Differential effects of HDAC8 targeting on Foxp3+ Tregs and effector T cells promote antitumor immunity
Fanhua Kong, Yan Xiong, Liqing Wang, Rongxiang Han, Hossein Fazelinia, Jennifer Roof, Lynn Spruce, Aaron B. Beeler, Wayne W. Hancock
Fanhua Kong, Yan Xiong, Liqing Wang, Rongxiang Han, Hossein Fazelinia, Jennifer Roof, Lynn Spruce, Aaron B. Beeler, Wayne W. Hancock
View: Text | PDF
Research Article Immunology Oncology

Differential effects of HDAC8 targeting on Foxp3+ Tregs and effector T cells promote antitumor immunity

Abstract

HDAC8, an evolutionarily distinct, X-linked, zinc-dependent class I histone/protein deacetylase, is implicated in developmental disorders, parasitic infections, myopathy, and cancers. Our study demonstrates the important role of HDAC8 in immune cells by conditional targeting of HDAC8 in murine T cells and application of selective HDAC8 inhibitors. Using flow cytometry, RNA-seq, and ChIP-seq analyses, we demonstrate that knocking down or inhibiting HDAC8 impaired murine regulatory T cell (Treg) suppressive function in vitro and in vivo, but promoted conventional host T cell responses, thereby limiting syngeneic tumor growth. Mechanistically, HDAC8 knockout downregulated Foxp3 expression, enhanced H3K27 acetylation levels, and promoted IL-2, IL-6, Fas, and FasL expression in both Treg and conventional effector T cells. Thus, our combined genetic and pharmacologic studies establish the central importance of HDAC8 in T cell responses and suggest that selective HDAC8 inhibitors represent a potential therapeutic approach in immuno-oncology.

Authors

Fanhua Kong, Yan Xiong, Liqing Wang, Rongxiang Han, Hossein Fazelinia, Jennifer Roof, Lynn Spruce, Aaron B. Beeler, Wayne W. Hancock

×

Figure 5

Conditional deletion or inhibition of HDAC8 impaired Treg suppressive function in vivo and in vitro.

Options: View larger image (or click on image) Download as PowerPoint
Conditional deletion or inhibition of HDAC8 impaired Treg suppressive fu...
(A) Treg suppression assays using pooled Tregs and Teffs (n = 3/group) from lymph nodes and spleens of mice (CD4-Cre and HDAC8–/–), as indicated. (B and C) Treg suppression assays using pooled Tregs and Teffs (3 mice/ group) from lymph nodes and spleens of treated mice (DMSO and HDAC8i, n = 3/group), as indicated. (D) Immunodeficient Rag1–/– C57BL/6 murine recipients of BALB/c cardiac allografts were injected with conventional HDAC8–/– T effector cells (Teffs) plus Tregs (2:1 ratio), and treated with HDAC8i (OJI-1) 5 mg/kg/d for 14 days via Alzet pumps (n = 4/group). (E) Immunodeficient Rag1–/– mice were injected with conventional Teffs with and without Tregs and treated with HDAC8i (OJI-1, 5 mg/kg/d) for 7 days (n = 3/group). Assays were run in triplicate and repeated at least 3 times. The results of a representative experiment are shown. Data expressed as the mean ± SD of 3 independent experiments. *P < 0.05, **P < 0.01. NS, not significant. Comparisons between 2 groups utilized a 2-tailed Student’s t test for normally distributed data.