Figure 2
Figure 2. MSCs can provide survival support to CLL cells in vitro. (A) CLL cells were cultured in the presence of increasing concentrations of MSC conditioned media (CM), which was prepared in 5% O2, and exposed to either 21% or 5% O2 for 3 days, at which point the CLL cells were collected for viability measurements by flow cytometry. Data from 4 different CLL patients are presented (mean ± SEM), which were normalized to day 0. The initial absolute viability of all samples at day 0 was of 66% ± 6% (mean ± SEM). Asterisks indicate significant difference between CM conditions and media control values in 5% O2 and 21% O2 (1-way ANOVA and Tukey posthoc test; ***P < .001, **P < .01, *P < .05). (B) CLL cells were cultured for 3 days in the presence of increasing amounts of MSC CM, which was prepared by incubating MSCs either in 5% O2 or 21% O2 for 6 days. CLL-cell viability was assessed by flow cytometry. Data on cells obtained from each of 3 different CLL patients are presented (mean ± SEM), which were normalized to day 0. The initial absolute viability of all samples at day 0 was of 87% ± 2% (mean ± SEM). Asterisks indicate significant difference measured by 1-way ANOVA and Tukey posthoc test (**P < .01, *P < .05). (C) The presence of CXCL12 was quantified in MSC CM prepared by incubating MSCs either in 5% O2 or 21% O2 for 6 days by ELISA. Left: CXCL12 concentration in the CM; right: CXCL12 secretion rate per 1 × 105 MSCs was estimated by dividing CXCL12 concentration in the CM by the number of MSCs collected at the end of the 6-day culture period. The data presented were obtained from MSCs derived from each of 2 patients, each tested in 2 independent experiments (mean ± SEM). Asterisks indicate significant difference measured by Student t test. (*P < .05). (D) CXCR4 expression levels on CLL cells (n = 6) cultured for 24 hours in 5% or 21% O2 were assessed by flow cytometry, which was gated on CD19PosCD5Pos cells. CXCR4 expression is presented as the absolute mean fluorescence intensity (MFI), which was the MFI of CD19+CD5+ cells stained for CXCR4 minus the MFI of the same cells stained with an isotype control antibody. Student t test was used to determine statistical significance. (E-F) MSCs generated in 5% O2 were plated in parallel cultures at 1000 cells/cm2 and subsequently placed in 5% or 21% O2 for 2 to 3 days before the addition of CLL cells (1 × 106 cells/mL). CLL cells from 4 different patients (3 ZAP-70Neg, 1 ZAP-70Pos) were seeded in duplicate either alone, directly on MSCs (E), or separated from the MSCs by transwell (TW) porous membrane (0.4 μm; F). CLL-cell viability was assessed after 0, 3, 6, 10, or 14 days and normalized to that of the cells on day 0 (mean ± SEM; n = 4). The initial absolute viability of all samples at day 0 was of 74% ± 5% (mean ± SEM). In panel E an asterisk indicates the significant difference between the percentage live CLL cells on MSCs in 21% O2 and 5% O2 (Student t test; P < .05). In panel F asterisks (*) or (**) indicate a P < .05 or P < .01, respectively (Student t test) for the differences between CLL cells cultured alone or with MSCs. (G) CLL cells from 4 different patients (3 ZAP-70Neg and 1 ZAP-70Pos) were cocultured with MSCs that were derived from 2 different ZAP-70Neg patients (bottom) or 2 ZAP-70Pos CLL patients (top) for 14 days, at which point the cells were collected for viability assessment by flow cytometry. The viability data presented have been normalized to day 0 (mean ± SEM). The initial absolute viability of all samples at day 0 was 74% ± 6% for the 4 samples plated on MSCs from ZAP-70Pos patients, and of 73% ± 10% for the 4 samples plated on MSCs from ZAP-70Neg patients (mean ± SEM). Asterisks indicate significant difference measured by Student t test. (*P < .05; **P < .01).

MSCs can provide survival support to CLL cells in vitro. (A) CLL cells were cultured in the presence of increasing concentrations of MSC conditioned media (CM), which was prepared in 5% O2, and exposed to either 21% or 5% O2 for 3 days, at which point the CLL cells were collected for viability measurements by flow cytometry. Data from 4 different CLL patients are presented (mean ± SEM), which were normalized to day 0. The initial absolute viability of all samples at day 0 was of 66% ± 6% (mean ± SEM). Asterisks indicate significant difference between CM conditions and media control values in 5% O2 and 21% O2 (1-way ANOVA and Tukey posthoc test; ***P < .001, **P < .01, *P < .05). (B) CLL cells were cultured for 3 days in the presence of increasing amounts of MSC CM, which was prepared by incubating MSCs either in 5% O2 or 21% O2 for 6 days. CLL-cell viability was assessed by flow cytometry. Data on cells obtained from each of 3 different CLL patients are presented (mean ± SEM), which were normalized to day 0. The initial absolute viability of all samples at day 0 was of 87% ± 2% (mean ± SEM). Asterisks indicate significant difference measured by 1-way ANOVA and Tukey posthoc test (**P < .01, *P < .05). (C) The presence of CXCL12 was quantified in MSC CM prepared by incubating MSCs either in 5% O2 or 21% O2 for 6 days by ELISA. Left: CXCL12 concentration in the CM; right: CXCL12 secretion rate per 1 × 105 MSCs was estimated by dividing CXCL12 concentration in the CM by the number of MSCs collected at the end of the 6-day culture period. The data presented were obtained from MSCs derived from each of 2 patients, each tested in 2 independent experiments (mean ± SEM). Asterisks indicate significant difference measured by Student t test. (*P < .05). (D) CXCR4 expression levels on CLL cells (n = 6) cultured for 24 hours in 5% or 21% O2 were assessed by flow cytometry, which was gated on CD19PosCD5Pos cells. CXCR4 expression is presented as the absolute mean fluorescence intensity (MFI), which was the MFI of CD19+CD5+ cells stained for CXCR4 minus the MFI of the same cells stained with an isotype control antibody. Student t test was used to determine statistical significance. (E-F) MSCs generated in 5% O2 were plated in parallel cultures at 1000 cells/cm2 and subsequently placed in 5% or 21% O2 for 2 to 3 days before the addition of CLL cells (1 × 106 cells/mL). CLL cells from 4 different patients (3 ZAP-70Neg, 1 ZAP-70Pos) were seeded in duplicate either alone, directly on MSCs (E), or separated from the MSCs by transwell (TW) porous membrane (0.4 μm; F). CLL-cell viability was assessed after 0, 3, 6, 10, or 14 days and normalized to that of the cells on day 0 (mean ± SEM; n = 4). The initial absolute viability of all samples at day 0 was of 74% ± 5% (mean ± SEM). In panel E an asterisk indicates the significant difference between the percentage live CLL cells on MSCs in 21% O2 and 5% O2 (Student t test; P < .05). In panel F asterisks (*) or (**) indicate a P < .05 or P < .01, respectively (Student t test) for the differences between CLL cells cultured alone or with MSCs. (G) CLL cells from 4 different patients (3 ZAP-70Neg and 1 ZAP-70Pos) were cocultured with MSCs that were derived from 2 different ZAP-70Neg patients (bottom) or 2 ZAP-70Pos CLL patients (top) for 14 days, at which point the cells were collected for viability assessment by flow cytometry. The viability data presented have been normalized to day 0 (mean ± SEM). The initial absolute viability of all samples at day 0 was 74% ± 6% for the 4 samples plated on MSCs from ZAP-70Pos patients, and of 73% ± 10% for the 4 samples plated on MSCs from ZAP-70Neg patients (mean ± SEM). Asterisks indicate significant difference measured by Student t test. (*P < .05; **P < .01).

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