Production of monoclonal antibodies against fullerene C60 and development of a fullerene enzyme immunoassay

The aim of the present study was to produce monoclonal anti-fullerene C(60) antibodies and to develop the enzyme immunoassay for the detection in the first use of free fullerene C(60) both in solutions and in multicomponent biological probes. The immunization of mice with the conjugate of fullerene C(60) carboxylic derivative with thyroglobulin synthesized by carbodiimide activation led to the production of eight clones of anti-fullerene antibodies. The specificity of the antibody-fullerene binding was confirmed. Indirect competitive enzyme-linked immunosorbent assay (ELISA) was developed for the determination of water-soluble protein-conjugated fullerene, the fullerene aminocaproic acid, fullerenol and for pristine fullerene in solution. To solubilize extremely hydrophobic free fullerene C(60) a specially selected water-organic mixture compatible with immunoassay was proposed. The detection limit of free fullerene C(60) in solution was 2 μg L(-1). Fullerene C(60) was also detected by ELISA in organ homogenates of rats intraperitoneally or intragastrically administered with fullerene. To reduce the influence of biomatrices on the assay results a technique was developed for the biological sample pretreatment by the extraction of C(60) from bioprobe by toluene followed by the evaporation of toluene and dissolution of the fullerene-containing extract in the selected water-organic media. The ELISA procedure in the first use allowed the detection of fullerene C(60) in different tissues.     

Thermodynamics of Micelle Asymmetrization in Aqueous Sodium Decyl Sulfate Solution

The process of asymmetrization of spherical micelles in an aqueous sodium decyl sulfate solution is studied by scanning calorimetry. This process represents the intermicellar phase transition with an equilibrium temperature of 300 K occurring at a sodium decyl sulfate concentration of 0.12 mol/kg. The partial molar heat capacities of sodium decyl sulfate in a solution are determined and the thermodynamic functions of the rearrangement of micelles and their temperature dependences are calculated. The regions of the thermodynamic stability of solutions that contain spherical and nonspherical micelles, the former being predominant, are revealed. Equilibrium constants of the process and fractions of surfactant aggregated into spherical and nonspherical micelles are calculated for the model of monomolecular reversible reaction. For nonspherical micelles, the shape of the ellipsoid of revolution is proposed.     

Comparison of two express immunotechniques with polyelectrolyte carriers, ELISA and FIIAA, for the analysis of atrazine

Conventional immunoassays on microtiterplates are very useful analytical tools in environmental analysis, but the long assay times, usually in the range of hours, are a drawback. To overcome this disadvantage, the development of fast (express) assay formats is described, which use polyelectrolytes as carriers. Two semi-homogeneous immunochemical methods, namely the polyelectrolyte-ELISA (enzyme-linked immunosorbent assay) and the express-FIIAA (flow injection immunoaffinity analysis) for the analysis of the herbicide atrazine were set-up. Using polyclonal antisera for atrazine, the following results were obtained. Standard curves for atrazine showed a linear range from 3 to 100 μg l⁻¹ in polyelectrolyte-ELISA and 0.3-100 μg l⁻¹ in express-FIIAA. The test midpoints in polyelectrolyte-ELISA and express-FIIAA were 12 and 5 μg l⁻¹, respectively. The duration time of the immunochemical reaction was in both assays 15 min, but the total assay time differed (30 min (polyelectrolyte-ELISA) and 18 min (express-FIIAA)). A significant difference between the formats could be observed in the number of samples that can be determined per day. The polyelectrolyte-ELISA can handle samples in parallel on a microtiterplate (usually 20/plate), whereas in the express-FIIAA the samples are automatically analysed one after another. This first demonstration of these techniques shows the potential of these methods, but also their limitations.     

Development of a rapid, specific fluorescence polarization immunoassay for the herbicide chlorsulfuron

A strategy for design of a derivative of chlorsulfuron, which mimics half of the herbicide molecule, was proposed. The 1-[(2-chloro)phenylsulfonyl]monoamidosuccinic acid was synthesized as a derivative of chlorsulfuron for conjugation to carrier proteins. Rabbits were immunized and the resulting polyclonal antibodies were assessed by the fluorescence polarization technique. The antibodies were highly specific to chlorsulfuron. Cross-reactivity to the structurally similar sulfonylurea and urea herbicides chlorbromuron, amidosulfuron, chlortoluron, isoproturon, diuron and linuron was less than 0.1%. A rapid fluorescence polarization immunoassay (FPIA) for chlorsulfuron detection in water samples was developed and optimized. The detection limit of chlorsulfuron in 50 μl of sample was 10 ng ml⁻¹. Total time for the measurement of 10 samples is 7 min. The proposed FPIA is suitable for rapid testing for pesticide contamination where the highest sensitivity is not critical or in combination with pre-concentration techniques.     

Comparative study of strategies for antibody immobilization onto the surface of magnetic particles in pseudo-homogeneous enzyme immunoassay of aflatoxin B1

Pseudo-homogeneous enzyme immunoassay (EIA) of aflatoxin B1 (AFB1) was accomplished using anti-AFM1 monoclonal antibodies conjugated with magnetic particles (MPs). The assay includes the concentration of AFB1 from the test sample on the surface of the MP-antibody conjugate, the binding of the AFB1-peroxidase conjugate to free sites of the antibodies, the separation of the complexes that formed from unreacted components by means of magnetic field, and the evaluation of the enzymatic activity of MP-bound peroxidase. A comparative study of antibody conjugates, which were prepared by three different methods, namely, by physical adsorption on native MP and covalent binding to oleic acidor polystyrene-coated MPs, was performed. For these conjugates, the detection limits of EIA for AFB1 are 2.6, 0.4, and 0.6 ng/mL, respectively. The advantages of the pseudo-homogeneous EIA format as a tool for the highly sensitive control of toxic contaminants in food are the shorter time of incubation of immunoassay reagents (5 min; the total assay time is 20 min) and the possibility of concentrating the analyte from the test samples.     

Detection Limits of Immunoanalytical Systems: Limiting Factors and Methods of Reduction

Journal of Analytical Chemistry - One of the priority directions in the development of modern immunoanalytical systems is a reliable determination of analytes in very low concentrations. In this...     

Factors influencing the detection limit of the lateral-flow sandwich immunoassay: a case study with potato virus X

Key factors influencing the analyte detection limit of the sandwich immunochromatographic assay (ICA), namely, the size of gold nanoparticles, the antibody concentration, the conjugation pH, and characteristics of membranes, are discussed. The impacts of these factors were quantitatively characterized and compared for the first time using the same antigen (potato virus X). The antibody-colloidal gold conjugates synthesized at pH 9.0-9.5 (the pH was examined in the range from 7.5 to 10.0) and at an antibody concentration of 15 μg/mL (the concentration was tested from 10 to 100 μg/mL) demonstrated maximum binding with the analyte. The relationship between the size of gold nanoparticles and the ICA detection limit was determined. The detection limit decreases from 80 to 3 ng/mL (for antibodies with K (D) = 1.0 × 10(-9) M, data were obtained using a BIAcore X instrument) for a series of particles with a diameter from 6.4 to 33.4 nm (electron microscopy and dynamic light scattering data). In the case of larger particles (52 nm in diameter), the detection limit increases and reaches 9 ng/mL. A 10 mM phosphate buffer, pH 8, and a 50 mM phosphate buffer, pH 7, were the conditions of choice for the deposition of reactants. Taking into account these facts, we developed a lateral-flow test system for the rapid (10 min) detection of potato virus X in plant leaves. The ICA provided a visual detection limit of 3 ng/mL. In the case of the instrumental processing, potato virus X can be determined in the concentration range from 3 to 300 ng/mL with a detection limit 2 ng/mL.     

Use of gold nanoparticle-labeled secondary antibodies to improve the sensitivity of an immunochromatographic assay for aflatoxin B1

We describe a sensitive method for the immunochromatographic determination of aflatoxin B1. It is based on the following steps: 1) Competitive interaction between non-labeled specific primary antibodies and target antigens in a sample and in the test zone of a membrane; 2) detection of the immune complexes on the membrane by using a secondary antibodies labeled with gold nanoparticles. The method enables precise adjustment of the required quantities of specific antibodies and the colloidal (gold) marker. It was applied in a lateral flow format to the detection of aflatoxin B1 and exhibits a limit of detection (LOD) of 160 pg · mL⁻¹ if detected visually, and of 30 pg · mL⁻¹ via instrumental detection. This is significantly lower than the LOD of 2 ng · mL⁻¹ achieved by conventional lateral flow analysis using the same reagents.

Immunochromatography with secondary labeled antibodies caused 10-fold decrease of detection limit