Filtration-based tyramide amplification technique—a new simple approach for rapid detection of aflatoxin B<Subscript>1</Subscript>

The catalyzed reporter deposition (CARD) method of signal amplification, also called “tyramide signal amplification”, has been used in immunoassays not only to increase sensitivity but also to reduce assay time. The current approach to tyramide amplification in immunoassays involves slow incubation with agitation. In this paper we describe new filtration-based tyramide amplification and substrate visualization techniques. Compared with the standard method, this new approach greatly enhances spot intensities in membrane immunoassay and reduces biotinylated tyramide (B-T) and substrate consumption approximately fiftyfold, without loss of specificity. An improved test device and a cost-effective method for preparation of membranes for Super-CARD amplification have also been developed. The techniques have been used for rapid detection of aflatoxin B₁ (AFB₁) in a variety of foodstuffs with a detection limit of 12.5 μg kg⁻¹. The assay procedure involves sequential addition of standards or sample, AFB₁–horseradish peroxidase (HRP) conjugate, B-T, avidin–HRP, and substrate solution over anti-AFB₁ antibody-spotted zones of the membrane surface. The method saves time, improves reproducibility, eliminates many washing steps and avoids manipulation of the membranes between the different steps, while maintaining the sensitivity of the standard method. Average recoveries from different non-infected food samples spiked with AFB₁ at concentrations from 25 to 100 mg kg⁻¹ were between 95 and 105%. AFB₁ results obtained on different days for Aspergillus parasiticus infection of corn and groundnut samples correlated well with estimates obtained by HPLC. Figure The principle of filtration-based tyramide filtration technique     

Modelling of the impedimetric responses of an aflatoxin B1 immunosensor prepared on an electrosynthetic polyaniline platform

Aflatoxins are a group of mycotoxins that have deleterious effects on humans and are produced during fungal infection of plants or plant products. An electrochemical immunosensor for the determination of aflatoxin B₁ (AFB₁) was developed with AFB₁antibody (AFB₁-Ab) immobilized on Pt electrodes modified with polyaniline (PANi) and polystyrene sulphonic acid (PSSA). Impedimetric analysis shows that the electron transfer resistances of the Pt/PANi–PSSA electrode, the Pt/PANi–PSSA/AFB₁-Ab immunosensor and Pt/PANi–PSSA/AFB₁-Ab incubated in bovine serum albumin (BSA) were 0.458, 720 and 1,066 kΩ, respectively. These results indicate that electrochemical impedance spectroscopy (EIS) is a suitable method for monitoring the change in electron transfer resistance associated with the immobilization of the antibody. Modelling of EIS data gave equivalent circuits which showed that the electron transfer resistance increased from 0.458 kΩ for the Pt/PANi–PSSA electrode to 1,066 kΩ for the Pt/PANi–PSSA/AFB₁-Ab immunosensor, indicating that immobilization of the antibody and incubation in BSA introduced an electron transfer barrier. The AFB₁ immunosensor had a detection limit of 0.1 mg/L and a sensitivity of 869.6 kΩ L/mg.     

Development of a monoclonal antibody-based enzyme-linked immunosorbent assay for the analysis of glycyrrhizic acid

Glycyrrhizic acid (GL) is a major active compound of licorice. The specific monoclonal antibody (MAb) (designated as 8F₈A₈H₄2H₇) against GL was produced with the immunogen GL–BSA conjugate. The dissociation constant (K _d) value of the MAb was approximately 9.96×10⁻¹⁰ M. The cross reactivity of the MAb with glycyrrhetic acid was approximately 2.6%. The conventional indirect competitive enzyme-linked immunosorbent assay (icELISA) and simplified icELISA adapted with a modified procedure were established using the MAb. The IC₅₀ value and the detect range by the conventional icELISA were 1.1 ng mL⁻¹ and 0.2–5.1 ng mL⁻¹, respectively. The IC₅₀ value and the detect range by the simplified icELISA were 5.3 ng mL⁻¹ and 1.2–23.8 ng mL⁻¹, respectively. The two icELISA formats were used to analyze GL contents in the roots of wild licorice and different parts of cultivated licorice (Glycyrrhiza uralensis Fisch). The results obtained with the two icELISAs agreed well with those of the HPLC analysis. The correlation coefficient was more than 0.98 between HPLC and the two icELISAs. The two icELISAs were shown to be appropriate, simple, and effective for the quality control of raw licorice root materials.     

AFB1–AP Conjugate for Enzyme Immunoassay of Aflatoxin B1 in Corn Samples

Abstract

This article describes the conjugation between aflatoxin B₁ (AFB₁), one of the major mycotoxins, and alkaline phosphatase (AP), one of the most used enzymes for immunoassays. In addition, an application of the ELISA method for aflatoxin B₁ determination in corn is presented. Three AFB₁–AP conjugates in different toxin–enzyme ratios were prepared and tested. The ELISA results, developed with the most effective conjugate obtained, showed a satisfactory working range between 2.4 and 4000 ng of toxin/g of corn. The detection limit was 2 ng/g in corn samples, and recoveries ranged from 105 to 120%.     

Determination of vitamin B<Subscript>1</Subscript> in seawater and microalgal fermentation media by high-performance liquid chromatography with fluorescence detection

A highly sensitive high-performance liquid chromatographic method with fluorescence detection has been developed for determination of vitamin B₁. Vitamin B₁ was converted into a fluorescent compound by treatment with hydrogen peroxide–horseradish peroxidase and the derivative was subsequently analyzed by HPLC on a Waters Spherisorb ODS2 column (250 mm×4.6 mm ID, 5 μm) with 40:60 methanol–pH 8.5 acetate buffer solution as mobile phase and fluorescence detection at 440 nm (with excitation at 375 nm). The calibration graph was linear from 5.00×10⁻¹⁰ mol L⁻¹ to 5.00×10⁻⁷ mol L⁻¹ for vitamin B₁ with a correlation coefficient of 0.9991 (n=9). The detection limit was 1.0×10⁻¹⁰ mol L⁻¹. The method was successfully used for determination of vitamin B₁ at pg mL⁻¹ levels in microalgal fermentation media and seawater after solid-phase extraction. Recovery was from 89 to 110% and the relative standard deviation was in the range 1.1 to 4.3%.     

FAD-modified SiO2/ZrO2/C ceramic electrode for electrocatalytic reduction of bromate and iodate

SiO₂/ZrO₂/C carbon ceramic material with composition (in wt%) SiO₂ = 50, ZrO₂ = 20, and C = 30 was prepared by the sol–gel-processing method. A high-resolution transmission electron microscopy image showed that ZrO₂ and the graphite particles are well dispersed inside the matrix. The electrical conductivity obtained for the pressed disks of the material was 18 S cm⁻¹, indicating that C particles are also well interconnected inside the solid. An electrode modified with flavin adenine dinucleotide (FAD) prepared by immersing the solid SiO₂/ZrO₂/C, molded as a pressed disk, inside a FAD solution (1.0 × 10⁻³ mol L⁻¹) was used to investigate the electrocatalytic reduction of bromate and iodate. The reduction of both ions occurred at a peak potential of −0.41 V vs. the saturated calomel reference electrode. The linear response range (lrr) and detection limit (dl) were: BrO₃ ⁻, lrr = 4.98 × 10⁻⁵–1.23 × 10⁻³ mol L⁻¹ and dl = 2.33 μmol L⁻¹; IO₃ ⁻, lrr = 4.98 × 10⁻⁵ up to 2.42 × 10⁻³ and dl = 1.46 μmol L⁻¹ for iodate.     

Limitations in the use of horseradish peroxidase as an enyzme probe in the development of a homogeneous immunoassay for aflatoxin B1

Horseradish peroxidase (HRPO) was used as a probe to quantitate aflatoxin B₁ by a homogeneous immunoassay. The conjugation of AFB₁ to HRPO resulted in 54% loss of enyzme activity. In the presence of AFB₁ specific antibodies, the HRPO-AFB₁ conjugate showed reversal of its lost enzyme activity by 12%. This positive modulatory effect of antibody on the enzyme activity was used as an analytical tool to quantitate AFB₁. The homogeneous assay carried out with free AFB₁ and HRPO-AFB₁ conjugate in the presence of antibodies indicated poor linearity as compared to the heterogeneous assay. It was observed that the number of HRPO-lysine residues involved in AFB₁ conjugation were 6–8. The low level of modulation of enzyme activity by antibody with respect to HRPO-AFB₁ conjugate, could possibly be attributed to the limited number of lysine residues in the HRPO molecule and its proximity to the active site of the enzyme. Thus, HRPO was found to be limiting as an enzyme with respect to the homogeneous enzyme immunoassay for AFB₁ analysis. The antibodies raised were specific for AFB₁, and showed excellent linearity even at high dilution for the detection of AFB₁ by ELISA indicating that antibodies per se were not the limiting factor.     

Determination of additives in an electrolytic zinc bath by q1H-NMR spectroscopy

The use of proton nuclear magnetic resonance (¹H-NMR) for the quantification of additives in an electrolytic Zn bath is reported. A simple and quick method is described that does not need any prior sample preparation. Contrary to other analytical methods, the three additives in the bath, benzylidene acetone (BDA), benzoic acid (BA) and poly(ethylene glycol) (PE400), can be quantified. Two calibration methods were tried: integration of NMR signals with the use of an internal standard and partial least squares (PLS) regression applied to the characteristic NMR peaks. Both methods are compared and the univariate method was preferred because of simplicity, accuracy and precision. The following limits of detection were found: 0.30 g L⁻¹ BA, 0.08 g L⁻¹ BDA and 0.7 g L⁻¹ PE400 with dynamic ranges of at least 1.0–6.0, 0.1–0.6 and 3.0–18.0 g L⁻¹ respectively. Those concentration ranges are suitable to follow the concentration of additives in the bath in real time. ¹H-NMR spectra provide evidence for the BDA degradation pattern.     

Determination of rutin using a CeO2 nanoparticle-modified electrode

CeO₂ nanoparticles approximately 12 nm in size were synthesized and subsequently characterized by XRD, TEM and UV-vis spectroscopy. Then, a gold electrode modified with CeO₂ nanoparticles was constructed and characterized by electrochemical impedance spectroscopy (EIS) and cyclic voltammetry (CV). The modified electrode demonstrated strong catalytic effects with high stability towards electrochemical oxidation of rutin. The anodic peak currents (measured by differential pulse voltammetry) increased linearly with the concentration of rutin in the range of 5.0 × 10⁻⁷–5.0 × 10⁻⁴ mol · L⁻¹. The detection limit (S/N = 3) was 2.0 × 10⁻⁷ mol · L⁻¹. The relative standard deviation (RSD) of 8 successive scans was 3.7% for 5.0 × 10⁻⁶ mol · L⁻¹ rutin. The method showed excellent sensitivity and stability, and the determination of rutin in tablets was satisfactory.     

Chemiluminescent imaging analysis of interferon alpha in serum samples

Enzyme-linked immunosorbent assay (ELISA), horseradish peroxidase (HRP)-catalyzed fluorescent reaction, and oxalate chemiluminescence imaging analysis have been combined to develop a sensitive, simple, and rapid method for analysis of interferon alpha (α-IFN) in human serum samples. A typical “sandwich type” immunoassay was used. Reaction of o-phenylenediamine (OPD) with hydrogen peroxide (H₂O₂), catalyzed by HRP, produced 2,3-diaminophenazine (PDA), which was detected by chemiluminescence imaging analysis with the bis(2,4,6-trichlorophenyl)oxalate (TCPO)–H₂O₂–glyoxaline–PDA chemiluminescent system. The TCPO chemiluminescent imaging system is more sensitive and the chemiluminescence quantum yield is at least five times higher than for the luminol–H₂O₂–HRP–PIP (p-iodophenol) chemiluminescent imaging system. The results showed there was a very good linear correlation between response and amount of α-IFN in the range 1.3–156.0 pg mL⁻¹ (R = 0.9991) and the detection limit was 0.8 pg mL⁻¹ (S/N=3). The relative standard deviation (n = 9) was 4.7%. The proposed method has been used for successful analysis of the amount of α-IFN in human serum. The results obtained compared well with those obtained by conventional colorimetric ELISA and luminol chemiluminescent ELISA. Figure Procedures of the proposed method     

Polar herbicides,pharmaceutical products,perfluorooctanesulfonate (PFOS), perfluorooctanoate (PFOA), and nonylphenol and its carboxylates and ethoxylates in surface and tap waters around Lake Maggiore in Northern Italy

A survey of contamination of surface and drinking waters around Lake Maggiore in Northern Italy with polar anthropogenic environmental pollutants has been conducted. The target analytes were polar herbicides, pharmaceuticals (including antibiotics), steroid estrogens, perfluorooctanesulfonate (PFOS), perfluoroalkyl carboxylates (including perfluorooctanoate PFOA), nonylphenol and its carboxylates and ethoxylates (NPEO surfactants), and triclosan, a bactericide used in personal-care products. Analysis of water samples was performed by solid-phase extraction (SPE) then liquid chromatography–triple-quadrupole (tandem) mass spectrometry (LC–MS–MS). By extraction of 1-L water samples and concentration of the extract to 100 μL, method detection limits (MDLs) as low as 0.05–0.1 ng L⁻¹ were achieved for most compounds. Lake-water samples from seven different locations in the Southern part of Lake Maggiore and eleven samples from different tributary rivers and creeks were investigated. Rain water was also analyzed to investigate atmospheric input of the contaminants. Compounds regularly detected at very low concentrations in the lake water included: caffeine (max. concentration 124 ng L⁻¹), the herbicides terbutylazine (7 ng L⁻¹), atrazine (5 ng L⁻¹), simazine (16 ng L⁻¹), diuron (11 ng L⁻¹), and atrazine-desethyl (11 ng L⁻¹), the pharmaceuticals carbamazepine (9 ng L⁻¹), sulfamethoxazole (10 ng L⁻¹), gemfibrozil (1.7 ng L⁻¹), and benzafibrate (1.2 ng L⁻¹), the surfactant metabolite nonylphenol (15 ng L⁻¹), its carboxylates (NPE₁C 120 ng L⁻¹, NPE₂C 7 ng L⁻¹, NPE₃C 15 ng L⁻¹) and ethoxylates (NPE _n Os, n = 3-17; 300 ng L⁻¹), perfluorinated surfactants (PFOS 9 ng L⁻¹, PFOA 3 ng L⁻¹), and estrone (0.4 ng L⁻¹). Levels of these compounds in drinking water produced from Lake Maggiore were almost identical with those found in the lake itself, revealing the poor performance of sand filtration and chlorination applied by the local waterworks.     

Determination of lead in wine by hydride generation atomic fluorescence spectrometry in the presence of hexacyanoferrate(III)

A rapid, accurate, and precise method is described for the determination of Pb in wine using continuous-flow hydride generation atomic fluorescence spectrometry (CF-HGAFS). Sample pretreatment consists of ten-fold dilution of wine followed by direct plumbane generation in the presence of 0.1 mol L⁻¹ HCl and 1% m/v K₃[Fe(CN)₆] with 1% m/v NaBH₄ as reducing agent. An aqueous standard calibration curve is recommended for Pb quantification in wine sample. The method provides a limit of detection and a limit of quantification of 0.3 μg L⁻¹ and 1 μg L⁻¹, respectively. The relative standard deviation varies between 2–6% (within-run) and 4–11% (between-run) at 3–30 μg L⁻¹ Pb levels in wine. Good agreement has been demonstrated between results obtained by CF-HGAFS and direct electrothermal atomic absorption spectrometry in analyses of red and white wines within the concentration range of 9.2–25.8 μg L⁻¹ Pb.     

Electrochemical study of Meldola's blue,methylene blue and toluidine blue immobilized on a SiO<Subscript>2</Subscript>/Sb<Subscript>2</Subscript>O3 binary oxide matrix obtained by the sol-gel processing method

SiO₂/Sb₂O₃ (SiSb), having a specific surface area, S _BET, of 788 m² g⁻¹, an average pore diameter of 1.9 nm and 4.7 wt% of Sb, was prepared by the sol-gel processing method. Meldola's blue (MeB), methylene blue (MB) and toluidine blue (TB) were immobilized on SiSb by an ion exchange reaction. The amounts of the dyes bonded to the substrate surface were 12.49, 14.26 and 22.78 μmol g⁻¹ for MeB, MB and TB, respectively. These materials were used to modify carbon paste electrodes. The midpoint potentials (E _m) of the immobilized dyes were −0.059, −0.17 and −0.18 V vs. SCE for SiSb/MeB, SiSb/MB and SiSb/TB modified carbon paste electrodes, respectively. A solution pH between 3 and 7 practically did not affect the midpoint potential of the immobilized dyes. The electrodes presented reproducible responses and were chemically stable under various oxidation-reduction cycles. Among the immobilized dyes, MeB was the most efficient to mediate the electron transfer for NADH oxidation in aqueous solution at pH 7. In this case, amperometric detection of NADH at an applied potential of 0 mV vs. SCE gives linear responses over the concentration range of 0.1–0.6 mmol L⁻¹, with a detection limit of 7 μmol L⁻¹.     

Limitations in the use of horseradish peroxidase as an enyzme probe in the development of a homogeneous immunoassay for aflatoxin B1

Horseradish peroxidase (HRPO) was used as a probe to quantitate aflatoxin B₁ by a homogeneous immunoassay. The conjugation of AFB₁ to HRPO resulted in 54% loss of enyzme activity. In the presence of AFB₁ specific antibodies, the HRPO-AFB₁ conjugate showed reversal of its lost enzyme activity by 12%. This positive modulatory effect of antibody on the enzyme activity was used as an analytical tool to quantitate AFB₁. The homogeneous assay carried out with free AFB₁ and HRPO-AFB₁ conjugate in the presence of antibodies indicated poor linearity as compared to the heterogeneous assay. It was observed that the number of HRPO-lysine residues involved in AFB₁ conjugation were 6–8. The low level of modulation of enzyme activity by antibody with respect to HRPO-AFB₁ conjugate, could possibly be attributed to the limited number of lysine residues in the HRPO molecule and its proximity to the active site of the enzyme. Thus, HRPO was found to be limiting as an enzyme with respect to the homogeneous enzyme immunoassay for AFB₁ analysis. The antibodies raised were specific for AFB₁, and showed excellent linearity even at high dilution for the detection of AFB₁ by ELISA indicating that antibodies per se were not the limiting factor.     

Estimation of measurement uncertainty for the determination of aflatoxin M1 in milk using immunoaffinity clean-up procedures

A measurement uncertainty estimated for aflatoxin M₁ determination in milk sample has been calculated using data generated from analytical method validation studies. The protocol adopted is described in detail in document LGC/VAM/1998/088. The uncertainty budget was based on precision, trueness and ruggedness data. The individual contributions are described in detail. The expanded uncertainty for aflatoxin M ₁ at a concentration of 20 ng L⁻¹ was estimated as 2.81 ng L⁻¹. This was calculated using a coverage factor of two which gives a level of confidence of approximately 95%. Presented at AOAC Europe / Eurachem Symposium March 2005, Brussels, Belgium     

Synthesis and spectral properties of titanium(iv) polynuclear hydroxo complexes stabilized in solution by the [PW11O39]7− heteropolyanion

Unsaturated heteropolyanions (HPA) [PW₁₁O₃₉]⁷⁻ stabilize Ti^IV hydroxo complexes in aqueous solutions (Ti: PW₁₁ [PW₁₁O₃₉]⁷⁻⪯12, pH 1–3). Spectral studies (optical,¹⁷O and³¹P NMR, and IR spectra) and studies by the differential dissolution method demonstrated that Ti^IV hydroxo complexes are stabilized through interactions of polynuclear Ti^IV hydroxo cations with heteropolyanions [PW₁₁TiO₄₀ ⁵⁻ formed. Depending on the reaction conditions, hydroxo cations Ti _n−1O _x H _y ^m+ either add to oxygen atoms of the W−O−Ti bridges of the heteropolyanions to form the complex [PW₁₁TiO₄₀·Ti _n−1O _x H _y ] ^k− (at [HPA]=0.01 mol L⁻¹) or interact with Ti^IV of the heteropolyanions through the terminal o atom to give the polynuclear complexes [PW₁₁O₃₉Ti−O−Ti _n−1O _x H _y ]^q− (at [HPA]=0.2 mol L⁻¹). When the complexes of the first type were treated with H₂O₂, Ti^IV ions added peroxo groups. Translated fromIzvestiya Akademii Nauk. Seriya Khimicheskaya, No. 5, pp. 914–920, May, 1997.     

Chemiluminescence Method for the Determination of Glutathione in Human Serum Using the Ru(phen)3 2+ – KMnO4 System

A simple, rapid and specific chemiluminescence (CL) method for the determination of glutathione has been developed. The method is based on the enhanced CL of the reaction between Ru(phen)₃ ²⁺ (phen = 1,10-phenanthroline) and KMnO₄ by glutathione in HCl medium. Under the optimum conditions, the response is linearly proportional to the concentration of glutathione between 1.5 × 10⁻⁷ and 1.0 × 10⁻⁵ mol L⁻¹. The dection limit for glutathione (5.8 × 10⁻⁸ mol L⁻¹) is about 10 and 200 times better than those of the spectrophotometric method using Ellman regent and the Lucigenin – CL method, respectively. The final procedure allows the determination of glutathione in human serum with recoveries of 92%–108%. A satisfactory agreement was obtained with a mean relative difference of 2.5% compared to the HPLC method.     

Immunosensors for pollutants working in organic media. Study of performances of different tracers with luminescent detection

A comparative study of enzymatic and non-enzymatic labels combined with luminescence detection, developed for immunosensing of pesticide residues (carbaryl, 1-naphthol, irgarol 1051) in organic media, is presented. Peroxidase and alkaline phosphatase enzymes with fluorogenic (3-p-hydroxyphenylpropanoic acid) and luminogenic (AMPPD derivative) substrates, respectively, were assessed as enzymatic markers. As an alternative, terbium(III) chelate, with time-resolved fluorescence detection, was evaluated as a non-enzymatic label. The best sensitivity was achieved by use of alkaline phosphatase in an immunocomplex capture assay format (I ₅₀ values 0.06, 0.27, and 7.45 μg L⁻¹ in buffer, 1:1 methanol–buffer, and methanol, respectively). Results were also good (I ₅₀ 1.00 and 6.30 μg L⁻¹ for water and aqueous–organic mixture, respectively) for Tb(III) chelate in an immobilized conjugate assay format. Use of alkaline phosphatase label to measure carbaryl (100 ng L⁻¹) in different spiked river water samples, after solid-phase extraction and analyte elution with an ethyl acetate–methanol mixture, resulted in recoveries ranging from 81 to 98%, with acceptable precision (CV 4–14%, n=4).     

Simultaneous ion chromatographic determination of selenium and metal ions in waters at trace level

Summary An ion-chromatographic procedure is described for the determination of selenium (VI) at μg L⁻¹ level in the presence of anions and heavy metal ions. Maximum permissible concentrations and effects from each interfering substance were investigated for the Se concentration range 12.5–1,000 μg L⁻¹. The method, optimized for the detection of SeO ₄ ²⁻ , gives results suitable for speciation analysis. Total selenium can be determined after complete conversion to selenate ion by oxidation with KMnO₄. The detection limit of selenium is 4.8 μg L⁻¹ (0.96 ng for 200 μL sample). Paper presented at the 41st Pittsburgh Conference, New York, March 5–9, 1990.     

Study of a toxin–alkaline phosphatase conjugate for the development of an immunosensor for tetrodotoxin determination

This paper describes a direct competitive immunoenzymatic spectrophotometric assay (ELISA) for tetrodotoxin (TTX) determination and the adaptation of this method for use in an electrochemical assay format. The novelty of this work involves the use of the antigen labelled with alkaline phosphatase (AP); this conjugate was prepared in our laboratory as there is no commercially available conjugate of any kind for TTX. The new conjugate was characterized in terms of its affinity for the specific antibody as well as the residual concentration and the residual activity of the enzyme (AP) incorporated as label. The proposed method based on the new conjugate showed satisfactory results for TTX determination: for the spectrophotometric method the dynamic range was 4–15 ng mL⁻¹ with a limit of detection (LOD) of 2 ng mL⁻¹ (R=0.9247), whereas for the electrochemical protocol the dynamic range was 2–50 ng mL⁻¹ and the LOD was1 ng mL⁻¹.