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首页> 外文期刊>Chemical research in toxicology >Generation of antibodies to Di- and trichloroacetylated proteins and immunochemical detection of protein adducts in rats treated with perchloroethene.
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Generation of antibodies to Di- and trichloroacetylated proteins and immunochemical detection of protein adducts in rats treated with perchloroethene.

机译:用全氯乙烯处理的大鼠中二氯和三氯乙酰化蛋白质的抗体的产生以及蛋白质加合物的免疫化学检测。

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摘要

Antibodies directed against chemical specific protein modifications are valuable tools to detect and comparatively quantify protein modifications. Both Nepsilon-(dichloroacetyl)-L-lysine and Nepsilon-(trichloroacety)l-L-lysine have been detected as modified amino acids in liver and kidneys of rats treated with perchloroethene (PER) after proteolysis. These protein modifications are formed by the interaction of reactive metabolites formed from PER with proteins. In this study we developed monospecific antibodies to dichloroacetylated and to trichloroacetylated amino acids to detect modified proteins in the target organs of PER toxicity. These antibodies were prepared by immunization of rabbits with modified keyhole limpet hemocyanin (KLH) coupled with either the dichloroacetyl or trichloroacetyl moiety. Enzyme-linked immunosorbent assays (ELISA) indicated that the polyclonal rabbit sera recognized dichloroacetylated or trichloroacetylated rabbit serum albumin (RSA), but not unmodified protein. Therefore, we further purified rabbit antisera on either Nepsilon-(dichloroacetyl)-L-lysine or Nepsilon-(trichloroacetyl)-L-lysine immobilized to immunoaffinity columns to obtain monospecific antibodies. The potential of these antibodies in the detection of di- and trichloroacetylated proteins and their selectivity for the desired dichloroacetyl or trichloroacetyl group was demonstrated in competitive enzme-linked immunosorbent assays with several structurally related compounds. Anti-dichloroacetyl (anti-DCA) antibody binding to dichloroacetylated RSA was inhibited by Nepsilon-(dichloroacetyl)-L-lysine with an IC50 value of 150 microM whereas inhibition by Nepsilon-(monochloroacetyl)-L-lysine and Nepsilon-(trichloroacetyl)-L-lysine showed an IC50 value of 100 mM. The binding of the anti-trichloroacetyl (anti-TCA) antibody to trichloroacetylated RSA was inhibited by Nepsilon-(dichloroacetyl)-L-lysine with an IC50 value of 80 mM. The inhibition by Nepsilon-(trichloroacetyl)-L-lysine was again 3 orders of magnitude stronger resulting in an IC50 value of 90 microM. Nepsilon-(acetyl)-L-lysine and unmodified RSA did not effect antibody binding to the chemically modified antigen. The antibodies were also successfully applied to detect modified proteins in subcellular fractions of liver and kidney from PER treated rats demonstrated in immunoblot. Protein adduct formation from different PER metabolism pathways was confirmed by the observation that the majority of dichloroacetylated proteins were located in kidney mitochondria and trichloroacetylated proteins were located in liver microsomes.
机译:针对化学特异蛋白质修饰的抗体是检测和比较定量蛋白质修饰的有价值的工具。蛋白水解后,在全氯乙烯(PER)处理的大鼠的肝脏和肾脏中,均已检测到Nepsilon-(二氯乙酰基)-L-赖氨酸和Nepsilon-(三氯乙酰基)1-L-赖氨酸为修饰氨基酸。这些蛋白质修饰是由PER形成的反应性代谢产物与蛋白质相互作用形成的。在这项研究中,我们开发了针对二氯乙酰化和三氯乙酰化氨基酸的单特异性抗体,以检测PER毒性靶器官中的修饰蛋白。这些抗体是通过用改良的锁孔in血蓝蛋白(KLH)结合二氯乙酰基或三氯乙酰基部分免疫兔来制备的。酶联免疫吸附试验(ELISA)表明,多克隆兔血清可识别二氯乙酰化或三氯乙酰化的兔血清白蛋白(RSA),但不能识别未修饰的蛋白。因此,我们在固定于免疫亲和柱的Nepsilon-(二氯乙酰基)-L-赖氨酸或Nepsilon-(三氯乙酰基)-L-赖氨酸上进一步纯化了兔抗血清,以获得单特异性抗体。这些抗体在检测二氯和三氯乙酰化蛋白中的潜力及其对所需二氯乙酰基或三氯乙酰基的选择性,已在竞争性酶联免疫吸附法中与几种结构相关的化合物进行了验证。 Nepsilon-(二氯乙酰基)-L-赖氨酸抑制结合二氯乙酰化RSA的抗二氯乙酰基(anti-DCA)抗体,IC50值为150 microM,而Nepsilon-(一氯乙酰基)-L-赖氨酸和Nepsilon-(三氯乙酰基)抑制-L-赖氨酸的IC50值为100 mM。 Nepsilon-(二氯乙酰基)-L-赖氨酸可抑制抗三氯乙酰基(anti-TCA)抗体与三氯乙酰化RSA的结合,IC50值为80 mM。 Nepsilon-(三氯乙酰基)-L-赖氨酸的抑制作用再强3个数量级,导致IC50值为90 microM。 Nepsilon-(乙酰基)-L-赖氨酸和未修饰的RSA不会影响抗体与化学修饰抗原的结合。该抗体还成功地用于检测免疫印迹中显示的PER治疗大鼠的肝和肾亚细胞部分的修饰蛋白。通过观察发现,大多数二氯乙酰化蛋白位于肾脏线粒体中,三氯乙酰化蛋白位于肝脏微粒体中,从而证实了来自不同PER代谢途径的蛋白质加合物形成。

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