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以霍乱毒素作为载体佐剂产生与伏马菌素B1、B2和B3反应的抗体。

Generation of antibodies reactive with fumonisins B1, B2, and B3 by using cholera toxin as the carrier-adjuvant.

作者信息

Azcona-Olivera J I, Abouzied M M, Plattner R D, Norred W P, Pestka J J

机构信息

Department of Food Science and Human Nutrition, Michigan State University, East Lansing 48824-1224.

出版信息

Appl Environ Microbiol. 1992 Jan;58(1):169-73. doi: 10.1128/aem.58.1.169-173.1992.

Abstract

Murine polyclonal antibodies reactive with fumonisins B1, B2, and B3 were produced after a novel immunization procedure with cholera toxin as both a hapten carrier protein and adjuvant. Immunization of mice with two 7.5-micrograms doses of fumonisin B1-cholera toxin conjugate without adjuvant resulted in the production of fumonisin B1-specific antibodies in all mice within 15 days when intraperitoneal, subcutaneous, and intravenous routes were used. In contrast, conventional immunization procedures with fumonisin B1-bovine serum albumin conjugates with and without Freund's adjuvant were largely ineffective. Fumonisin antibodies could be readily mass-produced in ascites fluid by using cholera toxin as a carrier-adjuvant. A competitive indirect enzyme-linked immunosorbent assay (ELISA) was devised whereby immobilized fumonisin B1-ovalbumin and free fumonisin B1 competed for antibody binding. The detection limit for fumonisin B1 in the ELISA was 100 ng/ml. The antiserum cross-reacted with fumonisins B2 and B3 but not with the hydrolyzed backbone of fumonisin B1 and tricarballylic acid. Concentrations of fumonisins B1, B2, and B3 required for 50% binding inhibition were 260, 300, and 650 ng/ml, respectively. These polyclonal antibodies should find wide usage in the ELISA for fumonisins in foods, feeds, and tissues.

摘要

通过一种以霍乱毒素作为半抗原载体蛋白和佐剂的新型免疫程序,制备了与伏马菌素B1、B2和B3发生反应的小鼠多克隆抗体。用两剂7.5微克无佐剂的伏马菌素B1 - 霍乱毒素偶联物对小鼠进行免疫,当采用腹腔内、皮下和静脉途径时,所有小鼠在15天内产生了伏马菌素B1特异性抗体。相比之下,使用和不使用弗氏佐剂的伏马菌素B1 - 牛血清白蛋白偶联物的传统免疫程序大多无效。通过使用霍乱毒素作为载体 - 佐剂,可以在腹水中轻松大量生产伏马菌素抗体。设计了一种竞争性间接酶联免疫吸附测定(ELISA),其中固定化的伏马菌素B1 - 卵清蛋白和游离伏马菌素B1竞争抗体结合。ELISA中伏马菌素B1的检测限为100纳克/毫升。抗血清与伏马菌素B2和B3发生交叉反应,但与伏马菌素B1的水解主链和三羧酸不发生交叉反应。50%结合抑制所需的伏马菌素B1、B2和B3浓度分别为260、300和650纳克/毫升。这些多克隆抗体在食品、饲料和组织中伏马菌素的ELISA检测中应具有广泛用途。

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