Abstract
Spices have been used since ancient times. Although they have been employed mainly as flavoring and coloring agents, their role in food safety is of increasing concern. In this study, the usefulness of a modified QuEChERS method, based on the d-SPE, with micro-HPLC–MS/MS system for the determination of selected perfluoroalkyl carboxylic acids (PFCAs) and perfluoroalkane sulfonates (PFSAs) in spices was addressed. The commonly used spices in Spain and Slovakia were investigated. The studies showed the presence of perfluorooctanoic acid in 19 spices of Spanish and Slovak origin, and it ranged from 0.11 ng g−1 for garlic to 0.67 ng g−1 for peppermint. The perfluorobutanoic acid was quantified in 10 Slovak spices (from 1.13 ng g−1 for allspice to 37.82 ng g−1 for star anise), whereas perfluorobutane sulfonate was identified only in 12 Spanish spices and it ranged from 0.24 ng g−1 for cinnamon to 1.01 ng g−1 for coriander. In contrast, perfluoroheptanoic acid was identified only in Slovak cardamom (1.94 ng g−1) and coriander (0.74 ng g−1). The average consumption of spices in Europe is approximately 0.5 g day−1, while in Asia and northern Africa, it is many times higher. Average content of PFASs in this evaluation has a value 4.67 ng g−1 giving 2.33 ng day−1 per person. This study showed that daily used spices may contribute to the overall contamination of food by perfluoroalkyl substances.
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Introduction
Spices are mostly plant origin substances added to food in order to improve their flavor, aroma and functionality. They are used also as food preservatives and folk medicines. Many spices also have been recognized as having inflammatory [1], antimicrobial [2], antifungal [3], antimutagenic and anticarcinogenic properties [4]. A growing body of epidemiological and preclinical evidence points to culinary herbs and spices as minor dietary constituents with multiple anticancer characteristics [4, 5]. They can be classified according to several criteria, such as: due to the origin, active substance content, whether due to parts of plants, from which it is derived. They can be prepared from fruits (pimento), fully ripe berries (white pepper), flower buds (clove), roots (ginger) or bark (cinnamon) [6] and can be added to food in form of whole or ground material or as extracts. Although spices contribute little to weight on our dish, they can be important contributors to our daily antioxidants [7] intake, especially in dietary cultures where spices are used regularly [8]. Due to the origin, cultivation conditions and type of processing, spices may also be a source of some contaminants such as pesticides [9, 10], heavy metals [11], illegal dyes [12, 13], mycotoxins [14, 15] and perfluoroalkyl substances.
Perfluoroalkyl substances (PFASs) are a wide group of synthetic compounds with high resistance to chemical, thermal, or biological degradation. PFASs comprise a diverse class of chemicals consisting of an alkyl chain which is partially of fully fluorinated and have different functional groups attached. Among them are perfluoroalkyl carboxylic acids (PFCAs) and perfluoroalkane sulfonates (PFSAs), which are the subject of our interest. They are widely used in various industrial and consumer applications, mainly thanks to their unique ability to repel both water and oil. As a consequence, these compounds show a global distribution all over the world and have been detected not only in environment samples [16, 17] but also in human blood [18, 19]. It show persistence in the environment [20] and some of them are related to different carcinogenic actions [21]. For example, perfluorooctanoic acid (PFOA) has been identified as a potent hepatocarcinogen in rodents [21, 22].
Nevertheless, as spices are consumed all the time in daily meal even though in tiny amount, long-term exposure to persistent organic pollutants may pose a health risk. However, no information is available on the presence of PFASs in spices up till now. Therefore, it is of importance to monitor them for the most often occurring PFASs identification and illustrate the food contamination level. What is more important, there is currently no legislation for perfluoroalkyl substances in food or feed within the EU. The EFSA Scientific Panel on Food Additives, Flavourings, Processing Aids and Materials in Contact with Food (AFC) issued an opinion on the safety of ammonium salt of PFOA as a food contact material, but this has not so far led to regulatory measures. Currently, there is a proposal for hazard classification for PFOS (perfluorooctane sulfonate) in the European Inventory of Existing Commercial Chemical Substances (EINECS). The Conference of the Parties of the Stockholm Convention on Persistent Organic Pollutants (POPs) at its fourth meeting held in May 2009, listed nine additional chemicals as new POPs. PFOS and their salts, as well as perfluorooctane sulfonyl fluoride are among these new POPs [23]. Moreover, in 2006, EPA (Environmental Protection Agency) invited the eight major fluoropolymer and telomere manufacturers to join in a global stewardship program with which was at first aimed to commit to achieve, no later than 2010, a 95 % reduction, measured from a year 2000 baseline, in both facility emissions to all media of PFOA, precursor chemicals that can break down to PFOA, and related higher homologue chemicals, and product content levels of these chemicals and secondly to commit to working toward the elimination of these chemicals from emissions and products by 2015. In January 2015, EPA released the most recent reports, for years 2013 and 2014, from participating companies on progress they have made in reaching the program’s phase-out goals. Results show that the companies are on track to reach the program’s goal of phasing out these chemicals by the end of 2015 [24].
Spices as foods must comply with the requirements of food law. There are Regulation (EC) No 178/2002 of The European Parliament and of the Council of 28 January 2002 laying down the general principles and requirements of food law, establishing the European Food Safety Authority and laying down procedures in matters of food safety and the Act of 25 August 2006 on food and nutrition safety. There is no legislation for perfluoroalkyl substances in food or feed within the EU [25]. The preliminary findings of EFSA indicate the need to identify PFASs in raw material as well as in food of plant origin [26]. Now there is increasing number of evidences that the pollution by PFASs, is a global issue, given the transboundary movement of these compounds [27]. EFSA’s Scientific Panel on Contaminants in the Food Chain therefore recommended that further data on perfluoroalkylated substance levels in food and humans would be desirable [25]. In March 2010, Commission Recommendation 2010/161/EU invited the Member States to monitor the presence of PFOS and PFOA in food systems, compounds similar to them but with different chain length and their precursors [28]. For this purpose, according to above-mentioned document, it is required to use a method of analysis that has been proven to generate reliable results. Ideally, the recovery rates should be in the range 70–120 %, with limits of quantification (LOQ) of 1 µg kg−1. Therefore, a sensitive method of perfluoroalkyl carboxylic acids and perfluoroalkane sulfonates determination in spices samples is extremely needed. Currently, due to its high sensitivity and selectivity, liquid chromatography hyphenated with tandem mass spectrometry (LC–MS/MS) operated in the multiple reaction monitoring mode (MRM) is the preferred technique for a quantitation of PFCAs and PFSAs trace levels. Moreover, micro-HPLC technique provides higher peak capacity, greater resolution, increased sensitivity and a higher speed of analysis compared to conventional LC system [29], mainly in combination with MS/MS.
The sample preparation method for PFASs determination is a challenge not only because of their low concentration levels in food samples but also of the complexity of matrices. Therefore, efficient sample preparation procedures and very sensitive determination technique are required. One of the three most common approaches such as pressurized liquid extraction [21], alkaline digestion [30–32] and ion pair extraction [20] was employed for sample preparation for PFASs analysis; however, each method showed some limitations. Procedures based on ion pair extraction have been widely used for this purpose, although sometimes these suffer from matrix effects. Tetra-n-butylammonium hydrogen sulfate solution and sodium carbonate buffer at pH 10 are used as the ion-pairing agents and methyl tert-butyl ether (MTBE) as the extractant [33, 34]. This method is relatively laborious and suffers from drawbacks such as co-extraction lipids and other lipophilic matrix components, which significantly complicate further chromatographic analysis. Several studies have been performed using KOH digestion or filtration followed by solid phase extraction (SPE) [35, 36]. SPE is a less laborious and faster alternative. Because of the different polarities of PFASs, different SPE cartridges have been evaluated. The widely used Oasis WAX cartridges yield good recoveries for short-chain (C4–C6) PFASs, whereas less polar phases (C18 and Oasis HLB) may be used for longer-chain PFASs. Unfortunately, none of the cartridges available at the market allows simultaneous retaining of all commonly monitored representatives of perfluorinated compounds [37]. Therefore, there is a need to develop an innovative approach that would allow for the accurate determination of an entire set of analytes of concern at an ultra-trace level and also high-throughput sample handling. Nowadays, there is a strong tendency to develop simply, minimum steps, and effective for cleaning up complex samples and useful in the analysis of residues in foods methods. Such features a fast and inexpensive extraction QuEChERS (Quick, Easy, Cheap, Effective, Rugged, Safe), method has been shown. It was introduced for a first time by Anastassiades [38]. Extraction based on partitioning via salting out extraction involving the equilibrium between an aqueous and an organic layer is the first step. Dispersive solid phase extraction (d-SPE) that involves further cleanup using combinations of anhydrous salt and various sorbents to remove interfering substances is the second step. The available evidence indicates for the benefits of use polymer-based ENV SPE Bulk Sorbent for the determination of perfluoroalkyl carboxylic acids (PFCAs) and perfluoroalkane sulfonates (PFSAs). This sample treatment has been previously reported for sample preparation for perfluoroalkyl substances determination in different food matrix [39] and animal tissues [40]. Previously, this method was also used for analysis of pesticides residues in vegetables [41], but it has been extended to other residues and matrixes [42–44].
To our best knowledge, the existing literature provides lack of information about the PFASs determination in spices, and thus no one used the QuEChERS methodology for this reason. Consequently, the aim of this study was to apply the modified QuEChERS method, based on the dispersive solid phase extraction (d-SPE), with micro-HPLC–MS/MS system [40] for the determination of selected perfluoroalkyl carboxylic acids (PFCAs) and perfluoroalkane sulfonates (PFSAs) in spices. This study tries to evaluate for the first time an extent of spices contamination by perfluoroalkyl substances which may be important for further EFSA recommendation on the health risk of these compounds in humans.
Experimental
Chemicals and reagents
Magnesium sulfate anhydrous p.a. and sodium chloride p.a. were purchased from POCh SA, Poland. ENV (styrene–divinylbenzene) SPE Bulk Sorbent derived from Agilent Technologies, USA. Reagents in MS grade including acetonitrile (MeCN), methanol (MeOH), formic acid (FA) were purchased from Sigma Chemical Co., St. Louis, MO. Water was purified with a Mili-Q system, Millipore, Bedford, USA. Acetonitrile (for extraction) HPLC grade was purchased from Merck KGaA, Germany. Native PFASs Solution/Mixture contains sulfonates: perfluorobutane (PFBS), perfluorohexane (PFHS), perfluorooctane (PFOS), and acids: perfluorobutanoic (PFBA), perfluoropentanoic (PFPeA), perfluorohexanoic (PFHxA), perfluoroheptanoic (PFHpA), perfluorooctanoic (PFOA), perfluorononanoic (PFNA), perfluorodecanoic (PFDA) and 1,2,3,4-13C- labeled PFOA were obtained from Wellington Laboratories, Canada. Stock, intermediate and working standard solutions of native PFASs and 1,2,3,4-13C4-labeled PFOA (IS–internal standard) was prepared in acetonitrile. Stock solution of PFASs at the concentration of 5 µg mL−1 and 1,2,3,4-13C4-labeled PFOA at a concentration of 49 µg mL−1 were purchased as a solution prepared in methanol. Intermediate (100 ng mL−1) and working (1 ng mL−1) standard solutions of native PFASs and IS were prepared in 20 % MeOH (v/v) with 1 % (v/v) of formic acid.
Matrix-matched calibration standards at concentrations of between 1 and 20 ng mL−1 were prepared by diluting the standard mixture solution to the corresponding blank sample extracts. The intention was to compare the matrix effects in calibration. A series of standard solutions in pure solvent were prepared by dilution of the standard mixture solution in 20 % MeOH (v/v) with 1 % (v/v) of formic acid at the same range as before and then were used for calibration curves construction. In both cases, 20 µL of the 1,2,3,4-13C4-labeled PFOA solution (concentration) was added to each standard solution. A series of standard solutions were prepared in triplicate.
Material
The analyzed spice samples, as a powder, in the amount about 100 g each, originated from two EU countries (Slovakia and Spain). Twelve types of spices collected for the study were as follows: anise (Pimpinella anisum), star anise (Illicum verum), white pepper (Piper nigrum), fennel (Foeniculum vulgare), cardamom (Elettaria cardamomum), clove (Syzygium aromaticum), coriander (Coriandrum sativum), nutmeg (Myristica fragrans), allspice (Pimenta dioica), cinnamon (Cinnamomum burmanni), vanilla (Vanilla planifolia), ginger (Zingiber officinale). Additionally, peppermint (Mentha piperita), parsley (Petroselinum crispum), thyme (Thymus vulgaris), laurel (Laurus nobilis), two oreganos (Origanum vulgare), garlic (Allium sativum), cumin (Cuminum cyminum), black paper (Piper nigrum), and two varieties of hot pepper (Capsicum annuum) (mild and hot) from Spain were analyzed.
Equipment
The micro-HPLC system (LC200, Eksigent, Canada) consisted of a multi-channel pump, an autosampler (set at 4 °C), a column oven and a system controller coupled with a mass spectrometer (QTRAP 5500, AB SCIEX, Canada) consisting of a triple quadrupole, ion trap and ion source of electro-spray ionization (ESI) and controlled by the Analyst 1.5.1 software was used to perform the LC–MS/MS analyses. All chromatographic determinations were performed on HALO C18 (50 mm × 0.5 mm × 2.7 µm) column (Eksigent, Canada) at 45 °C with the flow rate of 20 μL min−1. Compounds were eluted in gradient system composed of water/formic acid (99.0/1.0, phase A) and acetonitrile/formic acid (99.0/1.0, phase B). Gradient was as follows: 40 % B (0–0.5 min), 40–90 % B (0.5–3.0 min), 90 % B (3.0–4.0 min), 90–40 % (4.0–4.2 min) and 40 % (4.2–5.0 min). Qualitative and quantitative analysis was made using Multiple Reaction Monitoring (MRM) method. Optimal identification of compounds analyzed was achieved under the following conditions: negative ionization, curtain gas: 25 L min−1, collision gas: 9 L min−1, ion spray voltage: −4500 V, temperature: 350 °C, 1 ion source gas: 30 L/min, 2 ion source gas: 35 L/min, declustering potential: −30: −85 V, entrance potential: −10 V, collision energy: −10 to −65 eV, collision cell exit potential: −10:−38 V (Surma, Wiczkowski, Cieślik & Zieliński, 2015).
MPW 351R Centrifuge (MPW Med. Instruments, Warsaw, Poland) was used for sample preparation. The vacuum Concentrator plus (Eppendorf AG, Hamburg, Germany) was used for the extracts concentration.
Sample preparation method for PFCAs and PFSAs determination
The spices sample preparation for perfluoroalkyl carboxylic acids and perfluoroalkane sulfonates determination, based on dispersive solid phase extraction (d-SPE) followed by micro-HPLC–MS/MS, was conducted according to the methodology evaluated and validated in the previous study [39]. However, considering the fact that the majority of investigated spices has a very intense color, application of additional sorbent for sample clean-up was considered. Based on previous experiments with containing pigments samples preparation, GCB (graphitized carbon black) was selected from available silica-based sorbents (silica gel, florisil, SAX and NH2). Two variants of method were tested with or without GCB and they were marked as follow: 1 (ENV) and 2 (ENV + GCB). The extraction process was conducted as follow: 2 grams of a representative portion of spice were weighted into a 50-mL centrifuge tube and spiked with 20 µl of IS (internal standard) solution (2.5 µg mL−1). Then, 5 mL of water and 10 mL of MeCN with 150 µL of FA were added to each tube and the mixture was sonicated and vigorously shaken for 1 min, respectively. After that 1 g NaCl and 4 g MgSO4 were added, the tube was shaken immediately after addition of the salt. Then each sample was shaken vigorously for 1 min and centrifuged for 15 min at 8700 RCF. Next, 6 mL of the supernatant was transferred into a PP 15-mL tube containing 0,15 g ENV SPE Bulk Sorbent (method 1) and additionally, apart from ENV, GCB (method 2), to d-SPE used for extracts clean-up, and 0.900 g MgSO4. After 30 s shaking and 5 min centrifugation at 5000 RCF, 4 mL amount from each extracts was transferred into a 4-ml tubes and evaporated to dryness in the concentrator at 40 °C. The residues were dissolved in 1 mL of methanol. Just before injection, the samples were diluted fivefold in acidified dH2O (distillate water with 1 % (v/v) of formic acid addition). Finally, all cleaned up samples were analyzed by micro-HPL–MS/MS. Blank samples and reagent blanks were prepared according the same procedure. Each sample was prepared in triplicate. The most appropriate variant of the QuEChERS method was applied for perfluoroalkyl substances determination in spice samples. To better illustrate, the final sample preparation method is shown in Fig. 1.
As of now, spices and related food matrices with certified concentrations of perfluoroalkyl substances are not commonly available. Thus, the usefulness of the method was verified on the basis of the recovery ratio of analyzed compounds (analysis of fortified samples) which were previously used for recovery studies. Recovery studies involved homogenized samples of cinnamon being spiked with the standard solution of ten PFASs (7 perfluoroalkyl carboxylic acids and 3 perfluoroalkane sulfonates) to the fortification level of 0.005 mg kg−1. The procedure of sample preparation was the same as described above, except that the sample was fortified by native standard solution of PFASs at the beginning, mixed and left to stand for 15 min at room temperature prior to extraction.
The PFCAs and PFSAs involved in this study were identified by the retention time and MRM ion pairs. Calibration curves were constructed by plotting the ratio of the peak areas, divided by the peak area of the 1,2,3,4-13C4- labeled PFOA, against concentration of the analyte. Peak areas of the analytes from blank matrix (when was present) have been removed from analytes peaks area from fortified samples. Retention times and MRM ion pairs for analyzed PFASs are summarized in Table 1.
The analytical performance of the using QuEChERS method based on dispersive solid phase extraction for studied perfluoroalkyl substances was examined by looking at its linearity, selectivity, recovery, repeatability, the limit of detection (LOD), and limit of quantification (LOQ).
Results and discussion
Comparison of QuEChERS method with and without additional sorbent–recovery study
The recovery values for all tested analytes for fortified samples of cinnamon are presented in Fig. 2. They ranged from 87 to 105 % for method 1 (based on ENV sorbent) and from 67 to 94 % for method 2 (which in addition to ENV sorbent uses GCB). The better recovery ratios (according to the Commission Recommendation 2010/161/EU of 70–120 %) with RSD lower than 10 % for all analyzed perfluoroalkyl substances were obtained for the method 1 used ENV sorbent for extract clean-up. Method 2 uses the addition of GCB apart from ENV resulted in more diversified values, not be in the range of values set by Commission Recommendation 2010/161/EU (70–120 %). The use of additional sorbent–GCB in the sample preparation step caused decrease of the recovery values for all tested analytes. Moreover, the RSD (related standard deviation) value higher than 10 % was noted for one PFAS–perfluorononanoic acid (PFNA) with value 11, 2 %. At present, there is a lack of information about the allowed RSD value for recovery ratios for perfluoroalkyl substances determination in Commission Recommendation 2010/161/EU. However, a good laboratory practice and validation guidelines indicate the value of 10 %.
Analytical performance of the method
A method of least squares was used to obtain equations of calibration curves (y = ax + b). A goodness of fit being given by coefficient of determination (R 2), which is an evidence that linearity was observed for analyzed PFASs in the range of concentrations from 1 to 20 ng mL−1 (Table 2). Correlation coefficients were statistically significant and slope at a significance level (α) equal to 0.05. For the same hypothesis, the intercept from the regression models was not significantly different to zero. This means that absence of compound in any analyzed sample would imply that the analytical signal should be zero.
Recovery studies were conducted after cinnamon sample fortification of selected PFASs to the level of 0.005 mg kg−1 (Fig. 2). The received recovery values from 87 ± 2.8 % for PFBA to 105 ± 8.5 % for PFNA being in good agreement with the Commission Recommendation 2010/161/EU on the monitoring of perfluoroalkylated substances in food [28].
The repeatability, expressed as the relative standard deviation (RSD) of the analyzed samples, was lower than 10 % for all target analytes. There is a lack of information about the allowed RSD value for recovery ratios for PFASs determination in Commission Recommendation 2010/161/EU. However, good laboratory practice and validation guidelines indicate the value of 10 %. The limit of detection (LOD) was calculated as three times higher than the level of noise, and the limit of quantification (LOQ) was equal to ten times of the noise level. The level of noise was measured from the chromatograms obtained for the standard solutions with the lowest concentration, i.e. 1 ng mL−1. The LOD and LOQ for the used method calculated as a ratio signal to noise showed values from 0.013 to 0.039 µg kg−1 for PFHS to 0.073–0.219 µg kg−1 for PFBA, respectively (Table 2). LOQ values were in good agreement with value specified in the Commission Recommendation 2010/161/EU (1 µg kg−1) [28]. The sensitivity calculated as calibration slope coefficient was the highest for perfluorooctanoic acid while the lowest for perfluorononanoic acid.
Matrix effects (ME) (suppression or enhancement) were evaluated through the matrix effect percentage (% ME) calculation. The percentage was calculated as a difference between the slopes of the matrix match calibration curve and the solvent one according to literature report [45]. Signal enhancement would occur if the percentage of the difference between these slopes were positive. If it was negative, it would be indicative of signal suppression. Depending on the % ME value would be classified into three categories. A percentage between −20 and 20 % was considered as no matrix effect, because this variation would be close to the repeatability values. A medium matrix effect occurred when the values were between −50 and −20 % or 20 and 50 %, and a strong matrix effect would be below −50 % or above +50 %. In the studied matrix (cinnamon), no matrix effects were observed. For each analyzed PFASs %, ME ranged from −7.2 to 8.5 %. Therefore, in later determination, solvent calibration curves were used to PFCAs and PFSAs content calculation in analyzed spice samples.
Analysis of spice samples
In present study, we decided to fill out existing gap in the spices contamination with perfluoroalkyl substances. The results of spice samples analysis are presented in Table 3. In a group of selected perfluoroalkyl substances (7 perfluoroalkyl carboxylic acids and 3 perfluoroalkane sulfonates), three acids such as butanoic (PFBA), heptanoic (PFHpA) and octanoic (PFOA) and one sulfonate–perfluorobutane (PFBS) were quantified. Perfluorobutanoic acid was detected in 10 Slovak spice samples and ranged from 1.13 ng g−1 for allspice to 37.82 ng g−1for star anise. Spanish spices was free from PFBA contamination. The perfluorobutanoic acid concentration in Slovak spices increased in the following order: allspice < nutmeg < white pepper < ginger < vanilla < coriander < fennel < clove < anise < star anise. Perfluoroheptanoic acid (PFHpA) was identified only in two samples of Slovak spices: cardamom (1.94 ng g−1) and coriander (0.74 ng g−1). Perfluorooctanoic acid was quantified in the largest number of spice samples (19) but at not too high levels. There is ranged from 0.11 ng g−1 for garlic to 0.67 ng g−1 for peppermint. In both cases, it was spices from Spain. Generally, only four Slovak spices (anise, coriander, allspices and cinnamon) were contaminated by PFOA, while in Spanish spices PFOA was identified in 15 samples (additionally in star anise, nutmeg, peppermint, parsley, thyme, garlic, hot paper (mild and hot) and oregano). For both countries of origin, no increasing PFOA concentration trend has been noticed in investigated samples. In all cases, besides cinnamon, when analyzed samples were from two countries of origin globally, higher concentration of perfluoroalkyl carboxylic acids in Slovak spices was noticed. The highest amount of PFCAs was determined in Slovak star anise.
Reverse situation have placed in case of perfluoroalkane sulfonates. Perfluorobutane sulfonate is only one qualified in 12 Spanish spices and ranged from 0.24 ng g−1 for cinnamon to 1.01 ng g−1 for coriander. No PFASs were detected in Slovak spice samples. An example of LC–MS/MS chromatogram of spice sample is shown in Fig. 3.
There were some inconveniences with data received in this study comparing with another author data because, to our knowledge, no other studies regarding PFASs concentration in spice samples have been reported in the available literature. Looking at the existing literature, even EFSA [46] provides no information about the content of perfluoroalkyl substances in spices and the results presented in this paper are of great value. Following the above-mentioned document, authors’ foods of plant origin (n = 508) have been analyzed for a broad range of PFASs, but only a very limited number of positive results were found in the food of plant origin divided into grain and grain-based products, vegetables and vegetable products, potatoes and potatoes products, and legumes, nuts and oil seeds groups. Contamination levels ranged between 0.01 and 2 ng g−1 for the various PFASs detected. Spices were included in this division for a food groups to “Other foods” section with fruit juice, soft drinks, herbs, dressing, snacks and desserts. It is a much diversified group of food products, on the basis of which, it cannot be concluded about the spices contamination by perfluoroalkyl substances. Other scientific reports of EFSA [47] indicated that upper bond mean, calculated by weighting the results for the number of pooled samples for PFDA concentration, was 0.0095 µg kg−1. Only two undefined spice samples were analyzed from 30 samples taken considering the pooled samples. Proportion of left-censored results calculated on the number of reported analyses (LB%) was 100 %. To our best knowledge, no other information about perfluoroalkyl substances contamination level of spices is available.
A person can be exposed to these compounds through the consumption of food and drinking water, as a result of their migration to food from packaging as well as through the lungs and skin by daily contact with the products that surround us [48]. This is followed by the ingestion of dust and inhalation of air [49]. However, bioaccumulation in food products is the most significant source of human exposure to PFASs [50]. There are no systematic investigations of the occurrence of perfluoroalkyl substances in European food available that could form a basis for a comprehensive dietary exposure assessment. Due to the lack of data, it has not been possible to perform an assessment of the relative contribution from different foodstuffs to human exposure to PFASs. Based on the limited information available, seafood, in particular, is considered a major source of PFASs in humans [32], but contaminated drinking water can also be an important source of exposure in contaminated areas [49]. The average consumption of spices in Europe is approximately 0.5 g day−1, while in Asia and northern Africa, it is many times higher [51]. Average content of PFASs in this evaluation has a value 4.67 ng g−1 giving 2.33 ng day−1 per person. As was mentioned before, there is no legislation for perfluoroalkyl substances in food or feed within the EU so it is impossible to compare these values with some limitation. In recent decades, there is a growing interest in vegetarian diets and the favorable impact of reducing the consumption of animal products on the health of the people. In the diet, where traditionally rarely or never used the meat are used in large quantities numerous spices [52]. The recipes of some dishes in Indian cuisine include up to 60 different spices. However, level of spices contamination is quite low and PFASs are well absorbed from the intestines and accumulated primarily in the liver [50]. Man particularly finds it difficult to expel the substance from the body. For example, the half-life of PFOA in the adult rat serum is 7.5 days, while the human is approx. 9 years. Therefore, although there is no clear threat contamination of PFASs, there is a need to be caution and monitor their level in food.
Conclusion
This study provided for the first time evidences for spices contamination by PFASs from the two European countries diametrically located. The dispersive solid phase extraction (d-SPE) and micro-HPLC–MS/MS detection were highly applicable for the determination of selected perfluoroalkyl carboxylic acids and perfluoroalkane sulfonates in spices. The use of the polymer-based sorbent–ENV for the efficient PFASs extraction from spices based on QuEChERS method can be recommended. The level of spices contamination by perfluoroalkyl substances indicates that commonly and daily used spices may be contributor to the overall contamination of food by PFASs.
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Acknowledgments
We gratefully acknowledge project Grant No. 2015/17/B/NZ9/01623 from the National Science Centre, Poland.
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Magdalena Surma declares that she has no conflict of interest. Mariusz Piskuła declares that he has no conflict of interest. Wiesław Wiczkowski declares that he has no conflict of interest. Henryk Zieliński declares that he has no conflict of interest.
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Surma, M., Piskuła, M., Wiczkowski, W. et al. The perfluoroalkyl carboxylic acids (PFCAs) and perfluoroalkane sulfonates (PFSAs) contamination level in spices. Eur Food Res Technol 243, 297–307 (2017). https://doi.org/10.1007/s00217-016-2744-7
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DOI: https://doi.org/10.1007/s00217-016-2744-7