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一个主要线性C1q表位的鉴定使得通过一种基于特定肽的酶联免疫吸附测定法检测系统性红斑狼疮抗C1q抗体成为可能。

Identification of a major linear C1q epitope allows detection of systemic lupus erythematosus anti-C1q antibodies by a specific peptide-based enzyme-linked immunosorbent assay.

作者信息

Vanhecke Dominique, Roumenina Lubka T, Wan Hui, Osthoff Michael, Schaller Monica, Trendelenburg Marten

机构信息

University Hospital Basel, Switzerland.

出版信息

Arthritis Rheum. 2012 Nov;64(11):3706-14. doi: 10.1002/art.34605.

DOI:10.1002/art.34605
PMID:22740328
Abstract

OBJECTIVE

Autoantibodies against C1q strongly correlate with the occurrence of severe nephritis in patients with systemic lupus erythematosus (SLE). We undertook this study to determine whether identification of the C1q epitope(s) recognized by these autoantibodies might lead to a better diagnostic assay and help elucidate the putative role of C1q and anti-C1q in SLE.

METHODS

SLE patient-derived anti-C1q Fab were used in a microarray-based peptide scan to identify the peptide sequence recognized by anti-C1q. Anti-C1q Fab binding to the target peptide was further analyzed using real-time interaction measurements (surface plasmon resonance) and peptide-based enzyme-linked immunosorbent assays (ELISAs).

RESULTS

A peptide scan of the collagen-like region of C1q identified 2 regions, 1 on the A chain and 1 on the B chain, that were the targets of the anti-C1q Fab. Binding was confirmed by surface plasmon resonance and showed nanomolar affinity. The A chain-derived peptide could specifically be detected in a peptide-based ELISA by SLE patient sera. Competition experiments suggested that this peptide represented one of the major linear epitopes of C1q that is the target of anti-C1q in SLE. Serum antibodies from most SLE patients but not from healthy individuals specifically bound to this epitope. Binding to the peptide correlated with binding of the same sera to native C1q but was found to be more sensitive for the detection of lupus nephritis.

CONCLUSION

We identified a major linear epitope of C1q that is the target of anti-C1q in SLE. The ELISA using this peptide was more specific and more sensitive than a conventional anti-C1q assay for the detection of active nephritis in SLE patients.

摘要

目的

抗C1q自身抗体与系统性红斑狼疮(SLE)患者严重肾炎的发生密切相关。我们开展本研究以确定识别这些自身抗体所针对的C1q表位是否可能带来更好的诊断检测方法,并有助于阐明C1q及抗C1q在SLE中的假定作用。

方法

将SLE患者来源的抗C1q Fab用于基于微阵列的肽扫描,以识别抗C1q所识别的肽序列。使用实时相互作用测量(表面等离子体共振)和基于肽的酶联免疫吸附测定(ELISA)进一步分析抗C1q Fab与靶肽的结合。

结果

对C1q胶原样区域进行肽扫描,确定了2个区域,1个在A链上,1个在B链上,它们是抗C1q Fab的靶标。表面等离子体共振证实了结合,并显示出纳摩尔亲和力。A链衍生的肽可在基于肽的ELISA中被SLE患者血清特异性检测到。竞争实验表明,该肽代表了C1q的主要线性表位之一,是SLE中抗C1q的靶标。大多数SLE患者而非健康个体的血清抗体特异性结合该表位。与该肽的结合与相同血清与天然C1q的结合相关,但发现其对狼疮性肾炎的检测更敏感。

结论

我们确定了C1q的一个主要线性表位,它是SLE中抗C1q的靶标。使用该肽的ELISA在检测SLE患者的活动性肾炎方面比传统抗C1q检测更特异、更敏感。

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