrominated diphenyl ethers in fish, vegetables and meats and levels in human milk of nursing woman in Japan. Chemosphere 46: 689–696.

Petterson A, Karlsson H. 2001. Analysis and Toxicology of Brominated Flame Retardants with Emphasis on PBDEs PhD Dissertation]. Sweden:Örebro University.

Rahman F, Langford KH, Scrimshaw MD, Lester JN. 2001. Polybrominated diphenyl ether (PBDE) flame retardants. Sci Total Environ 275:1–17.

Sellström U, Jansson B, Kierkegaard A, de Witt C, Odsjö T, Olsson M. 1993. Polybrominated diphenyl ethers (PBDE) in biological samples from the Swedish environment. Chemosphere 26:1703–1718.

Sellström U, Kierkegaard A, de Wit C, Jansson B. 1998. Polybrominated diphenyl ethers and hexabromocyclododecane in sediment and fish from a Swedish river. Environ Toxicol Chem 17:1065–1072.

Söderström G, Sellström U, de Wit CA, Tysklind M. 2004. Photolytic debromination of decabromodiphenyl ether (BDE 209). Environ Sci Technol 38: 127–132.

van Leeuwen SPJ, Van Cleuvenbergen R, Abalos M, Pasini A-L, Eriksson U, Cleemann M, et al. 2006. New certified and candidate certified reference materials for the analysis of PCBs, PCDD/Fs, OCPs and BFRs in the environment and food. Trac Trend Anal Chem 25:397–409.

Vives I, Grimalt JO, Lacorte S, Guillamón M, Barceló D. 2004. Polybrominated diphenyl ether flame retardants in fish from lakes in European high mountains and Greenland. Environ Sci Technol 38: 2338–2344.

Watanabe I, Kashimoto T, Tatsukawa R. 1987. Polybrominated diphenyl ethers in marine fish, shellfish and river and marine sediments in Japan. Chemosphere 16: 2389–2396.

WHO. 1994. Brominated Diphenyl Ethers. Environmental Health Criteria 162. Geneva:World Health Organization.

WHO. 1997. Environmental Health Criteria 192: Flame Retardants–General Introduction. Geneva:World Health Organization.

Zweidinger RA, Cooper SD, Erickson MD, Michael LC, Pellizzari ED. 1979. Sampling and analysis for semivolatile brominated organics in ambient air. ACS Symp Ser 94:217–231.
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