![Figure 7. Effects of emTh-1 cells on antitumoral T lymphocytes and Tregs in vivo. (A) EmTh-1 plus CRCL immunotherapy induces tumor-specific killer T lymphocytes. B16 tumor–bearing mice were injected with control PBS or were treated with B16-derived CRCL and allogeneic emTh-1 cells as indicated in “Tumor growth in vivo and combination immunotherapy.” Seven days after the last vaccination, splenocytes were harvested and incubated for 3 days with CRCL (25 μg/mL) and 50 U/mL IL-2. T lymphocytes were then purified on a nylon wool column and incubated for 36 hours with either B16 tumor cells or irrelevant 4T1 breast cancer cell targets as indicated (effector T cells to target tumor cells ratio = 20:1). Cytotoxicity was determined as previously reported.28,50 + Control T, Tumor cells cultured with T lymphocytes from mice injected with PBS; +T [emTh-1], tumor cells cultured with T lymphocytes from mice treated with CRCL plus emTh-1. *P < .005, a significant difference compared with control T cells cultured with B16 melanoma cells. (B) EmTh-1 cells skew the differentiation of CD4+CD25−FoxP3− naive T lymphocytes toward CD4+CD25+FoxP3− effector T cells rather than Tregs in vivo. CD4+CD25−FoxP3− naive T lymphocytes isolated from Thy1.2 FoxP3EGFP transgenic BALB/c mice (107 cells) were transferred to 12B1 tumor–bearing congenic Thy1.1 BALB/c mice. Animals were treated with emTh-1 cells (+emTh-1 cells) or with control PBS (No emTh-1 cells). Endogenous T cells of recipient Thy1.1 mice express the Thy1.1 but not the Thy1.2 antigen, which allows the specific tracking and identification of Thy1.2 T lymphocytes in Thy1.1 mice. Spleens were harvested and dissociated, and conversion of transferred naive Thy1.2 CD4+CD25−FoxP3− T cells into GFP+ (FoxP3-expressing) Treg in vivo was determined by evaluating the frequency of Thy1.2+GFP+ cells after gating on the CD4+ T-cell population using flow cytometry. (C) EmTh-1 cells impair Treg suppressive function in vivo. Responder CD4+CD25− T lymphocytes were stimulated with anti-CD3/anti-CD28 T-cell expander beads in the absence (CD25−) or presence of Tregs isolated from the draining lymph nodes of untreated tumor-bearing mice (CD25− + [Treg]untreated) or of tumor-bearing mice treated with emTh-1 (CD25− + [Treg]emTh-1). Responder CD4+CD25− T-lymphocyte proliferation was determined after 48 hours using BrdU incorporation assays. NS, nonsignificant; *P < .02; **P < .001.](https://ash.silverchair-cdn.com/ash/content_public/journal/blood/117/5/10.1182_blood-2010-06-288621/4/zh89991065850007.jpeg?Expires=1723134584&Signature=zm~-JrN4zT11I8Wb8V~CvB7vBGz-eXexFtSt-TwFMkBDF5sMm8bjIUrlWCYXUdF3WToX3~9QVaaig8FQahG6j-6WJxLv8LM1LOJk1REeDSkJTSyDQcxNbXQs3r4~XfUwLehcQ7XPW3mbmX5khbLSnClfVDjaqyKJpPsLN1hes-DRJlWEFulNsIaPbnB9dqgAryyLnU4NkBdKKsOGomjyUqq0pGkawjO5yWf9bDuNrkPNUWCsixguDKiFEOGFgZXLuvPqZ9JwLTlbZR26-bv-tGx9ny2Ao0Aw-4WoVJtfnRv9r5RlDWXT6-Nwi~rWx0zU0rzqme6ABOEZ2QbX4bYXcw__&Key-Pair-Id=APKAIE5G5CRDK6RD3PGA)
Effects of emTh-1 cells on antitumoral T lymphocytes and Tregs in vivo. (A) EmTh-1 plus CRCL immunotherapy induces tumor-specific killer T lymphocytes. B16 tumor–bearing mice were injected with control PBS or were treated with B16-derived CRCL and allogeneic emTh-1 cells as indicated in “Tumor growth in vivo and combination immunotherapy.” Seven days after the last vaccination, splenocytes were harvested and incubated for 3 days with CRCL (25 μg/mL) and 50 U/mL IL-2. T lymphocytes were then purified on a nylon wool column and incubated for 36 hours with either B16 tumor cells or irrelevant 4T1 breast cancer cell targets as indicated (effector T cells to target tumor cells ratio = 20:1). Cytotoxicity was determined as previously reported.28,50 + Control T, Tumor cells cultured with T lymphocytes from mice injected with PBS; +T [emTh-1], tumor cells cultured with T lymphocytes from mice treated with CRCL plus emTh-1. *P < .005, a significant difference compared with control T cells cultured with B16 melanoma cells. (B) EmTh-1 cells skew the differentiation of CD4+CD25−FoxP3− naive T lymphocytes toward CD4+CD25+FoxP3− effector T cells rather than Tregs in vivo. CD4+CD25−FoxP3− naive T lymphocytes isolated from Thy1.2 FoxP3EGFP transgenic BALB/c mice (107 cells) were transferred to 12B1 tumor–bearing congenic Thy1.1 BALB/c mice. Animals were treated with emTh-1 cells (+emTh-1 cells) or with control PBS (No emTh-1 cells). Endogenous T cells of recipient Thy1.1 mice express the Thy1.1 but not the Thy1.2 antigen, which allows the specific tracking and identification of Thy1.2 T lymphocytes in Thy1.1 mice. Spleens were harvested and dissociated, and conversion of transferred naive Thy1.2 CD4+CD25−FoxP3− T cells into GFP+ (FoxP3-expressing) Treg in vivo was determined by evaluating the frequency of Thy1.2+GFP+ cells after gating on the CD4+ T-cell population using flow cytometry. (C) EmTh-1 cells impair Treg suppressive function in vivo. Responder CD4+CD25− T lymphocytes were stimulated with anti-CD3/anti-CD28 T-cell expander beads in the absence (CD25−) or presence of Tregs isolated from the draining lymph nodes of untreated tumor-bearing mice (CD25− + [Treg]untreated) or of tumor-bearing mice treated with emTh-1 (CD25− + [Treg]emTh-1). Responder CD4+CD25− T-lymphocyte proliferation was determined after 48 hours using BrdU incorporation assays. NS, nonsignificant; *P < .02; **P < .001.
