Your search keyword '"Tetala KK"' showing total 5 results

1. Selective depletion of neuropathy-related antibodies from human serum by monolithic affinity columns containing ganglioside mimics.

Author

Tetala KK, Heikema AP, Pukin AV, Weijers CA, Tio-Gillen AP, Gilbert M, Endtz HP, van Belkum A, Zuilhof H, Visser GM, Jacobs BC, and van Beek TA

Subjects

Adsorption, Animals, Antibodies, Monoclonal chemistry, Enzyme-Linked Immunosorbent Assay methods, Fluorescein-5-isothiocyanate pharmacology, G(M2) Ganglioside chemistry, Humans, Immunoglobulin M chemistry, Mice, Microscopy, Fluorescence methods, Peripheral Nervous System pathology, Peripheral Nervous System Diseases drug therapy, Chemistry, Pharmaceutical methods, Drug Design, Gangliosides chemistry

Abstract

Monolithic columns containing ganglioside GM2 and GM3 mimics were prepared for selective removal of serum anti-ganglioside antibodies from patients with acute and chronic immune-mediated neuropathies. ELISA results demonstrated that anti-GM2 IgM antibodies in human sera and a mouse monoclonal anti-GM2 antibody were specifically and selectively adsorbed by monolithic GM2 mimic columns and not by blank monolithic columns or monolithic GM3 mimic columns. In control studies, serum antibodies against the ganglioside GQ1b from another neuropathy patient were not depleted by monolithic GM2 mimic columns. Fluorescence microscopy with FITC-conjugated anti-human immunoglobulin antibodies showed that the immobilized ganglioside mimics were evenly distributed along the column. The columns were able to capture ∼95% of the anti-GM2 antibodies of patients after only 2 min of incubation. A monolithic column of 4.4 μL can deplete 28.2 μL of undiluted serum. These columns are potential diagnostic and therapeutic tools for neuropathies related to anti-ganglioside antibodies.

Published

2011

2. Bioaffinity chromatography on monolithic supports.

Author

Tetala KK and van Beek TA

Subjects

Aptamers, Peptide isolation & purification, Chromatography, Affinity instrumentation, Ligands, Proteins isolation & purification, Chromatography, Affinity methods

Abstract

Affinity chromatography on monolithic supports is a powerful analytical chemical platform because it allows for fast analyses, small sample volumes, strong enrichment of trace biomarkers and applications in microchips. In this review, the recent research using monolithic materials in the field of bioaffinity chromatography (including immunochromatography) is summarized and discussed. After giving an introduction into affinity chromatography, information on different biomolecules (antibodies, enzymes, lectins, aptamers) that can act as ligands in bioaffinity chromatography is presented. Subsequently, the history of monoliths, their advantages, preparation and formats (disks, capillaries and microchips) as well as ligand immobilization techniques are mentioned. Finally, analytical and preparative applications of bioaffinity chromatography on monoliths are presented. During the last four years 37 papers appeared. Protein A and G are still most often used as ligands for the enrichment of immunoglobulins. Antibodies and lectins remain popular for the analysis of mainly smaller molecules and saccharides, respectively. The highly porous cryogels modified with ligands are applied for the sorting of different cells or bacteria. New is the application of aptamers and phages as ligands on monoliths. Convective interaction media (epoxy CIM disks) are currently the most used format in monolithic bioaffinity chromatography.

Published

2010

3. A three-phase microfluidic chip for rapid sample clean-up of alkaloids from plant extracts.

Author

Tetala KK, Swarts JW, Chen B, Janssen AE, and van Beek TA

Subjects

Alkaloids chemistry, Chloroform chemistry, Models, Chemical, Nanotechnology, Solvents chemistry, Spectrometry, Mass, Electrospray Ionization, Strychnine analogs & derivatives, Strychnine chemistry, Strychnine isolation & purification, Time Factors, Alkaloids isolation & purification, Microfluidic Analytical Techniques methods, Plant Extracts chemistry

Abstract

A three-phase microchip was developed for the rapid and efficient small-scale purification of alkaloids from plant extracts. As part of the development of such a three-phase microchip, first a two-phase microchip with two channels (3.2 cm and 9.3 cm) was used to study the extraction efficiency of strychnine nitrate and strychnine at various flow rates. Strychnine was extracted from a basic aqueous phase to a chloroform phase (extraction) or strychnine was extracted from a chloroform phase into an acidic aqueous phase (back extraction). Subsequently, the "simultaneous extraction and back extraction" of strychnine was carried out in a three-phase microchip. The experimental extraction rate and yield were compared with model data. At a residence time of 25 sec, 79.5% of strychnine was extracted into the acidic aqueous phase using the three-phase microchip. In general, a good correlation was found between experimental results and model data for both two- and three-phase extractions. Finally, the three-phase microchip was employed in the purification of alkaloids (strychnine and brucine) from Strychnos seed extracts.

Published

2009

4. Single step synthesis of carbohydrate monolithic capillary columns for affinity chromatography of lectins.

Author

Tetala KK, Chen B, Visser GM, and van Beek TA

Subjects

Chemical Phenomena, Chemistry, Physical, Molecular Structure, Particle Size, Permeability, Reproducibility of Results, Sensitivity and Specificity, Time Factors, Chromatography, Affinity instrumentation, Chromatography, Affinity methods, Lectins analysis, Oligosaccharides chemical synthesis, Oligosaccharides chemistry

Abstract

Carbohydrate monolithic beds were synthesized in a single step in capillary columns to study affinity chromatography of lectins. In this method, carbohydrates (beta-galactose, beta-glucose, and alpha-mannose) with an easy to synthesize alkene terminated tetraethylene glycol spacer were used as functional monomers along the monomer 2-hydroxyethyl methacrylate (HEMA). As crosslinkers (+)-N,N'-diallyltartardiamide (DATD) and piperazine diacrylamide (PDA, 1,4-bisacryloyl-piperazine) were used. SEM showed the successful formation of monolithic beds in the capillary columns. The permeability of the columns was high. The specific interaction of the lectins Con A, Lens culinaris (LCA) and Arachis hypogaea (PNA) with the carbohydrate stationary phase was studied by frontal affinity chromatography (FAC). Con A and LCA were successfully eluted from the column using 0.1 M methyl-alpha-mannopyranoside and PNA with 0.1 M beta-galactose. Dissociation constants (Kd) for carbohydrate-lectin interactions were determined and compared with literature.

Published

2007

5. Preparation of a monolithic capillary column with immobilized alpha-mannose for affinity chromatography of lectins.

Author

Tetala KK, Chen B, Visser GM, Maruska A, Kornysova O, van Beek TA, and Sudhölter EJ

Subjects

Microscopy, Electron, Scanning, Microscopy, Fluorescence, Permeability, Polymers chemical synthesis, Polymers chemistry, Chromatography, Affinity methods, Lectins isolation & purification, Mannose chemistry

Abstract

A simple method for the preparation of an affinity monolithic (also called continuous bed) capillary column for alpha-mannose-specific lectins is described. 2-Hydroxyethyl methacrylate in combination with (+)-N,N -diallyltartardiamide (DATD) and piperazine diacrylamide (PDA, 1,4-bisacryloyl-piperazine) as crosslinkers, were used as monomers for the monolith. After oxidation of DATD with periodate, alpha-mannose with spacer was bound to the aldehyde groups of the polymeric skeleton via reductive amination to form an affinity column for the separation, enrichment or binding studies of mannose-specific lectins. The permeability of the column was excellent. The porosity of the monolith was investigated by scanning electron microscope (SEM) and inverse size exclusion chromatography (ISEC). The affinity of the monolith was evaluated by frontal analysis (FA) and fluorescence microscopy (FM) using fluorescently labeled concanavalin (Con A). Frontal affinity chromatography showed a specific interaction of two different lectins with the alpha-mannose-modified monolith. According to FM the affinity sites were evenly distributed over the monolithic bed.

Published

2007