Loss of ARHGEF1 causes a human primary antibody deficiency
Amine Bouafia, … , Eric Oksenhendler, Sven Kracker
Amine Bouafia, … , Eric Oksenhendler, Sven Kracker
Published December 6, 2018
Citation Information: J Clin Invest. 2019;129(3):1047-1060. https://doi.org/10.1172/JCI120572.
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Research Article Immunology

Loss of ARHGEF1 causes a human primary antibody deficiency

Abstract

ARHGEF1 is a RhoA-specific guanine nucleotide exchange factor expressed in hematopoietic cells. We used whole-exome sequencing to identify compound heterozygous mutations in ARHGEF1, resulting in the loss of ARHGEF1 protein expression in 2 primary antibody–deficient siblings presenting with recurrent severe respiratory tract infections and bronchiectasis. Both ARHGEF1-deficient patients showed an abnormal B cell immunophenotype, with a deficiency in marginal zone and memory B cells and an increased frequency of transitional B cells. Furthermore, the patients’ blood contained immature myeloid cells. Analysis of a mediastinal lymph node from one patient highlighted the small size of the germinal centers and an abnormally high plasma cell content. On the molecular level, T and B lymphocytes from both patients displayed low RhoA activity and low steady-state actin polymerization (even after stimulation of lysophospholipid receptors). As a consequence of disturbed regulation of the RhoA downstream target Rho-associated kinase I/II (ROCK), the patients’ lymphocytes failed to efficiently restrain AKT phosphorylation. Enforced ARHGEF1 expression or drug-induced activation of RhoA in the patients’ cells corrected the impaired actin polymerization and AKT regulation. Our results indicate that ARHGEF1 activity in human lymphocytes is involved in controlling actin cytoskeleton dynamics, restraining PI3K/AKT signaling, and confining B lymphocytes and myelocytes within their dedicated functional environment.

Authors

Amine Bouafia, Sébastien Lofek, Julie Bruneau, Loïc Chentout, Hicham Lamrini, Amélie Trinquand, Marie-Céline Deau, Lucie Heurtier, Véronique Meignin, Capucine Picard, Elizabeth Macintyre, Olivier Alibeu, Marc Bras, Thierry Jo Molina, Marina Cavazzana, Isabelle André-Schmutz, Anne Durandy, Alain Fischer, Eric Oksenhendler, Sven Kracker

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Figure 2

Histological analysis of mediastinal lymph node biopsies of P2, indicating a disturbed GC reaction.

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Histological analysis of mediastinal lymph node biopsies of P2, indicati...
Pictures of mediastinal lymph nodes of P2 and a control lymph node stained with the indicated antibodies, highlighting the GC structures. Original magnification, ×200; scale bar: 50 μm (H&E, CD3, CD5, CD20, CD79a, CD10, BCL6, PD1, Ki67, IgD, CD138, IgA, and IgM).Original magnification, ×100; scale bar: 100 μm (CD4 and CD8). Original magnification, ×50; scale bar: 200 μm (CD21).