Preparation of Monoclonal Antibodies Specifically Reacting with the Trichothecene Mycotoxins Nivalenol and 15-Acetylnivalenol via the Introduction of a Linker Molecule into Its C-15 Position

Author:

Noda Kyoko,Hirakawa Yuki,Nishino Tomomi,Sekizuka Ritsuto,Kishimoto Marin,Furukawa TomohiroORCID,Sawane Sakiko,Matsunaga Ayu,Kobayashi Naoki,Sugita Kazutoshi,Oonaka Kenji,Kawakami Hiroko,Otsuka Yuji,Yamamoto Tetsuya,Yamamoto Toshihiro,Yoshiya TakuORCID,Watanabe Maiko,Saka Machiko,Momma Keiko,Kushiro MasayoORCID,Miyake Shiro

Abstract

Nivalenol (NIV) is a trichothecene mycotoxin that is more toxic than deoxynivalenol. It accumulates in grains due to infection with Fusarium species, which are the causative agents of scab or Fusarium head blight. An immunoassay, which is a rapid and easy analytical method, is necessary for monitoring NIV in grains. However, a specific antibody against NIV has not been prepared previously. To establish an immunoassay, we prepared NIV, introduced a linker, and generated antibodies against it. NIV was prepared from a culture of Fusarium kyushuense obtained from pressed barley through chromatographic procedures with synthetic adsorbents and silica gel. NIV was reacted with glutaric anhydride, and the reaction was stopped before mono-hemiglutaryl-NIV was changed to di-hemiglutaryl-NIV. 15-O-Hemiglutaryl-NIV was isolated via preparative HPLC and bound to keyhole limpet hemocyanin (KLH) using the active ester method. Two different monoclonal antibodies were prepared by immunizing mice with the NIV-KLH conjugate. The 50% inhibitory concentration values were 36 and 37 ng/mL. These antibodies also showed high reactivity in a direct competitive enzyme-linked immunosorbent assay and specifically reacted with NIV and 15-acetyl-NIV but not with deoxynivalenol and 4-acetyl-NIV.

Funder

the Ministry of Agriculture, Forestry and Fisheries of Japan

Publisher

MDPI AG

Subject

Health, Toxicology and Mutagenesis,Toxicology

Reference37 articles.

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