Carp (Cyprinus carpio) vitellogenin: characterization of yolk proteins, development of immunoassays and use as biomarker of exposure to environmental estrogens.

Akihiko Hara, Kaori Hirano, Munetaka Shimizu, Haruhisa Fukada, Toshiaki Fujita, Fuminari Ito, Hideshige Takada, Masaru Nakamura, Taisen Iguchi
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Abstract

The precursor protein of egg yolk, vitellogenin (Vg), is cleaved into three major components (lipovitellin, phosvitin and beta'-component) at the time of incorporation by growing oocytes. We purified three yolk proteins (YP1, YP2 and YP3) from ovaries of the common carp (Cyprinus carpio) by a combined method of ammonium sulfate precipitation and column chromatography. Biochemical analyses of the purified proteins of this species suggest that YP1, YP2 and YP3 are lipovitellin, beta'-component and phosvitin, respectively. A specific antiserum against purified carp YP1 (lipovitellin) was used to develop a single radial immunodiffusion (SRID) technique and an enzyme-linked immunosorbent assay (ELISA) for carp Vg. By SRID and ELISA, we measured the circulating carp Vg level to be in the ranges of 12.5-400 microg/ml and 2.0-1000 ng/ml, respectively, which cover a wide range of Vg levels. From 1997-1998, male and female carp were captured at points of effluent discharge from a sewage treatment plant connected to the Tama River, where estrogenic compounds were later detected, and the presence of Vg in their circulation was examined. Vg was detected in both male and female carp at the mg/ml level, suggesting that estrogens such as estrone and estradiol were sufficiently high to induce Vg in male carp inhabiting this area. The result of this study supports the use of carp Vg as a biomarker of fish exposure to environmental estrogens.

鲤鱼卵黄原蛋白:卵黄蛋白的特性、免疫测定的发展和作为环境雌激素暴露的生物标志物的应用。
卵黄原蛋白(vitellogenin, Vg)是卵黄的前体蛋白,卵黄原蛋白(vitelgenin, Vg)在卵黄原蛋白与卵黄原蛋白结合时被卵黄原蛋白(lipovitellin)、卵黄原蛋白(phosvittin)和β -成分(beta -component)三种主要成分。采用硫酸铵沉淀和柱层析相结合的方法,从鲤鱼子房中分离纯化了3种卵黄蛋白(YP1、YP2和YP3)。纯化后的蛋白经生化分析表明,YP1、YP2和YP3分别为脂维磷脂(lipovitellin)、β′组分(beta′-component)和磷维磷脂(phosvitin)。采用纯化的鲤鱼脂卵磷脂(YP1)特异性抗血清,建立了单径向免疫扩散(SRID)技术和酶联免疫吸附试验(ELISA)。通过SRID和ELISA检测,我们测得循环鲤鱼的Vg水平分别在12.5 ~ 400 μ g/ml和2.0 ~ 1000 μ g/ml之间,覆盖了较宽的Vg水平范围。从1997年到1998年,在与多摩河相连的污水处理厂的排放点捕获了雄性和雌性鲤鱼,后来在那里检测到雌激素化合物,并检查了它们循环中Vg的存在。在雄性和雌性鲤鱼中均检测到Vg,含量均为mg/ml,表明雌酮和雌二醇等雌激素足以在该地区的雄性鲤鱼中诱发Vg。本研究结果支持使用鲤鱼Vg作为鱼类暴露于环境雌激素的生物标志物。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
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