Rapid detection of a foreign protein in milk using IMS–SERS

A method for rapid detection of foreign protein contamination in complex food matrices is critically needed. Here we present a novel method that combines immunomagnetic separation (IMS) and surface‐enhanced Raman scattering (SERS) to detect ovalbumin (OVA), an egg white protein, added into whole milk. IMS was used to specifically capture the OVA out of the milk. Then SERS was applied to analyze the IMS eluate using silver dendrites as the substrate. Two SERS sample preparation methods, namely solution based and substrate based, were used to prepare the IMS eluate for SERS analysis. Results show both methods were able to detect 1 µg OVA in 1 ml milk (1 part per million). Based on the results of principal component analysis and partial least‐squares analysis, solution SERS was more capable of quantitative analysis, while substrate SERS was more sensitive for qualitative analysis. The total analytical time for IMS–SERS was less than 20 min, which satisfied the requirement of rapid detection in a milk processing facility. Copyright © 2011 John Wiley & Sons, Ltd.     

On‐site detection of phosgene agents by surface‐enhanced Raman spectroscopy coupled with a chemical transformation approach

Phosgene and its analogs are greatly harmful to the public health, environmental safety and homeland security as widely used industrial substances with extremely high toxicity. In order to rapidly evaluate the emergency risk caused by these chemicals, a new highly sensitive method based on surface‐enhanced Raman spectroscopy (SERS) technique for measurement of phosgene agents was developed for the first time. Coupled with a chemical transformation approach, the highly toxic phosgene was conveniently converted to a SERS‐sensitive probe, i.e. iodine (I₂), with low toxicity or non‐toxicity. The characteristic SERS peak in 459 cm⁻¹ was used for quantitation and was presumed as a formation of triiodide anion (I₃⁻), which was induced in an iodide (I⁻)‐aggregation Au NPs system. The total measurement can be completed in ~20 min with the limits of detection of ~60 µg/l (phosgene) and ~30 µg/l (diphosgene), respectively, on a portable Raman spectrometer. This work is the first report of SERS measurement on phosgene and diphosgene in a quantitative level. This method is expected to meet the requirements of on‐site detection of phosgene agents, promote emergency responses and raise more opportunities for the portable SERS applications. Copyright © 2015 John Wiley & Sons, Ltd.     

Detection of melamine in liquid milk using surface‐enhanced Raman scattering spectroscopy

Melamine, a nitrogen‐rich chemical, has recently caused enormous economic losses to the food industry due to the cases of milk products adulterated by melamine. This has led to an urgent need of rapid and reliable methods for detection of melamine in food. In this study, surface‐enhanced Raman scattering (SERS) spectroscopy was used to detect melamine in liquid milk. The sample preparation with liquid milk is very easy; it has to be only diluted with double‐distilled water followed by centrifugation. By using a silver colloid, at least a 10⁵‐fold enhancement of the Raman signal was achieved for the measurement of melamine. The limit of detection by this method was 0.01 µg ml⁻¹ for melamine standard samples. Based on the intensity of the Raman vibrational bands normalised to that of the band at 928 cm⁻¹ (CH₂), an external standard method was employed for quantitative analysis. The linear regression square (R²) of the curve was 0.9998; the limit of quantitation using this approach was 0.5 µg ml⁻¹ of melamine in liquid milk; the relative standard deviation was ≤10%; and recoveries were from 93 to 109%. The test results for SERS were very precise and as good as those obtained by liquid chromatography/tandem mass spectrometry. The method was simple, fast(only needs about 3 min), cost effective, and sensitive for the detection of melamine in liquid milk samples. Therefore, it is more suitable for the field detection of melamine in liquid milk. Copyright © 2010 John Wiley & Sons, Ltd.     

Detection of protein molecules by surface‐enhanced Raman spectroscopy‐based immunoassay using 2–5 nm gold nanoparticle lables

Here we report the synthesis of 2–5 nm size gold nanoparticle labels for surface‐enhanced Raman Spectroscopy (SERS) based immunoassay to detect protein molecules. The Au nanoparticles were conjugated with fluorescein isothiocyanate (FITC) and goat anti‐h‐IgG (immunoglobin) and the resultant particles were used for the detection of h‐IgG. Commercially available nitrocellulose strip and silver enhancement method were used for SERS‐based immunoassays. The FITC acts as a Raman probe, and vibrational fingerprint of this molecule was used for the detection of h‐IgG in concentration ranging from 1 to 100 ng/µl. Our Raman probe is robust and small in size and has high water solubility with minimum steric effect during antigen–antibody binding. Copyright © 2007 John Wiley & Sons, Ltd.     

Simple and sensitive detection of cyanide using pinhole shell‐isolated nanoparticle‐enhanced Raman spectroscopy

Cyanide is a great threat to public health, environmental safety and homeland security because of its extremely high toxicity and widespread usage in industry. Countering such a threat can be greatly aided by a rapid, sensitive, on‐site detection method. Here, a pinhole shell‐isolated nanoparticle‐enhanced Raman spectroscopy (SHINERS) technique for cyanide sensing has been established, and a limit of detection lower to 1 µg l⁻¹ level in water was achieved on a portable Raman spectrometer, owing to the magnificent local electromagnetic field enhancement generated by the interaction between cyanide anion and the uncovered Au surface inside the pinholes. Meanwhile, the silica shell outside the Au core could significantly improve the stability of the substrate by preventing the dissolution of Au in cyanide solution, thereby making this assay more feasible for practical use. The linear range was from 1 to 100 µg l⁻¹ with excellent selectivity over thiocyanide and other common ions. For applications on complex matrices such as polluted water, beverages etc., a simple online hydrogen generator was designed and successfully coupled with pinhole SHINERS to achieve a good measurement of cyanide. This pinhole SHINERS‐based method is rapid, simple, with good stability and feasibility for the in‐field detection of cyanide, and we hope that it will further raise more opportunities for portable SERS applications. Copyright © 2014 John Wiley & Sons, Ltd.     

Rapid and simple detection of sodium thiocyanate in milk using surface‐enhanced Raman spectroscopy based on silver aggregates

Surface‐enhanced Raman spectroscopy (SERS) was used for rapid detection of sodium thiocyanate in milk employing silver aggregates as active substrate. Silver nanoparticles were induced to silver aggregates by trichloroacetic acid (TCA). The limit of detection (LOD) for sodium thiocyanate was 10⁻² µg ml⁻¹ in water with an analytical enhancement factor of 5.4 × 10⁶. The silver aggregates represent good reproducibility and stability. Good linear relationship was obtained for sodium thiocyanate in milk at concentration ranges from 0.1 to 10 µg ml⁻¹ (R² = 0.995). Using TCA as protein precipitator, silver colloid would aggregate spontaneously when mixing with samples during SERS measurement without the need of additional aggregating agent. The simple pretreatment procedures and analytical methods are less time consuming (<10 min) and environmentally friendly, making the proposed method much practical for in situ detection of sodium thiocyanate in market milk. Copyright © 2014 John Wiley & Sons, Ltd.     

Determination of Cr(III) and Cr(VI) in water by wavelength‐dispersive X‐ray fluorescence spectrometry after preconcentration with an ion‐exchange resin disk

A rapid and simple method using an ion‐exchange resin disk combined with wavelength‐dispersive X‐ray fluorescence (WDXRF) spectrometry was developed for the determination of Cr(III) and Cr(VI) in water. A 100‐ml water sample was first adjusted to pH 3 with nitric acid and then passed through an anion‐exchange resin disk placed on top of a cation‐exchange resin disk at a flow rate of 1 ml min^?1 to separate Cr(III) and Cr(VI). Anionic Cr(VI) was preconcentrated on the upper anion‐exchange resin disk, whereas cationic Cr(III) was preconcentrated on the lower cation‐exchange resin disk. Each ion‐exchange resin disk was dried at 100 °C for 30 min in an electric oven and coated with a commercially available laminate film. The specimens were measured using a WDXRF spectrometer. The calibration curves of Cr(III) and Cr(VI) showed good linearity in the range 1–10 µg. The detection limits corresponding to three times the standard deviation (n = 5) of blank values were 0.17 µg for Cr(III) and 0.16 µg for Cr(VI). If a 1‐l water sample is used, these limits would be 0.17 and 0.16 µg l^?1, respectively. A spike test for 50 µg l^?1 Cr(III) and Cr(VI) in tap water and river water showed quantitative recoveries (94–114%), although this was not observed for mineral drinking water owing to the overlap of V Kβ with Cr Kα. The recovery after overlap correction was satisfactory (115%). Copyright © 2011 John Wiley & Sons, Ltd.     

Detection of the potential tumor marker of AFP using surface‐enhanced Raman scattering‐based immunoassay

The development of rapid, highly sensitive detection methods for α‐fetoprotein (AFP) is very important. As hepatocellular carcinoma is closely related to the level of AFP in the blood, it is necessary to maintain an AFP concentration below the safety limit. In this paper, we propose a universal, rapid, sensitive, and highly specific immunoassay system utilizing gold nanoparticles (AuNPs) and surface‐enhanced Raman scattering (SERS). This new system features a sandwich structure combining mercaptobenzoic acid‐labeled immunogold nanoparticles with the antigen and the antibody atop a pre‐designed substrate made of a glass slide modified with AuNPs. This SERS‐based immunoassay can detect AFP concentrations as low as 100 pg/ml, which is a significant improvement on the capabilities of the enzyme‐linked immunosorbent assay method. A good linear relationship between the SERS peak intensity and the logarithm of antigen concentrations (from 1 ng/ml to 100 ng/ml) was observed. This technique provides an effective model for the detection of biomarkers in medical diagnostics, criminal investigation, and other fields. Copyright © 2013 John Wiley & Sons, Ltd.     

SERS microRaman spectral probing of adsorbate‐containing,liquid‐overlayed nanosponge Ag aggregates assembled from fractal aggregates

Adsorbate‐containing, nanosponge Ag aggregates overlayed by a thin (~1.5 mm) liquid layer are reported as a new type of sample for Surface‐enhanced Raman scattering (SERS) microRaman spectral measurements and adsorbate (analyte) detection. Macroscopic Ag aggregates (of about 1.5 × 1.0 × 0.025 mm size) with the nanosponge internal morphology (revealed by Scanning electron microscopy (SEM)) were prepared by 3D assembling of fused fractal aggregates (D = 1.84 ± 0.04) formed in Ag nanoparticle hydrosol/HCl/adsorbate systems with 2,2’‐bipyridine (bpy) and/or a cationic free‐base tetrakis(2‐methyl‐4‐pyridiniumyl) porphine (H₂TMPyP) as the testing adsorbates. For SERS microRaman measurements, the macroscopic aggregate was overlayed by a thin (~1.5 mm) layer of the residual liquid. Preparation procedure, nanoscale imaging, and SERS spectral probing including the determination of the detection limits of the adsorbates revealed the following advantages of the adsorbate‐containing, liquid‐overlayed 3D nanosponge aggregate as a sample for SERS microRaman spectral measurements: (1) localization of adsorbate (analyte) into hot spots and, simultaneously, prevention of the analyte decomposition during the spectral measurement (carried out without an immersion objective), (2) fast and simple sample preparation, and (3) minimization of sample volume and an efficient concentration of hot spots into the focus of the laser beam. The advantages of the nanosponge Ag aggregates are further demonstrated by the 40 fmol limit of detection of bpy as Ag(0)‐bpy surface complex, as well as by preservation of the native structure of the cationic free‐base porphyrin H₂TMPyP. Copyright © 2015 John Wiley & Sons, Ltd.     

Surface‐enhanced Raman scattering‐based approach for DNA detection at low concentrations via polyvinyl alcohol‐protected silver grasslike patterns

A simple method is demonstrated to detect DNA at low concentrations on the basis of surface‐enhanced Raman scattering (SERS) via polyvinyl alcohol‐protected silver grasslike patterns (PVA‐Ag GPs) grown on the surface of the common Al substrate. By the SERS measurements of sodium citrate and thymine, the PVA‐Ag GPs are shown to be an excellent SERS substrate with good activity, stability and reproducibility. With the use of the tested molecule of thymine, the enhancement factor of the PVA‐Ag GPs is up to ~1.4 × 10⁸. The PVA‐Ag GPs are also shown to be an excellent SERS substrate with good biocompatibility for DNA detection, and the detection limit is down to ~10⁻⁵ mg/g. Meanwhile, the assignations of the Raman bands and the adsorption behaviors of the DNA molecules are also analyzed. In this work, the geometry optimization and the wavenumber analysis of adenine–Ag and guanine–Ag complexes for the ground states are performed using density functional theory, B3LYP functional and the LanL2DZ basis set. The transition energies and the oscillator strengths of adenine–Ag and guanine–Ag for the lowest six singlet excited states were calculated by using the time‐dependent density functional theory method with the same functional and basis set. The results show that the charge transfer in the adenine–Ag and guanine–Ag complexes should be the chemical factor for the SERS of the DNA molecules. Lastly, this method may be employed in large‐scale preparation of substrates that have been widely applied in the Raman analysis of DNA because the fabrication process is simple and inexpensive. Copyright © 2011 John Wiley & Sons, Ltd.     

A SERS‐active enzymatic product used for the quantification of disease‐related molecules

In this paper, a method for enhancing the analysis of biologic materials was designed. This method incorporated the surface‐enhanced Raman scattering (SERS) technique and an enzyme catalysis‐based bioassay to develop a more efficient analysis procedure. Using this combination, the quick and simple detection of disease‐related molecules (the human cardiac isoform of troponin T, cTnT) in human serum was achieved. This method utilizes enzyme catalysis to develop a H₂O₂‐horseradish peroxidase (HRP)‐3,3′,5,5′‐tetramethylbenzidine (TMB) chromogenic system, and the final enzymatic product TMB²⁺ revealed perfect SERS activities. By analyzing a concentration‐dependent SERS spectrum, the quantitative analysis was accomplished. Our findings reveal that the proposed method has a wider linear range and a more sensitive detection limit compared with traditional chromogenic tests. In summary, two existing methods have been combined to create a new model, which has the potential to be used for the bioanalysis and early diagnosis of diseases. Copyright © 2013 John Wiley & Sons, Ltd.     

SERS detection of proteins on micropatterned protein‐mediated sandwich substrates

One of the greatest challenges in developing protein chips is the detection of trace amounts of proteins on their surfaces. Traditionally employed techniques, such as optical microscopy and fluorescence, are effective and widely used, but it is sometimes hard to obtain fingerprint signals of biomolecules. In this paper, we use surface‐enhanced Raman scattering (SERS) spectroscopy as a platform for protein detection. Micropatterned protein‐mediated Au/Ag sandwich structures were employed as the detecting objects. Two types of proteins, pure hemoprotein and immunocomplex, were used as the media. Au/Ag layers were used as the SERS substrates. The resulting spectra showed good sensitivity and resolution. It indicates that SERS is a powerful tool in protein detection and has great potential for application in protein chips. Copyright © 2011 John Wiley & Sons, Ltd.     

A stable ‘sandwich’ system of Surface‐Enhanced Resonance Raman Scattering for the analysis of β‐carotenes in a photosynthetic pigment‐protein complex

In plants, Photosystem I (PSI) is composed of a core complex and a membrane‐associated antenna complex light‐harvesting complex I that captures light and funnels its energy to the core complex. To obtain Raman structural information on β‐carotenes embedded in the PSI core complex, a ‘sandwich’ system of roughened silver slice: target protein complexes: single silver nanoparticles was fabricated for Surface‐Enhanced Resonance Raman Scattering (SERRS) measurements. This study provided a method to overcome spectral irreproducibility, which is the main drawback of Surface‐Enhanced Raman Scattering/SERRS‐based studies. The Raman spectra of β‐carotenes embedded in the PSI core complex can be obtained at very low sample concentrations (1–5 µg Chl/ml) and high signal/noise ratios. The β‐carotenes in the spinach PSI core complex were predominantly all‐trans configuration. The membrane protein‐mediated adsorption of silver nanoparticles induced the uniform distribution of a large number of single nanoparticles, which contributed to achieving highly reproducible SERRS spectra. This study is the first to apply single silver nanoparticle‐based SERRS analysis in membrane proteins. Copyright © 2013 John Wiley & Sons, Ltd.     

Near‐infrared surface‐enhanced Raman spectroscopy (NIR‐SERS) studies on oxyheamoglobin (OxyHb) of liver cancer based on PVA‐Ag nanofilm

A near‐infrared surface‐enhanced Raman spectroscopy (NIR‐SERS) method was employed for oxyheamoglobin (OxyHb) detection to develop a simple blood test for liver cancer detection. Polyvinyl alcohol protected silver nanofilm (PVA‐Ag nanofilm) used as the NIR‐SERS active substrate to enhance the Raman scattering signals of OxyHb. High quality NIR‐SERS spectrum from OxyHb adsorbed on PVA‐Ag nanofilm can be obtained within 16 s using a portable Raman spectrometer. NIR‐SERS measurements were performed on OxyHb samples of healthy volunteers (control subjects, n = 30), patients (n = 40) with confirmed liver cancer (stage I, II and III) and the liver cancer patients after surgery (n = 30). Meanwhile, the tentative assignments of the Raman bands in the measured NIR‐SERS spectra were performed, and the results suggested cancer specific changes on molecule level, including a decrease in the relative concentrations and the percentage of aromatic amino acids of OxyHb, changes of the vibration modes of the C_aH_m group and pyrrole ring of OxyHb of liver cancer patients. In this paper, principal component analysis (PCA) combined with independent sample T test analysis of the measured NIR‐SERS spectra separated the spectral features of the two groups into two distinct clusters with the sensitivity of 95.0% and the specificity of 85.7%. Meanwhile, the recovery situations of the liver cancer patients after surgery were also assessed using the method of discriminant analysis‐predicting group membership based on PCA. The results show that 26.7% surgeried liver cancer patients were distinguished as the normal subjects and 63.3% were distinguished into the cancer. Our study demonstrated great potentials for developing NIR‐SERS OxyHb analysis into a novel clinical tool for non‐invasive detection of liver cancers. Copyright © 2013 John Wiley & Sons, Ltd.     

Quick detection of contaminants leaching from polypropylene centrifuge tubes with surface‐enhanced Raman spectroscopy and ultraviolet absorption spectroscopy

Anomalous surface‐enhanced Raman scattering (SERS) peaks were identified for liquid sample stored in polypropylene (PP) centrifuge tubes for months. We observed unexpected Raman peaks during experiments with thiamine hydrochloride aqueous solutions stored in PP tubes for 2 months. In order to identify the contaminants, we have performed SERS experiments on deionized (DI) water stored in PP centrifuge tubes for 2 months and compared them with those from fresh DI water sample. We have also carried out ultraviolet (UV) absorption spectra for both fresh and contaminated water. We believe that the water is contaminated because of chemicals leaching from the PP tube. From the gas chromatography‐mass spectrometry data, the main contaminants were found to be phthalic acid (PA) and its derivatives. Further SERS and UV absorption experiment for PA correlated well with the anomalous peaks identified earlier. We qualitatively confirmed the identification and quantitatively estimated the concentration of the suspect contaminants as between 1 and 10 µM with both SERS and UV absorption spectroscopy. With UV absorption spectroscopy, we precisely estimated the concentration as 2.1 µM . We have shown that the sample in PP tube can be contaminated by the leaching chemicals upon long‐term storage, and suggest SERS and UV absorption spectroscopy as two quick and simple techniques to detect the contamination. Copyright © 2011 John Wiley & Sons, Ltd.     

Solution‐based SERS method to detect dithiocarbamate fungicides in different real‐world matrices

Surface‐enhanced Raman scattering (SERS) has become a valuable tool for the characterization of trace quantities of environmental toxins. Utilizing established wet chemical synthetic protocols, dogbone‐shaped colloidal gold nanoparticle substrates with sharp features were prepared with regions that exhibit significant SERS enhancement due to the lightning rod effect. These highly enhancing substrates were utilized for the quantitative determination of two dithiocarbamate fungicides by SERS in several complex matrices such as tap water, apple juice, and vegetable juice. Limits of detection and quantitation are reported and compared with Environmental Protection Agency mandated maximum allowable concentrations in tap water. In the case of tap water, limits of detection of 13.39 ± 3.89 nM for thiram and 1.78 ± 0.20 nM for ferbam was achieved. The sensitivity of the solution‐based SERS method decreased with increasing complexity of the matrix in which the limit of detection achieved in apple juice is 47.22 nM for thiram and 11.88 ± 1.38 nM for ferbam and that for vegetable juice is 87.01 ± 2.88 nM for thiram and 36.72 ± 2.90 nM for ferbam. It was found that using the solution‐based SERS method results in sensitivities that are greater than that required by Environmental Protection Agency mandated maximum allowable concentrations for complex matrices such as apple and vegetable juice. Copyright © 2013 John Wiley & Sons, Ltd.     

A facile method for the synthesis of large‐size Ag nanoparticles as efficient SERS substrates

Silver nanoparticles (Ag NPs) enjoy a reputation as an ultrasensitive substrate for surface‐enhanced Raman spectroscopy (SERS). However, large‐scale synthesis of Ag NPs in a controlled manner is a challenging task for a long period of time. Here, we reported a simple seed‐mediated method to synthesize Ag NPs with controllable sizes from 50 to 300 nm, which were characterized by scanning electron microscopy (SEM) and UV–Vis spectroscopy. SERS spectra of Rhodamine 6G (R6G) from the as‐prepared Ag NPs substrates indicate that the enhancement capability of Ag NPs varies with different excitation wavelengths. The Ag NPs with average sizes of ~150, ~175, and ~225 nm show the highest SERS activities for 532, 633, and 785‐nm excitation, respectively. Significantly, 150‐nm Ag NPs exhibit an enhancement factor exceeding 10⁸ for pyridine (Py) molecules in electrochemical SERS (EC‐SERS) measurements. Furthermore, finite‐difference time‐domain (FDTD) calculation is employed to explain the size‐dependent SERS activity. Finally, the potential of the as‐prepared SERS substrates is demonstrated with the detection of malachite green. Copyright © 2016 John Wiley & Sons, Ltd.     

Silica‐overcoated substrates for detection of proteins by surface‐enhanced Raman spectroscopy

Ag film over nanosphere (AgFON) substrates for surface‐enhanced Raman spectroscopy (SERS) are shown to be ineffective for the detection of proteins in phosphate buffer solution (PBS) because of the decomposition of the substrate resulting in a total loss of SERS activity. However, modification of these substrates with SiO₂ overlayers overcomes this problem. The SiO₂ overlayers are produced by filtered arc deposition (FAD) and are characterised by atomic force microscopy (AFM). Their porosity is examined using Raman spectroscopy and the detection of cytochrome c and bovine serum albumin in PBS is successfully demonstrated. These findings show promise for the detection of proteins in biologically relevant conditions using Ag‐based SERS substrates. Copyright © 2008 John Wiley & Sons, Ltd.     

Biocompatible gold/silver nanostars for surface‐enhanced Raman scattering

Raman‐enhancing properties of chitosan (CS)‐coated gold/silver nanostars (Au/AgNSs) were demonstrated by using them as a surface‐enhanced Raman scattering (SERS) probe. Based on the energy‐dispersive X‐ray spectroscopy element distribution maps and highly enhanced SERS spectra, we suggest that the incorporation of silver into the NS tips leads to a stronger SERS behavior. The SERS spectra of the proteins adsorbed on the NS surface greatly differ from their respective Raman spectra in both the band positions and relative intensities, indicating that the protein molecules penetrate through the CS coating layer and interact closely with the NS surface. Raman and SERS spectra of Chlamydia trachomatis protease/proteasomelike activity factor are reported for the first time, demonstrating the potential of these NSs for the development of a diagnosis method for Chlamydia based on SERS. The results showed a good SERS performance of the Au/AgNSs and their potential for SERS detection of biomolecules. Copyright © 2016 John Wiley & Sons, Ltd.     

Preparation of arsenic‐containing white rice grains as calibration standards for X‐ray fluorescence analysis of total arsenic in cereals

A preparation method of arsenic‐containing white rice grains as calibration standards was developed for the X‐ray fluorescence (XRF) analysis of arsenic in rice grains. Calibration standards were prepared by adding 10 g of white rice grains (from Japan) to 100 ml methanol‐containing dimethylarsinic acid corresponding to 2–100 µg arsenic. The mixture was heated, dried at 150 °C, cooled to room temperature, and then stored in a silica gel desiccator. A total of 5.0 g of each calibration standard was packed into a polyethylene cup (32 mm internal diameter and 23 mm height) covered with a 6‐µm‐thick polypropylene film and then analyzed by wavelength‐dispersive XRF spectrometry. The calibration curve for arsenic obtained from the white rice grains containing arsenic showed good linearity over a concentration range of 0.21–5.00 mg kg^?1 arsenic. The limit of detection of arsenic was 0.080 mg kg^?1. To check the reliability of the XRF method, the concentrations of arsenic in six samples of grain cereals and two samples of flour were compared with those obtained by atomic absorption spectrometry after acid decomposition. The values obtained by both analytical methods showed good agreement. Copyright © 2016 John Wiley & Sons, Ltd.