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针对EYRKK水泡性口炎病毒相关肽的抗体仅占抗Ro60kD抗体的少数。

Antibodies to EYRKK vesicular stomatitis virus-related peptide account only for a minority of anti-Ro60kD antibodies.

作者信息

Routsias J G, Sakarellos-Daitsiotis M, Detsikas E, Tzioufas A G, Sakarellos C, Moutsopoulos H M

机构信息

Department of Internal Medicine, School of Medicine, University of Ioannina, Greece.

出版信息

Clin Exp Immunol. 1994 Dec;98(3):414-8. doi: 10.1111/j.1365-2249.1994.tb05506.x.

Abstract

Previous studies demonstrated a possible antigenic relation between the carboxyl terminal portion of anti-Ro60kD autoantigen and a nucleocapsid protein (N) of vesicular stomatitis virus (VSV). In order to investigate whether anti-Ro60kD autoantibodies react with the VSV homologous region of the Ro60kD protein we synthesized, according to Merrifield's method, the EYRKKMDI octapeptide (8p) sharing a common sequence with the N protein of VSV. Sera from 61 patients with autoimmune rheumatic diseases (34 systemic lupus erythematosus (SLE), 21 Sjörgren's syndrome (SS) and six rheumatoid arthritis (RA)) as well as 59 from normal blood donors were tested for the presence of anti-Ro60kD autoantibodies by ELISA and immunoblot (IB) and anti-8p antibodies by ELISA. Antibodies to 8p were found in 9/31 of anti-Ro60kD IB-positive sera, 5/30 of anti-Ro60kD-negative sera and 2/59 of normal control sera. The concordance between the anti-8p ELISA and the anti-Ro60kD IB was very poor (chi 2 = 0.71, P = 0.4) in contrast to the anti-Ro60kD ELISA and the anti-Ro IB (chi 2 = 27.6, P = 10(-7)). Subsequent affinity purification of the anti-8p antibodies from a strong positive anti-8p and anti-Ro60kD SLE serum yielded 95% depletion of the anti-8p activity and 37% reduction of the anti-Ro60kD activity. Inhibition assays with the affinity-purified anti-8p antibodies demonstrated that the octapeptide gave 94.5% inhibition of the anti-Ro60kD activity, while Ro60kD protein led to 42.3% inhibition of the anti-8p. Preincubation of the serum with the octapeptide produced 4% inhibition of anti-Ro60kD ELISA. These results indicate that the anti-8p antibodies account only for a minority of the anti-Ro60kD autoantibodies.

摘要

先前的研究表明,抗Ro60kD自身抗原的羧基末端部分与水疱性口炎病毒(VSV)的核衣壳蛋白(N)之间可能存在抗原关系。为了研究抗Ro60kD自身抗体是否与我们根据梅里菲尔德方法合成的Ro60kD蛋白的VSV同源区域发生反应,合成了与VSV的N蛋白具有共同序列的EYRKKMDI八肽(8p)。通过酶联免疫吸附测定(ELISA)和免疫印迹(IB)检测了61例自身免疫性风湿病患者(34例系统性红斑狼疮(SLE)、21例干燥综合征(SS)和6例类风湿关节炎(RA))以及59名正常献血者的血清中抗Ro60kD自身抗体的存在情况,并通过ELISA检测了抗8p抗体。在抗Ro60kD IB阳性血清的31份中有9份、抗Ro60kD阴性血清的30份中有5份以及正常对照血清的59份中有2份检测到抗8p抗体。与抗Ro60kD ELISA和抗Ro IB相比(卡方值=27.6,P=10⁻⁷),抗8p ELISA与抗Ro60kD IB之间的一致性非常差(卡方值=0.71,P=0.4)。随后,从一份强阳性抗8p和抗Ro60kD的SLE血清中对抗8p抗体进行亲和纯化,结果显示抗8p活性降低了95%,抗Ro60kD活性降低了37%。用亲和纯化的抗8p抗体进行的抑制试验表明,八肽对抗Ro60kD活性的抑制率为94.5%,而Ro60kD蛋白对抗8p的抑制率为42.3%。血清与八肽预孵育后,抗Ro60kD ELISA的抑制率为4%。这些结果表明,抗8p抗体仅占抗Ro60kD自身抗体的一小部分。

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