Figure 4.
CLL cells from patients with disease progression on pirtobrutinib show increased BCR signaling, increased cytokine secretion, reduced inhibition of proliferation, reduced in vitro cell death, and increased cell viability. (A-J) Primary CLL cells obtained at baseline (day 0), responding, and progression time points during pirtobrutinib treatment were used in the analysis. (A) Western blots of lysates from CLL cells of 3 patients whose disease progressed, looking at total and phospho-BTK, total and phospho-ERK, total and phospho-AKT, and GAPDH without additional in vitro drug treatment. (B-C) Densitometry plots for phospho-BTK, phospho-ERK, and phospho-AKT normalized to the corresponding total protein. (D-E) Plasma CCL3 and CCL4 levels measured by Luminex multiplex assay and enzyme-linked immunosorbent assay, respectively. Data points in panels B to E are color coded by patient. (F) CLL cells at responding and progression time points for each of the 3 patients were incubated with indicated doses of pirtobrutinib for 48 hours and effect on viability was analyzed using CellTitre-Glo reagent. Data reported as mean ± standard error of the mean from n = 3. (G-J) Cells were cocultured with HS-5 green fluorescent protein stroma cells. (G-H) Apoptosis was induced by 1 μM pirtobrutinib for 48 hours and analyzed by flow cytometry. (I-J) CTV-labeled cells were stimulated to proliferate as described in “Methods” and incubated with or without 1 μM pirtobrutinib with proliferation analyzed by flow cytometry. Data in panels G-J represent mean from 3 technical replicates. Graphs generated using GraphPad Prism software version 9.3. Analysis of variance and paired t test were used to calculate significance. ∗P ≤ .05 and ∗∗P ≤ .01. Prog, progression; resp, responding.

CLL cells from patients with disease progression on pirtobrutinib show increased BCR signaling, increased cytokine secretion, reduced inhibition of proliferation, reduced in vitro cell death, and increased cell viability. (A-J) Primary CLL cells obtained at baseline (day 0), responding, and progression time points during pirtobrutinib treatment were used in the analysis. (A) Western blots of lysates from CLL cells of 3 patients whose disease progressed, looking at total and phospho-BTK, total and phospho-ERK, total and phospho-AKT, and GAPDH without additional in vitro drug treatment. (B-C) Densitometry plots for phospho-BTK, phospho-ERK, and phospho-AKT normalized to the corresponding total protein. (D-E) Plasma CCL3 and CCL4 levels measured by Luminex multiplex assay and enzyme-linked immunosorbent assay, respectively. Data points in panels B to E are color coded by patient. (F) CLL cells at responding and progression time points for each of the 3 patients were incubated with indicated doses of pirtobrutinib for 48 hours and effect on viability was analyzed using CellTitre-Glo reagent. Data reported as mean ± standard error of the mean from n = 3. (G-J) Cells were cocultured with HS-5 green fluorescent protein stroma cells. (G-H) Apoptosis was induced by 1 μM pirtobrutinib for 48 hours and analyzed by flow cytometry. (I-J) CTV-labeled cells were stimulated to proliferate as described in “Methods” and incubated with or without 1 μM pirtobrutinib with proliferation analyzed by flow cytometry. Data in panels G-J represent mean from 3 technical replicates. Graphs generated using GraphPad Prism software version 9.3. Analysis of variance and paired t test were used to calculate significance. P ≤ .05 and ∗∗P ≤ .01. Prog, progression; resp, responding.

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