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U1 RNA茎环II上自身免疫表位的体外RNA筛选。

In vitro RNA selection of an autoimmune epitope on stem-loop II of U1 RNA.

作者信息

St Clair E W, Burch J A

机构信息

Department of Medicine, Division of Rheumatology, Allergy, and Clinical Immunology, Duke University Medical Center, Durham, North Carolina 27710., USA.

出版信息

Clin Immunol Immunopathol. 1996 Apr;79(1):60-70. doi: 10.1006/clin.1996.0051.

Abstract

Autoantibodies to U1 RNA occur frequently in sera from patients with SLE and SLE-overlap syndromes. These autoantibodies have been previously shown to recognize major epitopes on stem-loops II and IV of U1 RNA. To further define these recognition sites, in vitro RNA selection was performed to identify the individual nucleotides which form the antibody binding site. Serum autoantibodies were used in this procedure to select synthetic variants from a library of RNA oligomers with a central region of 25 degenerate nucleotides in a linear context. A consensus sequence was derived from the autoantibody-selected RNA ligands that corresponded to a region of stem-loop II. It contained six continuous nucleotides (U63-C64-C65,-A66-X-U68) and one presumed discontinuous nucleotide (U79). In vitro selection of RNA ligands from simpler sublibraries consisting of oligomers with random loops and fixed U1 stem II sequences yielded no consensus sequence, suggesting that autoimmune recognition occurs independent of loop nucleotides. Competition assays confirmed the specificity of these binding reactions. The structural nature of this autoimmune U1 RNA epitope is compatible with a model of autoantibody production based on stimulation by native small nuclear ribonucleoprotein particles.

摘要

针对U1 RNA的自身抗体常见于系统性红斑狼疮(SLE)患者和SLE重叠综合征患者的血清中。这些自身抗体先前已被证明可识别U1 RNA茎环II和IV上的主要表位。为了进一步确定这些识别位点,进行了体外RNA筛选,以鉴定构成抗体结合位点的单个核苷酸。在此过程中,使用血清自身抗体从具有25个简并核苷酸中心区域的线性RNA寡聚体文库中筛选合成变体。从自身抗体选择的RNA配体中获得了一个与茎环II区域相对应的共有序列。它包含六个连续核苷酸(U63 - C64 - C65 - A66 - X - U68)和一个推测的不连续核苷酸(U79)。从由具有随机环和固定U1茎II序列的寡聚体组成的更简单亚文库中进行RNA配体的体外筛选未产生共有序列,这表明自身免疫识别独立于环核苷酸发生。竞争试验证实了这些结合反应的特异性。这种自身免疫性U1 RNA表位的结构性质与基于天然小核核糖核蛋白颗粒刺激的自身抗体产生模型相符。

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