![ZAP-70 contributes to the constitutive phosphorylation of AKT and GSK3β in IGHV–unmutated CLL cells. (A) Representative kinetic blots show the calcium flux of IGHV–unmutated (UM-CLL) or IGHV–mutated (M-CLL) CLL cells with NSC or ZAP-70 siRNA transfection. CLL cells were harvested and labeled with Fluo-4 (fluorescein isothiocyanate). BCR-signaling was activated with anti-IgM beads, triggered 20 to 30 seconds after flow cytometric measurement started. (B) Quantification of calcium flux response of CLL samples (n = 4 for both UM-CLL and M-CLL) transfected with NSC or ZAP-70 siRNA. The Ca2+ ratios were calculated by using kinetic blots and divided peak Fluo-4 (FITC-A) mean intensity upon anti-IgM activation by baseline. (C) Phospho-AKT (T308), phospho-AKT (S473), total AKT, ZAP-70, and β-actin immunoblots of primary M-CLL cells monocultured for 24 hours after nonspecific control siRNA or ZAP-70 siRNA transfection. For anti-IgM stimulated samples, CLL cells were treated with beads-bound anti-IgM for 20 minutes. (D) Phosphorylated protein levels of AKT (relative to total AKT levels) 24 hours after siRNA transfection in M-CLL samples. For anti-IgM stimulated samples, monocultured M-CLL cells were treated with beads-bound anti-IgM for 20 minutes (n = 4 for pi-AKT [T-308] and n = 3 for pi-AKT [S473]). (E) Phospho-GSK-3β (S9), total GSK-3β, ZAP-70, and β-actin immunoblots of primary UM-CLL or M-CLL cells monocultured for 24 hours after nonspecific control siRNA or ZAP-70 siRNA transfection. For anti-IgM stimulated samples, monocultured CLL cells were treated with beads-bound anti-IgM for 20 minutes. (F) Phosphorylated GSK-3β levels (relative to total GSK-3β levels) 24 hours after siRNA transfection in UM-CLL and M-CLL samples. For anti-IgM stimulated samples, monocultured CLL cells were treated with beads-bound anti-IgM for 20 minutes (n = 3 for both UM-CLL and M-CLL). (G) Cell viability of primary CLL cells assessed using annexin-V/propidium iodide staining, 9 days after siRNA transfection. Cells were monocultured for 48 hours after nonspecific control siRNA or ZAP-70 siRNA transfection for 7 days on stromal cells. (H) MCL1 and β-actin immunoblots of primary UM-CLL cells cultured under identical conditions as described in panel G. (I) Relative MCL1 protein level (compared to with β-actin levels) 24 hours after siRNA transfection in UM-CLL samples (n = 3). Statistical significance between samples was assessed by paired 2-tailed Student t tests. ∗P < 5 × 10−2, ∗∗∗P < 10−4. LE, long exposure; ns, not significant; NSC, non-specific control; SE, short exposure.](https://ash.silverchair-cdn.com/ash/content_public/journal/bloodadvances/8/5/10.1182_bloodadvances.2022009557/2/blooda_adv-2022-009557-gr1.jpeg?Expires=1724246483&Signature=abYvuAGaur0YKQLEABIDxyyfidzs0w2W1bXNM059HPOV4H6w-ofWO8KAD8vPnmT6zc4FWLB5wiqjeIWA-uAYRwHvj38dHFzZMjznOkG00vBP7i1offEbxsecH5fNke0afdmVVRfroGaa6O7Hxv45j8jK2PAFq0p9nT9VJbaOvZExw33gyCHL-E9zfmS4c9LUWrMlz46Xmajnnj2eFFhef~HjDw08J687A9~xfLvR8rTL77nL5n8NDDy1yHHEZ83M8Dzn2LrdkYiVA3Js2DnhvKUidXqMNUxKNnqkHg1TmNjqtshIgO4SuPI0h90URgqlOfS1wquaXtNQQEWT5YlR5w__&Key-Pair-Id=APKAIE5G5CRDK6RD3PGA)
ZAP-70 contributes to the constitutive phosphorylation of AKT and GSK3β in IGHV–unmutated CLL cells. (A) Representative kinetic blots show the calcium flux of IGHV–unmutated (UM-CLL) or IGHV–mutated (M-CLL) CLL cells with NSC or ZAP-70 siRNA transfection. CLL cells were harvested and labeled with Fluo-4 (fluorescein isothiocyanate). BCR-signaling was activated with anti-IgM beads, triggered 20 to 30 seconds after flow cytometric measurement started. (B) Quantification of calcium flux response of CLL samples (n = 4 for both UM-CLL and M-CLL) transfected with NSC or ZAP-70 siRNA. The Ca2+ ratios were calculated by using kinetic blots and divided peak Fluo-4 (FITC-A) mean intensity upon anti-IgM activation by baseline. (C) Phospho-AKT (T308), phospho-AKT (S473), total AKT, ZAP-70, and β-actin immunoblots of primary M-CLL cells monocultured for 24 hours after nonspecific control siRNA or ZAP-70 siRNA transfection. For anti-IgM stimulated samples, CLL cells were treated with beads-bound anti-IgM for 20 minutes. (D) Phosphorylated protein levels of AKT (relative to total AKT levels) 24 hours after siRNA transfection in M-CLL samples. For anti-IgM stimulated samples, monocultured M-CLL cells were treated with beads-bound anti-IgM for 20 minutes (n = 4 for pi-AKT [T-308] and n = 3 for pi-AKT [S473]). (E) Phospho-GSK-3β (S9), total GSK-3β, ZAP-70, and β-actin immunoblots of primary UM-CLL or M-CLL cells monocultured for 24 hours after nonspecific control siRNA or ZAP-70 siRNA transfection. For anti-IgM stimulated samples, monocultured CLL cells were treated with beads-bound anti-IgM for 20 minutes. (F) Phosphorylated GSK-3β levels (relative to total GSK-3β levels) 24 hours after siRNA transfection in UM-CLL and M-CLL samples. For anti-IgM stimulated samples, monocultured CLL cells were treated with beads-bound anti-IgM for 20 minutes (n = 3 for both UM-CLL and M-CLL). (G) Cell viability of primary CLL cells assessed using annexin-V/propidium iodide staining, 9 days after siRNA transfection. Cells were monocultured for 48 hours after nonspecific control siRNA or ZAP-70 siRNA transfection for 7 days on stromal cells. (H) MCL1 and β-actin immunoblots of primary UM-CLL cells cultured under identical conditions as described in panel G. (I) Relative MCL1 protein level (compared to with β-actin levels) 24 hours after siRNA transfection in UM-CLL samples (n = 3). Statistical significance between samples was assessed by paired 2-tailed Student t tests. ∗P < 5 × 10−2, ∗∗∗P < 10−4. LE, long exposure; ns, not significant; NSC, non-specific control; SE, short exposure.
