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CD4+ follicular helper T cell infiltration predicts breast cancer survival
Chunyan Gu-Trantien, … , Christos Sotiriou, Karen Willard-Gallo
Chunyan Gu-Trantien, … , Christos Sotiriou, Karen Willard-Gallo
Published June 17, 2013
Citation Information: J Clin Invest. 2013;123(7):2873-2892. https://doi.org/10.1172/JCI67428.
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Research Article Oncology Article has an altmetric score of 27

CD4+ follicular helper T cell infiltration predicts breast cancer survival

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Abstract

CD4+ T cells are critical regulators of immune responses, but their functional role in human breast cancer is relatively unknown. The goal of this study was to produce an image of CD4+ T cells infiltrating breast tumors using limited ex vivo manipulation to better understand the in vivo differences associated with patient prognosis. We performed comprehensive molecular profiling of infiltrating CD4+ T cells isolated from untreated invasive primary tumors and found that the infiltrating T cell subpopulations included follicular helper T (Tfh) cells, which have not previously been found in solid tumors, as well as Th1, Th2, and Th17 effector memory cells and Tregs. T cell signaling pathway alterations included a mixture of activation and suppression characterized by restricted cytokine/chemokine production, which inversely paralleled lymphoid infiltration levels and could be reproduced in activated donor CD4+ T cells treated with primary tumor supernatant. A comparison of extensively versus minimally infiltrated tumors showed that CXCL13-producing CD4+ Tfh cells distinguish extensive immune infiltrates, principally located in tertiary lymphoid structure germinal centers. An 8-gene Tfh signature, signifying organized antitumor immunity, robustly predicted survival or preoperative response to chemotherapy. Our identification of CD4+ Tfh cells in breast cancer suggests that they are an important immune element whose presence in the tumor is a prognostic factor.

Authors

Chunyan Gu-Trantien, Sherene Loi, Soizic Garaud, Carole Equeter, Myriam Libin, Alexandre de Wind, Marie Ravoet, Hélène Le Buanec, Catherine Sibille, Germain Manfouo-Foutsop, Isabelle Veys, Benjamin Haibe-Kains, Sandeep K. Singhal, Stefan Michiels, Françoise Rothé, Roberto Salgado, Hugues Duvillier, Michail Ignatiadis, Christine Desmedt, Dominique Bron, Denis Larsimont, Martine Piccart, Christos Sotiriou, Karen Willard-Gallo

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Figure 3

Conventional Th subset marker expression in TIL.

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Conventional Th subset marker expression in TIL.
(A–C) Th subset marker ...
(A–C) Th subset marker genes were quantified in the patient confirmation set by (A and B) qRT-PCR and (C) flow cytometry. (A) Mean ΔCt values (relative to the Th-specific endogen CASC3) are inversely proportional to the relative intensity of gene expression; CD4+ TIL (n = 6) are compared with D-PB (n = 6). (B) CD4+ TIL from extensively infiltrated tumors (n = 6) are compared with minimally infiltrated tumors (n = 12). “n = <18” indicates that the number of minimally infiltrated tumors assessed was as noted. (C) Protein expression was assessed by flow cytometry (Supplemental Figure 2). (D–F) Microarray data from the patient discovery set and (G) qRT-pCR data of memory versus total CD4+ T cells from healthy donor cells are shown for comparison with (D) CD4+ T cells isolated from the first tissue (i.e., TIL) relative to the second tissue (i.e., P-PB), (E) CD4+ T cells isolated from ER– relative to ER+ tumors, (F) CD4+ T cells isolated from extensively infiltrated tumors relative to minimally infiltrated tumors, and (G) D-PB CD4+CD45RO+ memory T cells (n = 3) compared with total CD4+ T cells (n = 3). (H) Microarray data of D-PB memory CD4+ T cells after S or tumor SN treatment (Figure 6 and Supplemental Table 6). Fold change or ratio values are shown as blue (downregulated) and orange (upregulated); P values (2-tailed Student’s t test with unequal variance) in green are significant (P < 0.05); n.d., not determined (for qRT-PCR data no data = n.d.); nc, no change (for microarray data empty cells = nc). For gene symbols, “v” indicates transcript variant.

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ISSN: 0021-9738 (print), 1558-8238 (online)

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