Identification of novel genes associated with dysregulation of B cells in patients with primary Sjogren's syndrome

被引:26
|
作者
Inamo, Jun [1 ]
Suzuki, Katsuya [1 ]
Takeshita, Masaru [1 ]
Kassai, Yoshiaki [2 ]
Takiguchi, Maiko [2 ]
Kurisu, Rina [2 ]
Okuzono, Yuumi [2 ]
Tasaki, Shinya [3 ,4 ]
Yoshimura, Akihiko [5 ]
Takeuchi, Tsutomu [1 ]
机构
[1] Keio Univ, Dept Internal Med, Div Rheumatol, Sch Med,Shinjuku Ku, 35 Shinanomachi, Tokyo 1608582, Japan
[2] Takeda Pharmaceut Co Ltd, Lmmunol Unit, Pharmaceut Res Div, Yokohama, Kanagawa, Japan
[3] Takeda Pharmaceut Co Ltd, Integrated Technol Res Labs, Pharmaceut Res Div, Yokohama, Kanagawa, Japan
[4] Rush Univ, Rush Alzheimers Dis Ctr, Med Ctr, Chicago, IL 60612 USA
[5] Keio Univ, Dept Microbiol & Immunol, Sch Med, Tokyo, Japan
关键词
Primary Sjogren's syndrome; B cells; Long non-coding RNA; Transcriptome; Gene co-expression network; LONG NONCODING RNAS; CLASSIFICATION CRITERIA; T-CELLS; EXPRESSION; INTERFERON; TOLERANCE; SOX4;
D O I
10.1186/s13075-020-02248-2
中图分类号
R5 [内科学];
学科分类号
1002 ; 100201 ;
摘要
BackgroundThe aim of this study was to identify the molecular mechanism of dysregulation of B cell subpopulations of primary Sjogren's syndrome (pSS) at the transcriptome level.MethodsWe enrolled patients with pSS (n=6) and healthy controls (HCs) (n=6) in the discovery cohort using microarray and pSS (n=14) and HCs (n=12) in the validation cohort using quantitative PCR (qPCR). Peripheral B cells acquired from these subjects were separated by cell sorting into four subsets: CD38(-)IgD(+) (Bm1), CD38(+)IgD(+) (naive B cells), CD38(high)IgD(+) (pre-germinal centre B cells) and CD38IgD(-) (memory B cells). We performed differentially expressed gene (DEG) analysis and weighted gene co-expression network analysis (WGCNA).ResultsExpression of the long non-coding RNA LINC00487 was significantly upregulated in all B cell subsets, as was that of HLA and interferon (IFN) signature genes. Moreover, the normalized intensity value of LINC00487 significantly correlated with the disease activity score of all pSS B cell subsets. Studies of human B cell lines revealed that the expression of LINC00487 was strongly induced by IFN alpha. WGCNA revealed six gene clusters associated with the B cell subpopulation of pSS. Further, SOX4 was identified as an inter-module hub gene.ConclusionOur transcriptome analysis revealed key genes involved in the dysregulation of B cell subpopulations associated with pSS.
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页数:11
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