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与鼠单克隆抗体识别的表位相比,SS - B/La的人自身抗体反应性表位高度保守。

Human autoantibody-reactive epitopes of SS-B/La are highly conserved in comparison with epitopes recognized by murine monoclonal antibodies.

作者信息

Chan E K, Tan E M

机构信息

W.M. Keck Autoimmune Disease Center, Scripps Clinic and Research Foundation, La Jolla, California 92037.

出版信息

J Exp Med. 1987 Dec 1;166(6):1627-40. doi: 10.1084/jem.166.6.1627.

Abstract

SS-B/La, an ubiquitous nuclear protein of 46-48 kD, is a target antigen of autoantibodies in SLE and Sjogren's syndrome and is involved in the maturation of RNA polymerase III transcripts such as 5S RNA and tRNAs. We have previously shown (14, 15) that SS-B consists of two protease-resistant domains of 23 and 28 kD, with the latter containing the RNA binding site. The epitopes of SS-B/La reactive with human autoantibodies are conserved among several mammalian species examined. BALB/c mice immunized with affinity-purified calf thymus SS-B produce IgG anti-SS-B/La antibodies, which reacted with bovine, human, and rabbit SS-B but not with mouse SS-B/La. The spleen of a mouse with the highest antibody titer was selected for fusion with P3 myeloma. Five IgG1k mAbs (A1-5) were selected by ELISA and immunoblotting. All except A3 reacted with the 28-kD domain. A1, A2, and A3 were capable of immuno-precipitating the 48-kD SS-B protein and its associated RNAs. A1, A2, and A3 also gave fine nuclear speckled staining on human, monkey, bovine, and rabbit cells that was similar in appearance to that with human autoantibodies, but in contrast to staining with human autoantibodies, they did not stain cells from rat, mouse, or rat kangaroo. It appears that human autoantibodies target highly conserved epitopes that can be distinguished from epitopes recognized by immunization-induced murine mAbs. Taken together with other data, it appears that human autoantibodies may be recognizing epitopes that are active or catalytic sites of molecules subserving important cellular functions.

摘要

SS - B/La是一种普遍存在的46 - 48 kD核蛋白,是系统性红斑狼疮(SLE)和干燥综合征自身抗体的靶抗原,参与RNA聚合酶III转录本(如5S RNA和tRNA)的成熟过程。我们之前已经表明(14, 15),SS - B由两个抗蛋白酶结构域组成,分别为23 kD和28 kD,后者含有RNA结合位点。与人类自身抗体反应的SS - B/La表位在几种被检测的哺乳动物物种中是保守的。用亲和纯化的小牛胸腺SS - B免疫BALB/c小鼠可产生IgG抗SS - B/La抗体,该抗体可与牛、人及兔的SS - B反应,但不与小鼠的SS - B/La反应。选择抗体滴度最高的小鼠脾脏与P3骨髓瘤细胞进行融合。通过酶联免疫吸附测定(ELISA)和免疫印迹法筛选出5种IgG1k单克隆抗体(A1 - 5)。除A3外,所有抗体均与28 kD结构域反应。A1、A2和A3能够免疫沉淀48 kD的SS - B蛋白及其相关RNA。A1、A2和A3在人、猴、牛和兔细胞上也呈现出精细的核斑点染色,其外观与人类自身抗体染色相似,但与人类自身抗体染色不同的是,它们不染色大鼠、小鼠或大鼠袋鼠的细胞。似乎人类自身抗体靶向的是高度保守的表位,这些表位可与免疫诱导的鼠单克隆抗体识别的表位相区分。结合其他数据来看,似乎人类自身抗体可能识别的是作为重要细胞功能分子的活性或催化位点的表位。

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J Autoimmun. 1989 Aug;2(4):321-7. doi: 10.1016/0896-8411(89)90159-5.

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