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Published in: Arthritis Research & Therapy 1/2017

Open Access 01-12-2017 | Research article

Circulating plasmablasts/plasma cells: a potential biomarker for IgG4-related disease

Authors: Wei Lin, Panpan Zhang, Hua Chen, Yu Chen, Hongxian Yang, Wenjie Zheng, Xuan Zhang, Fengxiao Zhang, Wen Zhang, Peter E. Lipsky

Published in: Arthritis Research & Therapy | Issue 1/2017

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Abstract

Background

Immunoglobulin G4 (IgG4)-related disease (IgG4-RD) is a multisystem fibroinflammatory disease. We previously reported that a circulating cell population expressing CD19+CD24CD38hi was increased in patients with IgG4-RD. In this study, we aimed to document that this cell population represented circulating plasmablasts/plasma cells, to identify the detailed phenotype and gene expression profile of these IgG4-secreting plasmablasts/plasma cells, and to determine whether this B-cell lineage subset could be a biomarker in IgG4-related disease (IgG4-RD).

Methods

A total of 42 untreated patients with IgG4-RD were evaluated. Peripheral B-cell subsets, including CD19+CD24CD38hi plasmablasts/plasma cells, CD19+CD24+CD38 memory B cells, CD19+CD24intCD38int naïve B cells, and CD19+CD24hiCD38hi regulatory B cells, were assessed and sorted by flow cytometry. Microarray analysis was used to measure gene expression of circulating B-cell lineage subsets. Further characterization of CD19+CD24CD38hi plasmablasts/plasma cells was carried out by evaluating additional surface markers, including CD27, CD95, and human leukocyte antigen (HLA)-DR, by flow cytometric assay. In addition, various B-cell lineage subsets were cultured in vitro and IgG4 concentrations were measured by cytometric bead array.

Results

In untreated patients with IgG4-RD, the peripheral CD19+CD24CD38hi plasmablast/plasma cell subset was increased and positively correlated with serum IgG4 levels, the number of involved organs, and the IgG4-related Disease Responder Index. It decreased after treatment with glucocorticoids. Characterization of the plasmablast/plasma cell population by gene expression profiling documented a typical plasmablast/plasma cell signature with higher expression of X-box binding protein 1 and IFN regulatory factor 4, but lower expression of paired box gene 5 and B-cell lymphoma 6 protein. In addition, CD27, CD95, and HLA-DR were highly expressed on CD19+CD24CD38hi plasmablasts/plasma cells from patients with IgG4-RD. Furthermore, CD19+CD24CD38hi plasmablasts/plasma cells secreted more IgG4 than other B-cell populations.

Conclusions

Circulating CD19+CD24CD38hi plasmablasts/plasma cells are elevated in active IgG4-RD and decreased after glucocorticoid treatment. This IgG4-secreting plasmablast/plasma cell population might be a potentially useful biomarker for diagnosis and assessing response to treatment.
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Metadata
Title
Circulating plasmablasts/plasma cells: a potential biomarker for IgG4-related disease
Authors
Wei Lin
Panpan Zhang
Hua Chen
Yu Chen
Hongxian Yang
Wenjie Zheng
Xuan Zhang
Fengxiao Zhang
Wen Zhang
Peter E. Lipsky
Publication date
01-12-2017
Publisher
BioMed Central
Published in
Arthritis Research & Therapy / Issue 1/2017
Electronic ISSN: 1478-6362
DOI
https://doi.org/10.1186/s13075-017-1231-2

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