Issue 4, 2003

Solid-phase immunoassay detection of peptides from complex matrices without a separation

Abstract

A simple and sensitive solid-phase fluorescence immunoassay method was developed to detect peptides without separating them from a biological matrix. A near infrared fluorescence detection system was constructed for scanning analyte spots blotted onto protein binding membranes. Hydrophobic membranes were used with a modified vacuum spot blotting system to concentrate the peptide solution into a small area and the overall assay time was thus reduced by eliminating blocking steps. Both direct and indirect immunoassay methods are demonstrated; the indirect is more sensitive and features a 1 pmol detection limit of neat dynorphin A solutions. To further increase the immunoassay sensitivity, a novel capillary blotting system with hydrophilic membranes was designed where optimized sample volumes of 167 nL were deposited for each spot. The area-reduced blotting method shows a 1000-fold improved, 1.3 fmol spot−1 detection limit of a dynorphin A diluted in a buffered solution of 150 mg L−1 of casein. Low-flow push-pull perfusates with volumes of 1 µL sampled from the striatum of the rat were assayed for dynorphin A by the method of standard addition. The detection limit was estimated to be 1.9 fmol in the low-flow push-pull perfusates. These data demonstrate a solid-phase near infrared immunofluorescence strategy for the study of peptides directly blotted from chemically complex biological fluid matrices.

Article information

Article type
Paper
Submitted
01 Nov 2002
Accepted
07 Mar 2003
First published
19 Mar 2003

Analyst, 2003,128, 357-362

Solid-phase immunoassay detection of peptides from complex matrices without a separation

X. Zhao, S. Kottegoda and S. A. Shippy, Analyst, 2003, 128, 357 DOI: 10.1039/B210782A

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