Issue 12, 2005

Microplate-based screening methods for the efficient development of sandwich immunoassays

Abstract

The selection of suitable antibodies is a critical step in immunoassay development, since the final assay performance is predetermined by this decision to a large extent. Particularly, the screening for matching pairs in sandwich immunoassays is difficult, if both antibodies are derived from one species or when monoclonal antibodies are only available as cell supernatants. Several microplate-based approaches for in situ labeling of detection antibodies were tested, in order to avoid time consuming purification of antibodies for enzyme conjugate synthesis. We investigated labeling with anti-species antibodies and Fab fragments thereof, labeling with protein G and biotinylation of cell supernatants without prior purification. Antibodies against peanut proteins were used as a model and signal-to-blank ratios were used in all cases as a measure of the antibody pair performance. Amongst the investigated approaches, preincubation of the detection antibody with labeled anti-species antibody turned out to be most suitable under our conditions. Diagrams, showing the performance of all possible antibody combinations, were generated with this method and were compared to results obtained with covalently labeled detection antibodies. Finally, a flowchart is presented, suggesting an efficient strategy for the development of highly sensitive sandwich immunoassays.

Graphical abstract: Microplate-based screening methods for the efficient development of sandwich immunoassays

Supplementary files

Article information

Article type
Paper
Submitted
02 Jun 2005
Accepted
23 Sep 2005
First published
12 Oct 2005

Analyst, 2005,130, 1580-1588

Microplate-based screening methods for the efficient development of sandwich immunoassays

M. Kiening, R. Niessner and M. G. Weller, Analyst, 2005, 130, 1580 DOI: 10.1039/B507794J

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