CD4 T 细胞 repertoire 的高通量测序揭示了 IgG4 相关疾病中的疾病特异性特征。
High-throughput sequencing of CD4 T cell repertoire reveals disease-specific signatures in IgG4-related disease.
机构信息
Department of Rheumatology, Peking Union Medical College Hospital, Chinese Academy of Medical Science & Peking Union Medical College, Key Laboratory of Rheumatology and Clinical Immunology, Ministry of Education, No.41 Da Mu Cang, Western District, Beijing, 100032, People's Republic of China.
Department of General Surgery, Ruijin Hospital, School of Medicine, Shanghai Jiao Tong University, Shanghai, China.
出版信息
Arthritis Res Ther. 2019 Dec 19;21(1):295. doi: 10.1186/s13075-019-2069-6.
BACKGROUND
CD4 T cells play critical roles in the pathogenesis of IgG4-related disease (IgG4-RD). The aim of this study was to investigate the TCR repertoire of peripheral blood CD4 T cells in IgG4-RD.
METHODS
The peripheral blood was collected from six healthy controls and eight IgG4-RD patients. TCR β-chain libraries of CD4 T cells were constructed by 5'-rapid amplification of cDNA ends (5'-RACE) and sequenced by Illumina Miseq platform. The relative similarity of TCR repertoires between samples was evaluated according to the total frequencies of shared clonotypes (metric F), correlation of frequencies of shared clonotypes (metric R), and total number of shared clonotypes (metric D).
RESULTS
The clonal expansion and diversity of CD4 T cell repertoire were comparable between healthy controls and IgG4-RD patients, while the proportion of expanded and coding degenerated clones, as an indicator of antigen-driven clonal expansion, was significantly higher in IgG4-RD patients. There was no significant difference in TRBV and TRBJ gene usage between healthy controls and IgG4-RD patients. The complementarity determining region 3 (CDR3) length distribution was skewed towards longer fragments in IgG4-RD. Visualization of relative similarity of TCR repertoires by multi-dimensional scaling analysis showed that TCR repertoires of IgG4-RD patients were separated from that of healthy controls in F and D metrics. We identified 11 IgG4-RD-specific CDR3 amino acid sequences that were expanded in at least 2 IgG4-RD patients, while not detected in healthy controls. According to TCR clonotype networks constructed by connecting all the CDR3 sequences with a Levenshtein distance of 1, 3 IgG4-RD-specific clusters were identified. We annotated the TCR sequences with known antigen specificity according to McPAS-TCR database and found that the frequencies of TCR sequences associated with each disease or immune function were comparable between healthy controls and IgG4-RD patients.
CONCLUSION
According to our study of CD4 T cells from eight IgG4-RD patients, TCR repertoires of IgG4-RD patients were different from that of healthy controls in the proportion of expanded and coding degenerated clones and CDR3 length distribution. In addition, IgG4-RD-specific TCR sequences and clusters were identified in our study.
背景
CD4 T 细胞在 IgG4 相关疾病(IgG4-RD)的发病机制中发挥关键作用。本研究旨在探讨 IgG4-RD 患者外周血 CD4 T 细胞的 TCR 库。
方法
采集 6 名健康对照者和 8 名 IgG4-RD 患者的外周血。通过 5'-快速扩增 cDNA 末端(5'-RACE)构建 CD4 T 细胞 TCRβ 链文库,并通过 Illumina Miseq 平台进行测序。根据共享克隆型的总频率(度量 F)、共享克隆型频率的相关性(度量 R)和共享克隆型的总数(度量 D)评估样本之间 TCR 库的相对相似性。
结果
健康对照组和 IgG4-RD 患者的 CD4 T 细胞受体库的克隆扩增和多样性相当,而作为抗原驱动克隆扩增的指标,IgG4-RD 患者的扩增和编码退化克隆的比例显著更高。健康对照组和 IgG4-RD 患者之间的 TRBV 和 TRBJ 基因使用没有显著差异。IgG4-RD 中互补决定区 3(CDR3)长度分布偏向于较长片段。多维尺度分析显示相对相似性的 TCR 库的可视化 IgG4-RD 患者的 TCR 库在 F 和 D 度量中与健康对照组分离。我们鉴定了 11 个 IgG4-RD 特异性 CDR3 氨基酸序列,这些序列在至少 2 个 IgG4-RD 患者中扩增,而在健康对照中未检测到。根据连接所有 CDR3 序列的 Levenshtein 距离为 1 的 TCR 克隆型网络构建,鉴定了 3 个 IgG4-RD 特异性聚类。根据 McPAS-TCR 数据库,我们根据已知抗原特异性对 TCR 序列进行注释,发现健康对照组和 IgG4-RD 患者之间与每种疾病或免疫功能相关的 TCR 序列的频率相当。
结论
根据我们对 8 名 IgG4-RD 患者的 CD4 T 细胞的研究,IgG4-RD 患者的 TCR 库在扩增和编码退化克隆的比例以及 CDR3 长度分布方面与健康对照组不同。此外,在本研究中鉴定了 IgG4-RD 特异性 TCR 序列和聚类。
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