Figure 6.
Figure 6. Pharmacologic inhibition of IRE-1α/XBP-1 prevents cGVHD in MHC-matched BMT model. Lethally irradiated BALB/c recipients were transplanted with TCD-BM (5 × 106/mouse) from B10.D2 donors with (n = 30) or without (n = 4) whole splenocytes at 5 × 106/mouse. Groups were either given no treatment (n = 4), given daily IP injection of DMSO vehicle alone starting on day 0 and continued for 3 weeks (days 0-21; n = 10) or beginning on day 21 (days 21-42; n = 5), or IP injected with B-I09 at a dose of 25 mg/kg beginning at day 0 and continued for 3 weeks (days 0-21; n = 10), or beginning on day 21 (days 21-42; n = 5). Recipient mice were monitored for cGVHD clinical scores (A) until experiment endpoint on day 60. On day 45, images were taken of prophylactically treated vehicle and B-I09 groups (B). Skin biopsies were sectioned and stained with hematoxylin and eosin (magnification ×200) (C) and analyzed by an independent pathologist for signs of cGVHD skin damage (D). On day 60, mice were killed, and spleens and trunk skin were excised for processing into single-cell suspension for flow cytometric analysis of donor CD229.1− (Ly9.1−) CD4, CD8, and CD11c lymphocyte skin infiltrates (E). Quantification of CD4 (F), CD8 (G), and CD11c (H) cells in skin is shown. Splenic donor CD8+ T cells were analyzed via flow cytometry for expression of PD-1 (I). Data shown in panels A-C are representative of 2 separate experiments. Data shown in panel D are pooled from 2 replicate experiments. P < .05 indicates statistical significance. Data in panel E are representative flow plots from 2 separate experiments, which are quantified as pooled data in panels F-I. Statistical analysis of cGVHD clinical scores was performed using a Mann-Whitney U test of the entire experimental time course. P < .05 indicates statistical significance.

Pharmacologic inhibition of IRE-1α/XBP-1 prevents cGVHD in MHC-matched BMT model. Lethally irradiated BALB/c recipients were transplanted with TCD-BM (5 × 106/mouse) from B10.D2 donors with (n = 30) or without (n = 4) whole splenocytes at 5 × 106/mouse. Groups were either given no treatment (n = 4), given daily IP injection of DMSO vehicle alone starting on day 0 and continued for 3 weeks (days 0-21; n = 10) or beginning on day 21 (days 21-42; n = 5), or IP injected with B-I09 at a dose of 25 mg/kg beginning at day 0 and continued for 3 weeks (days 0-21; n = 10), or beginning on day 21 (days 21-42; n = 5). Recipient mice were monitored for cGVHD clinical scores (A) until experiment endpoint on day 60. On day 45, images were taken of prophylactically treated vehicle and B-I09 groups (B). Skin biopsies were sectioned and stained with hematoxylin and eosin (magnification ×200) (C) and analyzed by an independent pathologist for signs of cGVHD skin damage (D). On day 60, mice were killed, and spleens and trunk skin were excised for processing into single-cell suspension for flow cytometric analysis of donor CD229.1 (Ly9.1) CD4, CD8, and CD11c lymphocyte skin infiltrates (E). Quantification of CD4 (F), CD8 (G), and CD11c (H) cells in skin is shown. Splenic donor CD8+ T cells were analyzed via flow cytometry for expression of PD-1 (I). Data shown in panels A-C are representative of 2 separate experiments. Data shown in panel D are pooled from 2 replicate experiments. P < .05 indicates statistical significance. Data in panel E are representative flow plots from 2 separate experiments, which are quantified as pooled data in panels F-I. Statistical analysis of cGVHD clinical scores was performed using a Mann-Whitney U test of the entire experimental time course. P < .05 indicates statistical significance.

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