Immunochromatographic assay for simple and rapid detection of Satsuma dwarf virus and related viruses using monoclonal antibodies

Nario Kusano; Keita Hirashima; Minoru Kuwahara; Kenji Narahara; Tadashi Imamura; Tomohiro Mimori; Ken Nakahira; Kuniaki Torii

doi:10.1007/s10327-006-0316-6

Immunochromatographic assay for simple and rapid detection of Satsuma dwarf virus and related viruses using monoclonal antibodies

J Gen Plant Pathol. 2007;73(1):66-71. doi: 10.1007/s10327-006-0316-6. Epub 2007 Feb 16.

Authors

Nario Kusano¹, Keita Hirashima¹, Minoru Kuwahara¹, Kenji Narahara², Tadashi Imamura², Tomohiro Mimori², Ken Nakahira², Kuniaki Torii²

Affiliations

¹ Fukuoka Agricultural Research Center, 587 Yoshiki, Chikushino, Fukuoka, 818-8549 Japan.
² Mizuho Medy Co., Ltd., Tosu, Japan.

Abstract

A simple and rapid immunochromatographic assay (ICA) to detect Satsuma dwarf virus (SDV) was developed using colloidal gold conjugates of anti-SDV monoclonal antibodies. Of six homogenization buffers tested, 0.1 M citrate buffer (pH 7.0) gave the best results for the ICA. In the ICA, addition of 0.1% thioglycolic acid in the homogenization buffers that have been widely used in enzyme-linked immunosorbent assays (ELISA) was deleterious to the reaction because of undesirable coagulation of the colloidal gold. ICA using the anti-SDV monoclonal antibodies was 8 times and 16 times more sensitive than double antibody sandwich-ELISA and ICA using the anti-SDV polyclonal antibody, respectively. The analysis is complete in only 15 min. Furthermore, ICA using the anti-SDV monoclonal antibodies could also detect SDV-related viruses.

Keywords: Detection; ELISA; Immunochromatographic assay; Satsuma dwarf virus.