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一种单克隆二硝基苯基特异性大鼠IgE的制备以及用于估计大鼠抗二硝基苯基-猪蛔虫IgE抗体浓度的IgE捕获ELISA的建立。

Production of a monoclonal dinitrophenyl-specific rat IgE and establishment of an IgE capture ELISA for estimating the concentration of rat IgE antibodies to dinitrophenyl-Ascaris suum.

作者信息

Hanashiro K, Nakamura M, Tamaki N, Kosugi T

机构信息

1st Department of Physiology, University of the Ryukyus, Okinawa, Japan.

出版信息

Int Arch Allergy Immunol. 1996 Aug;110(4):371-9. doi: 10.1159/000237330.

Abstract

A hybridoma producing monoclonal rat IgE antibodies of antidinitrophenyl (anti-DNP) specificity was generated by fusion of Sp2/0-Ag 14 (SP2) mouse myeloma cells and spleen cells from a DNP-Ascaris-sensitized Brown-Norway rat. Subsequently, the supernatant of the hybridoma (FE-3) was applied to an affinity column of DNP-bovine serum albumin-Sepharose 4B. The adsorbed protein fraction was pooled, concentrated, and further purified using Sephadex G-200. The molecular weight of the isolated protein was approximately 200,000 by SDS-PAGE, and the protein reacted with peroxidase (POD) mouse antirat myeloma IgE on Western blotting. Rabbit antibodies against DNP-specific rat IgE were also prepared by immunizing Japanese white rabbits with monoclonal DNP-specific rat IgE. These antibodies against DNP-specific rat IgE were applied to an affinity column of normal rat serum-Sepharose 4B and monoclonal DNP-specific rat IgG2b-Sepharose 4B to remove any other reactive substances apart from IgE contained in the serum proteins of the rat sensitized with DNP-Ascaris. On ELISA, it was found that the specificity of POD rabbit antibodies against DNP-specific rat IgE for monoclonal DNP-specific rat IgE was the same as that for rat myeloma IgE (IR 162). In addition, determinations of the monoclonal DNP-specific rat IgE revealed that the sensitivity of ELISA using POD-rabbit antibodies against DNP-specific rat IgE [POD-RA(DNP)RE] was higher than that using POD goat antibodies against rat myeloma IgE. Furthermore, an IgE capture ELISA employing the above-mentioned RA(DNP)RE was established for estimating the rat IgE antibodies to DNP-Ascaris suum. A good correlation was found between the antigen-specific IgE antibodies in the serum of Wistar rats estimated by this IgE capture ELISA and those estimated by passive cutaneous anaphylaxis.

摘要

通过将Sp2/0-Ag 14(SP2)小鼠骨髓瘤细胞与来自二硝基苯-蛔虫致敏的棕色挪威大鼠的脾细胞融合,产生了一种产生具有抗二硝基苯(抗DNP)特异性的单克隆大鼠IgE抗体的杂交瘤。随后,将杂交瘤(FE-3)的上清液应用于二硝基苯-牛血清白蛋白-琼脂糖4B亲和柱。收集吸附的蛋白质部分,浓缩,并使用葡聚糖G-200进一步纯化。通过SDS-PAGE测定,分离出的蛋白质的分子量约为200,000,并且该蛋白质在Western印迹中与过氧化物酶(POD)小鼠抗大鼠骨髓瘤IgE发生反应。还通过用单克隆DNP特异性大鼠IgE免疫日本白兔制备了针对DNP特异性大鼠IgE的兔抗体。将这些针对DNP特异性大鼠IgE的抗体应用于正常大鼠血清-琼脂糖4B和单克隆DNP特异性大鼠IgG2b-琼脂糖4B亲和柱,以去除用DNP-蛔虫致敏的大鼠血清蛋白中除IgE之外的任何其他反应性物质。在ELISA中,发现POD兔抗DNP特异性大鼠IgE对单克隆DNP特异性大鼠IgE的特异性与对大鼠骨髓瘤IgE的特异性相同(IR 162)。此外,对单克隆DNP特异性大鼠IgE的测定表明,使用POD兔抗DNP特异性大鼠IgE [POD-RA(DNP)RE]的ELISA的灵敏度高于使用POD山羊抗大鼠骨髓瘤IgE的ELISA的灵敏度。此外,建立了一种使用上述RA(DNP)RE的IgE捕获ELISA,用于估计大鼠针对猪蛔虫的IgE抗体。通过这种IgE捕获ELISA估计的Wistar大鼠血清中的抗原特异性IgE抗体与通过被动皮肤过敏反应估计的抗体之间发现了良好的相关性。

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