Issue 1, 2012

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

Abstract

The aim of the present study was to produce monoclonal anti-fullerene C60 antibodies and to develop the enzyme immunoassay for the detection in the first use of free fullerene C60 both in solutions and in multicomponent biological probes. The immunization of mice with the conjugate of fullerene C60 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 C60 a specially selected water–organic mixture compatible with immunoassay was proposed. The detection limit of free fullerene C60 in solution was 2 μg L−1. Fullerene C60 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 C60 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 C60 in different tissues.

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

Supplementary files

Article information

Article type
Paper
Submitted
17 Aug 2011
Accepted
26 Sep 2011
First published
03 Nov 2011

Analyst, 2012,137, 98-105

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

O. Hendrickson, N. Fedyunina, A. Zherdev, O. Solopova, P. Sveshnikov and B. Dzantiev, Analyst, 2012, 137, 98 DOI: 10.1039/C1AN15745K

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