采用 LC-MS/MS 多重反应监测模式对可溶性共刺激分子进行定量分析，作为类风湿关节炎潜在的诊断生物标志物。

Quantitative analysis of soluble costimulatory molecules as potential diagnostic biomarkers for rheumatoid arthritis using LC-MS/MS in MRM mode.

机构信息

Department of Chemistry, University of Quebec at Montreal, Montreal, QC H3C3P8, Canada.

Department of Medical Laboratory Sciences, Jordan University of Science and Technology, Irbid 22110, Jordan.

出版信息

Clin Chim Acta. 2023 Aug 1;548:117501. doi: 10.1016/j.cca.2023.117501. Epub 2023 Jul 27.

DOI:10.1016/j.cca.2023.117501

PMID:37516334

Abstract

BACKGROUND AND AIMS

Rheumatoid arthritis (RA) is a chronic autoimmune disease. RA-induced immunological responses are coordinated by T-cell stimulation. The costimulatory signal CD28-B7 is essential for T-cell activation by interacting CD28 with CD80 and CD86 costimulatory proteins. CTLA4 is another costimulatory protein that binds to CD80 and CD86 to inhibit T-cell activity. The soluble costimulatory proteins: sCD80, sCD86, sCD28, and sCTLA-4 were detected and quantified in human plasma and correlated with RA development. As potential diagnostic biomarkers for RA, developing a sensitive, specific, and reproducible method for quantifying these costimulatory molecules in human plasma and establishing quantitative ranges for each protein in healthy and RA patients' plasma is essential for advancing the clinical diagnostic and health outcomes.

MATERIALS AND METHODS

A novel quantitative liquid chromatography-tandem spectrometry (LC-MS/MS) technique using multiple reaction monitoring (MRM) modes was developed and validated to measure soluble costimulatory molecules sCTLA4, sCD28, sCD80, and sCD86 in human plasma samples. Furthermore, the method was applied to determine sCTLA4, sCD28, sCD80, and sCD86 levels in plasma samples from RA patients (n = 23) and healthy controls (n = 21).

RESULTS

The method was successfully developed and validated according to international inter- and intra-assay precision and accuracy guidelines. The linearity of the method was achieved between 0.5 nM and 100 nM for each protein with a correlation coefficient of > 0.998. The plasma level of sCTLA4, sCD80, and sCD86 in RA patients was significantly elevated compared to controls. RA patients had 63.32 ± 17.63 nM sCTLA4 and controls 36.05 ± 18.83 nM; p < 0.0001. The performance of the four proteins was determined using ROC curves, where sCTLA4 showed the highest diagnostic and clinical performance compared to the others.

CONCLUSIONS

This study reports the first use of LC-MS/MS in MRM mode to accurately quantify soluble costimulatory molecules in plasma samples as potential RA diagnostic biomarkers. Determination of the reference range for each protein with high selectivity and sensitivity increases the potential for utilizing this method as a clinical diagnostic.

摘要

背景与目的

类风湿关节炎（RA）是一种慢性自身免疫性疾病。RA 诱导的免疫反应由 T 细胞刺激协调。共刺激信号 CD28-B7 通过与共刺激蛋白 CD80 和 CD86 相互作用对于 T 细胞的激活至关重要。CTLA4 是另一种共刺激蛋白，它与 CD80 和 CD86 结合以抑制 T 细胞活性。可溶性共刺激蛋白：sCD80、sCD86、sCD28 和 sCTLA-4 在人血浆中被检测和定量，并与 RA 的发展相关。作为 RA 的潜在诊断生物标志物，开发一种灵敏、特异和可重复的方法来定量检测人血浆中的这些共刺激分子，并建立健康和 RA 患者血浆中每种蛋白的定量范围，对于推进临床诊断和健康结果至关重要。

材料和方法

开发并验证了一种新型的液相色谱-串联质谱（LC-MS/MS）技术，该技术使用多重反应监测（MRM）模式来测量人血浆样品中的可溶性共刺激分子 sCTLA4、sCD28、sCD80 和 sCD86。此外，该方法还应用于确定 RA 患者（n=23）和健康对照者（n=21）血浆样品中的 sCTLA4、sCD28、sCD80 和 sCD86 水平。

结果

该方法根据国际间和内分析精度和准确性指南成功开发和验证。每种蛋白的线性范围均为 0.5 nM 至 100 nM，相关系数均>0.998。与对照组相比，RA 患者的 sCTLA4、sCD80 和 sCD86 血浆水平显著升高。RA 患者的 sCTLA4 为 63.32±17.63 nM，对照组为 36.05±18.83 nM；p<0.0001。使用 ROC 曲线确定了这四种蛋白的性能，其中 sCTLA4 与其他蛋白相比具有最高的诊断和临床性能。