Lupus-associated atypical memory B cells are mTORC1-hyperactivated and functionally dysregulated

Chunmei Wu; Qiong Fu; Qiang Guo; Sheng Chen; Shyamal Goswami; Shuhui Sun; Teng Li; Xingjian Cao; Fuying Chu; Zechuan Chen; Mei Liu; Yuanhua Liu; Ting Fu; Pei Hao; Yi Hao; Nan Shen; Chunde Bao; Xiaoming Zhang

doi:10.1136/annrheumdis-2019-215039

Lupus-associated atypical memory B cells are mTORC1-hyperactivated and functionally dysregulated

Chunmei Wu(Shanghai Jiao Tong University), Qiong Fu(Shanghai Jiao Tong University), Qiang Guo(Shanghai Jiao Tong University), Sheng Chen(Shanghai Jiao Tong University), Shyamal Goswami(Chinese Academy of Sciences), Shuhui Sun(Shanghai Jiao Tong University), Teng Li(Chinese Academy of Sciences), Xingjian Cao(Nantong University), Fuying Chu(Nantong University), Zechuan Chen(Chinese Academy of Sciences), Mei Liu(Chinese Academy of Sciences), Yuanhua Liu(Chinese Academy of Sciences), Ting Fu(Chinese Academy of Sciences), Pei Hao(Chinese Academy of Sciences), Yi Hao(Huazhong University of Science and Technology), Nan Shen(Shanghai Jiao Tong University), Chunde Bao(Shanghai Jiao Tong University), Xiaoming Zhang(Chinese Academy of Sciences)

Annals of the Rheumatic Diseases

May 29, 2019

10.1136/annrheumdis-2019-215039

Cited by 97Open Access

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Abstract

<h3>Objectives</h3> A population of atypical memory B cells (AtMs) are greatly expanded in patients with active lupus, but their generation and pathophysiological roles are poorly defined. The aim of this study was to comprehensively characterise lupus AtMs with a purpose to identify therapeutic clues to target this B cell population in lupus. <h3>Methods</h3> Peripheral B cell subsets were measured by flow cytometry. Sorting-purified B cell subsets were subject to RNA sequencing and functional studies. Plasma cytokines and secreted immunoglobulins were detected by Luminex or ELISA. In situ renal B cells were detected by multiplexed immunohistochemistry. <h3>Results</h3> CD24<sup>−</sup>CD20<sup>hi</sup> AtMs were strongly increased in two Chinese cohorts of patients with treatment-naïve lupus. Gene expression profile indicated that B cell signalling and activation, lipid/saccharide metabolism and endocytosis pathways were abnormally upregulated in lupus AtMs. In addition, the mammalian target of rapamycin complex 1 (mTORC1) pathway was remarkably activated in lupus AtMs, and blocking mTORC1 signalling by rapamycin abolished the generation of T-bet<sup>+</sup> B cells and terminal differentiation of lupus AtMs. Furthermore, lupus AtMs displayed a dysfunctional phenotype, underwent accelerated apoptosis, poorly co-stimulated T cells and produced proinflammatory cytokines. Interestingly, lupus AtMs were in a paradoxically differentiated status with markers pro and against terminal differentiation and enriched with antinucleosome reactivity. Finally, AtMs were accumulated in the kidneys of patients with lupus nephritis and associated with disease severity. <h3>Conclusions</h3> These findings demonstrated that mTORC1-overactivated lupus AtMs are abnormally differentiated with metabolic and functional dysregulations. Inhibiting mTORC1 signalling might be an attractive option to target AtMs and to improve therapeutic effectiveness in patients with lupus.

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