DOCK8 is essential for LFA-1–dependent positioning of T follicular helper cells in germinal centers
Erin Janssen, … , Facundo Batista, Raif S. Geha
Erin Janssen, … , Facundo Batista, Raif S. Geha
Published June 23, 2020
Citation Information: JCI Insight. 2020;5(15):e134508. https://doi.org/10.1172/jci.insight.134508.
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Research Article Immunology

DOCK8 is essential for LFA-1–dependent positioning of T follicular helper cells in germinal centers

Abstract

T follicular helper (Tfh) cell migration into germinal centers (GCs) is essential for the generation of GC B cells and antibody responses to T cell–dependent (TD) antigens. This process requires interactions between lymphocyte function–associated antigen 1 (LFA-1) on Tfh cells and ICAMs on B cells. The mechanisms underlying defective antibody responses to TD antigens in DOCK8 deficiency are incompletely understood. We show that mice selectively lacking DOCK8 in T cells had impaired IgG antibody responses to TD antigens, decreased GC size, and reduced numbers of GC B cells. However, they developed normal numbers of Tfh cells with intact capacity for driving B cell differentiation into a GC phenotype in vitro. Notably, migration of DOCK8-deficient T cells into GCs was defective. Following T cell receptor (TCR)/CD3 ligation, DOCK8-deficient T cells had impaired LFA-1 activation and reduced binding to ICAM-1. Our results therefore indicate that DOCK8 is important for LFA-1–dependent positioning of Tfh cells in GCs, and thereby the generation of GC B cells and IgG antibody responses to TD antigen.

Authors

Erin Janssen, Mira Tohme, Jordan Butts, Sophie Giguere, Peter T. Sage, Francisco E. Velázquez, Christy Kam, Elena Milin, Mrinmoy Das, Ali Sobh, Salem Al-Tamemi, Francis W. Luscinskas, Facundo Batista, Raif S. Geha

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Figure 2

Cd4-CreTgDock8fl/fl mice have a marked reduction in GC B cells after immunization with TD antigen.

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Cd4-CreTgDock8fl/fl mice have a marked reduction in GC B cells after im...
Draining LNs from Cd4-CreTgDock8fl/fl and control mice immunized in the hocks with TNP-KLH were examined on day 2 for pre-GC B cells, on day 7 for GC B cells, and on day 10 for GC size. (A) Representative immunofluorescence photomicrograph of popliteal LNs (left). B cell follicles (IgD+) are in green, GCs (GL7+) in red, and the T cell zones (TCRβ+) in blue. Images are at ×20 magnification. Quantification of GC size (right). n = 4–5 mice/group in 2 pooled independent experiments. ANOVA; *P < 0.05. (B) TNP-specific IgG affinity determined on day 14 after immunization. n = 4 mice/group. Results are representative of 2 independent experiments. (C) Representative flow cytometry plots, and percentages and numbers of FAS+GL7+ GC B cells in draining LNs. n = 7 mice/group. (D) MFI of surface FAS and GL7 by B220+GL7+ and B220+FAS+ cells, respectively. n = 5–6 mice/group. (E) Percentages of BCL6+KI-67+ B cells in draining LNs. n = 4 mice/group. (F) MFI of BCL6 and KI-67 (right) in BCL6+ B cells. n = 4 mice/group. (G) Percentage of FASintGL7loIgDhiCCR6hi pre-GC B cells and MFI of KI-67 in pre-GC B cells. n = 7 mice/group from 2 pooled experiments. D–F show a representative experiment of 3. Data are presented as mean ± SEM. Student’s t test; *P < 0.05, **P < 0.01, ***P < 0.001.