Gordon T P, Jovanovich S A, Sykes P, Bradley J, Roberts-Thomson P J
Department of Clinical Immunology, Flinders Medical Centre, Bedford Park, South Australia.
Rheumatol Int. 1990;10(3):99-102. doi: 10.1007/BF02274822.
Antibodies to ribosomal P proteins are markers for systemic lupus erythematosus (SLE) but are often missed by assays utilizing routine immunofluorescence or immunoprecipitation. Expression of autoantigenic sites encoded by complementary DNA (cDNA) clones offers an inexpensive source of antigen for use in quantitative immunoassays. Using a monospecific ribosomal P positive serum to screen a human placental lambda gt11 expression library, a cDNA clone was isolated which reacted with all anti-P human sera tested. Autoantibodies which were affinity purified from the expressed cDNA reacted with the 38 kDa ribosomal Po protein and reactivity was blocked by absorption with recombinant fusion protein. A stable beta-galactosidase fusion protein of 150 kDa was partially purified by a simple differential centrifugation method and used in an enzyme-linked immunoabsorbent assay to reliably quantitate anti-P responses, with a sensitivity and specificity equal to Western blotting. A survey of 84 normals and 151 patients with autoimmune diseases confirmed the high specificity of anti-P antibodies for SLE. The availability of cloned autoantigen will facilitate more detailed clinico-serologic correlations for anti-P antibodies.
核糖体P蛋白抗体是系统性红斑狼疮(SLE)的标志物,但利用常规免疫荧光或免疫沉淀的检测方法常常会漏检。互补DNA(cDNA)克隆编码的自身抗原位点的表达为定量免疫测定提供了一种廉价的抗原来源。用单特异性核糖体P阳性血清筛选人胎盘λgt11表达文库,分离出一个与所有检测的抗P人血清发生反应的cDNA克隆。从表达的cDNA中亲和纯化的自身抗体与38 kDa核糖体Po蛋白发生反应,并且反应性被重组融合蛋白吸收所阻断。通过简单的差速离心法部分纯化了一种稳定的150 kDaβ-半乳糖苷酶融合蛋白,并将其用于酶联免疫吸附测定,以可靠地定量抗P反应,其灵敏度和特异性与蛋白质印迹法相当。对84名正常人和151名自身免疫性疾病患者的调查证实了抗P抗体对SLE具有高度特异性。克隆的自身抗原的可得性将有助于对抗P抗体进行更详细的临床-血清学相关性研究。
