BRD7 as key factor in PBAF complex assembly and CD8+ T cell differentiation
Feng Huang, Yingtong Lin, Yidan Qiao, Yaochang Yuan, Zhihan Zhong, Baohong Luo, Yating Wu, Jun Liu, Jingliang Chen, Wanying Zhang, Hui Zhang, Bingfeng Liu
Feng Huang, Yingtong Lin, Yidan Qiao, Yaochang Yuan, Zhihan Zhong, Baohong Luo, Yating Wu, Jun Liu, Jingliang Chen, Wanying Zhang, Hui Zhang, Bingfeng Liu
View: Text | PDF
Research Article Immunology Infectious disease

BRD7 as key factor in PBAF complex assembly and CD8+ T cell differentiation

Abstract

Upon infection, naive CD8+ T cells differentiate into cytotoxic effector cells to eliminate the pathogen-infected cells. Although many mechanisms underlying this process have been demonstrated, the regulatory role of chromatin remodeling system in this process remains largely unknown. Here we show that BRD7, a component of the polybromo-associated BAF complex (PBAF), was required for naive CD8+ T cells to differentiate into functional short-lived effector cells (SLECs) in response to acute infections caused by influenza virus or lymphocytic choriomeningitis virus (LCMV). BRD7 deficiency in CD8+ T cells resulted in profound defects in effector population and functions, thereby impairing viral clearance and host recovery. Further mechanical studies indicate that the expression of BRD7 significantly turned to high from naive CD8+ T cells to effector cells, which bridged BRG1 and PBRM1 to the core module of PBAF complex, consequently facilitating the assembly of PBAF complex rather than BAF complex in the effector cells. The PBAF complex changed the chromatin accessibility at the loci of Tbx21 gene and upregulated its expression, leading to the maturation of effector T cells. Our research demonstrates that BRD7 and the PBAF complex are key in CD8+ T cell development and present a significant target for advancing immune therapies.

Authors

Feng Huang, Yingtong Lin, Yidan Qiao, Yaochang Yuan, Zhihan Zhong, Baohong Luo, Yating Wu, Jun Liu, Jingliang Chen, Wanying Zhang, Hui Zhang, Bingfeng Liu

×

Figure 4

BRD7 controls SLEC differentiation during LCMV infection.

Options: View larger image (or click on image) Download as PowerPoint
BRD7 controls SLEC differentiation during LCMV infection. (A) Flow cytom...
(A) Flow cytometry of Arm gp33+CD8+ T cells from spleen of Brd7fl/fl (n = 3) and Brd7ΔT (n = 4) mice. Brd7fl/fl and Brd7ΔT mice were infected with LCMV-Arm virus, and antigen-specific gp33 tetramer was stained in spleen CD8+ T cells at day 8 p.i. Numbers beside outlined areas indicate percent of gp33+CD8+ T cells. (B) Frequency (left) and cell number (right) of gp33-specific cells among CD8+ T cells in A. (C) Flow cytometry of KLRG1 and CD127 on gp33+CD8+ T cells in the spleen obtained from Brd7fl/fl (n = 3) or Brd7ΔT (n = 4) mice infected with Arm at 8 d p.i. Numbers in quadrants indicate percent of KLRG1+CD127 SLECs (top left) or KLRG1CD127+ MPECs (bottom right). (D) Frequency of KLRG1+CD127 SLECs or KLRG1CD127+ MPECs among gp33+CD8+ T cells in C. (E and F) Intracellular cytokine staining of IFN-γ (E) or TNF-α (F) produced by splenic CD8+ T cells from Brd7fl/fl (n = 3) and Brd7ΔT (n = 4) mice infected with Arm virus stimulated with gp33 peptide at day 8 p.i. Number beside outlined areas indicates percentage of IFN-γ+CD8+ (E) or TNF-α+CD8+ (F) T cells. Frequency of IFN-γ+ (E) or TNF-α+ (F) cells among CD8+ T cells in left. (G) LCMV Arm virus titers in the spleen of Brd7fl/fl (n = 3) or Brd7ΔT (n = 4) mice infected with LCMV Arm strain were determined at day 8 p.i. Data are shown as mean ± SEM. *P < 0.05, **P < 0.01 (2-tailed Student’s t test). Data are representative of 3 independent experiments.