Production and characterization of a monoclonal antibody specific for ubiquitin-like polypeptide responsible for nonspecific immune suppression.

Journal of immunoassay Pub Date : 1998-02-01 DOI:10.1080/01971529808005471

Y Nariai, M Nakamura, T Kondoh, Y Tanigawa

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引用次数: 1

Abstract

Monoclonal nonspecific suppressor factor (MNSF) is a lymphokine product of a murine T cell hybridoma that inhibits the immune response in an antigen nonspecific manner. Recently, we found that a novel ubiquitin-like protein (Ubi-L), a subunit of MNSF, is responsible for its biological activity. We developed a monoclonal antibody with specific activity against Ubi-L. Inhibition experiments showed that this mAb, termed NA4, preferentially recognizes Ubi-L but not irrelevant proteins such as ubiquitin. With the use of NA4, we established an ELISA method for the quantitation of Ubi-L. By this ELISA system, approximately 40 ng/ml of MNSF was detected in the culture supernatants of concanavalin A (Con A)- or interferon gamma (IFN gamma)-activated splenocytes, whereas MNSF in the supernatant of IFN alpha- and IFN beta-stimulated splenocytes was nil. In addition, NA4 could abrogate the action of Ubi-L. Thus NA4 was confirmed to be a pertinent tool for elucidation of the underlying mechanism of action of MNSF.

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非特异性免疫抑制泛素样多肽特异性单克隆抗体的制备和鉴定。

单克隆非特异性抑制因子(MNSF)是小鼠T细胞杂交瘤的淋巴因子产物，以抗原非特异性的方式抑制免疫反应。最近，我们发现了一种新的泛素样蛋白(Ubi-L)，它是MNSF的一个亚基，负责其生物活性。我们制备了一种具有特异活性的Ubi-L单克隆抗体。抑制实验表明，这种mAb，称为NA4，优先识别Ubi-L，而不是不相关的蛋白质，如泛素。利用NA4建立了ELISA法定量Ubi-L的方法。通过该ELISA系统，在番豆蛋白A (Con A)或干扰素γ (IFN γ)激活的脾细胞培养上清中检测到约40 ng/ml的MNSF，而在IFN α和IFN β刺激的脾细胞上清中检测到的MNSF为零。NA4能使Ubi-L丧失作用。因此，NA4被证实是阐明MNSF潜在作用机制的一个相关工具。

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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Journal of immunoassay

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