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强烈炎症对于关节软骨特异性瓜氨酸化抗原的表达至关重要。

[Strong inflammation is essential for expression of articular cartilage-specific citrullinated antigens].

作者信息

Qin Guicheng, Lin Xiaoyin, Liang Peibin, Li Yanpeng, Zhou Chun, Kutty Selva Nandakumar, Rikard Holmdahl

机构信息

SMU-KI United Medical Inflammation Center, School of Pharmaceutical Sciences, Southern Medical University, Guangzhou 510515, China.

Medical Inflammation Research, Department of Medical Biochemistry and Biophysics, Karolinska Institute, SE-17177, Stockholm, Sweden.

出版信息

Nan Fang Yi Ke Da Xue Xue Bao. 2020 Aug 30;40(8):1081-1089. doi: 10.12122/j.issn.1673-4254.2020.08.03.

Abstract

OBJECTIVE

To investigate the expression of citrullinated epitopes in articular cartilage protein and whether its expression is sufficient to induce anti-citrullinated protein antibody (ACPA) response in mice.

METHODS

The experimental group was treated with different concentrations of lipopolysaccharide (LPS), heat-inactivated bacteria ( and ) or specific monoclonal antibody against type Ⅱ collagen to induce citrullination of articular cartilage protein, with PBS as the control. Immunohistochemistry with the monoclonal antibody ACC4 (IgG1) that specifically binds to the citrullinated epitope of cartilage protein was performed for detecting the expression of citrullinated protein, with ACC1 (IgG2a) as a positive control antibody and L243 (IgG2a) and Hy2.15 (IgG1) as the negative isotype control. In the in vivo experiment, SD rats were subjected to injection of different doses of LPS in the right knee (with PBS as the controls in the left knee), and 3 days later frozen sections were prepared for immunohistochemical detection of the expression of citrullinated protein. Models of collagen-induced arthritis (CIA) established in different mouse strains were observed for incidence and severity of CIA. Serum samples collected from these models and the sera from rheumatoid arthritis patients were examined for anti-citrullinated protein antibody, and immunohistochemistry was performed to detect the expression of citrullinated protein in the cartilage of the mouse.

RESULTS

The citrullinated CII epitope-specific antibody ACC4 did not bind to articular cartilage tissues with different treatments as compared with the positive control antibody ACC1. The ACC4 antibody and the antibodies from patients with rheumatoid arthritis with high titers of anti-citrullinated protein antibody were capable of binding to the synovial tissue around the articular cartilage of the CIA. Luminex analysis showed that the anti-citrullinated protein antibody was lowly expressed in mouse serum, but the anti-type Ⅱ collagen triple helix structure peptide antibody exhibited strong reactivity.

CONCLUSIONS

Mild acute inflammatory response is not enough to cause citrullination of articular cartilage protein, and the expression of specific epitope requires a high-intensity inflammatory response. Inflammatory articular cartilage protein can express citrullinated epitopes in type Ⅱ collagen-induced arthritis in mice, but the expression of citrullinated epitopes is not sufficient to induce an immune response to anti-citrullinated antibodies. Stronger stimulation signals are required to induce an immune response for producing anti-citrullinated protein antibodies.

摘要

目的

研究瓜氨酸化表位在关节软骨蛋白中的表达情况,以及其表达是否足以在小鼠中诱导抗瓜氨酸化蛋白抗体(ACPA)反应。

方法

实验组用不同浓度的脂多糖(LPS)、热灭活细菌(和)或抗Ⅱ型胶原特异性单克隆抗体处理,以诱导关节软骨蛋白瓜氨酸化,以PBS作为对照。用特异性结合软骨蛋白瓜氨酸化表位的单克隆抗体ACC4(IgG1)进行免疫组织化学检测瓜氨酸化蛋白的表达,以ACC1(IgG2a)作为阳性对照抗体,L243(IgG2a)和Hy2.15(IgG1)作为阴性同型对照。在体内实验中,给SD大鼠右膝注射不同剂量的LPS(左膝以PBS作为对照),3天后制备冰冻切片用于免疫组织化学检测瓜氨酸化蛋白的表达。观察不同小鼠品系建立的胶原诱导性关节炎(CIA)模型的CIA发病率和严重程度。检测这些模型收集的血清样本以及类风湿关节炎患者血清中的抗瓜氨酸化蛋白抗体,并进行免疫组织化学检测小鼠软骨中瓜氨酸化蛋白的表达。

结果

与阳性对照抗体ACC1相比,瓜氨酸化CII表位特异性抗体ACC4未与不同处理的关节软骨组织结合。ACC4抗体以及来自高滴度抗瓜氨酸化蛋白抗体的类风湿关节炎患者的抗体能够与CIA关节软骨周围的滑膜组织结合。Luminex分析显示,抗瓜氨酸化蛋白抗体在小鼠血清中低表达,但抗Ⅱ型胶原三螺旋结构肽抗体表现出强反应性。

结论

轻度急性炎症反应不足以导致关节软骨蛋白瓜氨酸化,特定表位的表达需要高强度炎症反应。炎症性关节软骨蛋白在小鼠Ⅱ型胶原诱导性关节炎中可表达瓜氨酸化表位,但瓜氨酸化表位的表达不足以诱导对抗瓜氨酸化抗体的免疫反应。需要更强的刺激信号来诱导产生抗瓜氨酸化蛋白抗体的免疫反应。

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[The pathogenic role of ACPA in rheumatoid arthritis].[抗环瓜氨酸肽抗体在类风湿关节炎中的致病作用]
Nihon Rinsho Meneki Gakkai Kaishi. 2017;40(6):391-395. doi: 10.2177/jsci.40.391.

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