Abstract
A protein stationary phase for frontal affinity chromatography was prepared, containing biotinylated β-galactosidase immobilized to controlled pore glass beads via covalently bonded streptavidin. Single microaffinity columns of approximately 30 pmol of active β-galactosidase were prepared from this material and characterized with a known ligand by frontal analysis. These columns were used to measure the specific interactions between the bound β-galactosidase and a library of modified β-galactopyranosides using electrospray mass spectrometry as the means of detection. The library contained 89 entries, each representing 4 diastereomers for a total of 356 library members. A single entry was analysed revealing differential activity among the 4 isomers. The library was grouped into 10 mixtures of 24-40 members each with each mixture infused under frontal chromatographic conditions. This deconvolution procedure led to the identification of 34 entries containing isomers with Kd values better than 10 μM. A method based on a displacement principle was implemented as a rapid prescreen which served as the basis for a parallel column high throughput screening assay.
Keywords: frontal affinity chromatography
Combinatorial Chemistry & High Throughput Screening
Title: Frontal Affinity Chromatography for the Screening of Mixtures
Volume: 5 Issue: 5
Author(s): N. W.C. Chan, D. F. Lewis, S. Hewko, O. Hindsgaul and D. C. Schriemer
Affiliation:
Keywords: frontal affinity chromatography
Abstract: A protein stationary phase for frontal affinity chromatography was prepared, containing biotinylated β-galactosidase immobilized to controlled pore glass beads via covalently bonded streptavidin. Single microaffinity columns of approximately 30 pmol of active β-galactosidase were prepared from this material and characterized with a known ligand by frontal analysis. These columns were used to measure the specific interactions between the bound β-galactosidase and a library of modified β-galactopyranosides using electrospray mass spectrometry as the means of detection. The library contained 89 entries, each representing 4 diastereomers for a total of 356 library members. A single entry was analysed revealing differential activity among the 4 isomers. The library was grouped into 10 mixtures of 24-40 members each with each mixture infused under frontal chromatographic conditions. This deconvolution procedure led to the identification of 34 entries containing isomers with Kd values better than 10 μM. A method based on a displacement principle was implemented as a rapid prescreen which served as the basis for a parallel column high throughput screening assay.
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Cite this article as:
Chan W.C. N., Lewis F. D., Hewko S., Hindsgaul O. and Schriemer C. D., Frontal Affinity Chromatography for the Screening of Mixtures, Combinatorial Chemistry & High Throughput Screening 2002; 5 (5) . https://dx.doi.org/10.2174/1386207023330192
DOI https://dx.doi.org/10.2174/1386207023330192 |
Print ISSN 1386-2073 |
Publisher Name Bentham Science Publisher |
Online ISSN 1875-5402 |
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