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Proteomic analysis of saliva: a unique tool to distinguish primary Sjogren's syndrome from secondary Sjogren's syndrome and other sicca syndromes

机译:唾液蛋白质组学分析:区分原发性干燥综合征与继发性干燥综合征和其他干燥综合征的独特工具

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摘要

Introduction: A growing interest has arisen in salivary proteomics as a tool for the identification of biomarkers for primary Sjogren's syndrome (pSS). Nonetheless, only a limited number of preclinical validation studies have been performed, limiting the possibility of translating proteomic results into clinical practice. The primary aim of this study was to refine the diagnostic power of a panel of candidate salivary biomarkers described in pSS with respect to both healthy volunteers and pathological controls. We also explored the pathogenetic function of the detected putative biomarkers both in the local exocrinopathy and in the systemic inflammatory processes of SS. Methods: One hundred and eighty patients were included in the study overall. In the first "exploratory phase", we enrolled 40 females with pSS, 40 sex-and age-matched healthy volunteers, 10 patients with sicca non-SS and 15 secondary SS (sSS) patients. The testing cohort of the second "challenge phase" of the study was represented by 75 unselected, consecutive subjects: 19 pSS, 21 healthy volunteers, 10 sicca non-SS and 25 sSS patients. Salivary proteomic analysis was performed combining two-dimensional electrophoresis (2DE) and matrix-assisted laser desorption/ionisation time-of-flight mass spectrometry (MALDI-TOF-MS). Western blot (WB) analysis and enzyme-linked immunosorbent assay (ELISA) were employed to validate 2DE results. Ingenuity Pathway Analysis (IPA) Knowledge base was adopted to associate candidate biomarkers in a signalling pathogenetic network. Results: A total of 28, 6, 7 and 12 protein spots were found to be significantly different in pSS samples with respect to healthy volunteers, non-SS sicca syndrome, SSc-sSS and rheumatoid arthritis-sSS, leading to the identification of 15 differently expressed proteins. Among them, alpha-amylases precursor, carbonic anhydrase VI, beta-2 microglobulin, glyceraldehydes-3-phosphate dehydrogenase (G3PDH), epidermal fatty acid binding protein (E-FABP) and immunoglobulin k light chain (IGK-light chain) apparently showed the most significant differences in pSS when compared to healthy volunteers and non-SS pathological controls. On the other hand, as expected, pSS and sSS salivary profiles shared a great number of similarities. Conclusions: This study demonstrated that salivary fluid might represent a novel ideal milieu for the detection of a diagnostic panel of candidate biomarkers for pSS, and to gain an insight into the pathogenetic processes underlying glandular and systemic autoimmune disorders.
机译:简介:唾液蛋白质组学作为一种识别原发性干燥综合征(pSS)的生物标志物的工具已引起越来越多的关注。但是,仅进行了有限的临床前验证研究,从而限制了将蛋白质组学结果转化为临床实践的可能性。这项研究的主要目的是针对健康志愿者和病理对照患者,完善pSS中描述的一组唾液生物标志物的诊断能力。我们还探讨了在局部外分泌病和SS的全身炎症过程中检测到的假定生物标志物的致病功能。方法:总共包括180名患者。在第一个“探索阶段”,我们招募了40名患有pSS的女性,40名性别和年龄相匹配的健康志愿者,10例非干燥性非SS患者和15例继发性SS(sSS)患者。该研究的第二个“挑战阶段”的测试队列由75名未选择的连续受试者代表:19名pSS,21名健康志愿者,10名非sicca非SS和25名sSS患者。结合二维电泳(2DE)和基质辅助激光解吸/电离飞行时间质谱(MALDI-TOF-MS)进行唾液蛋白质组学分析。 Western blot(WB)分析和酶联免疫吸附测定(ELISA)用于验证2DE结果。采用了机敏途径分析(IPA)知识库来关联信号致病性网络中的候选生物标记。结果:与健康志愿者,非SS干燥综合征,SSc-sSS和类风湿关节炎-sSS相比,pSS样品中共有28、6、7和12个蛋白斑点显着不同,从而鉴定出15个表达不同的蛋白质。其中,α-淀粉酶前体,碳酸酐酶VI,β-2微球蛋白,甘油醛-3-磷酸脱氢酶(G3PDH),表皮脂肪酸结合蛋白(E-FABP)和免疫球蛋白k轻链(IGK-轻链)明显显示与健康志愿者和非SS病理对照相比,pSS的最显着差异。另一方面,正如预期的那样,pSS和sSS的唾液谱具有许多相似之处。结论:这项研究表明,唾液可能代表了一种新颖的理想环境,可用于检测pSS候选生物标志物的诊断小组,并深入了解腺体和全身性自身免疫性疾病的致病过程。

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