In vitro differentiated neutrophils from ECOMG cells were used as a model system to study nuclear architecture in response to calcium influx in neutrophils. ECOMG cells were cultured and differentiated as previously described (Zhu et al. 2017 (link)). For inhibitors, neutrophils were treated with 10 µM Triptolide (Cayman), 100 µM 5,6-dichloro-1-β-D-ribofuranosyl-1H-benzimidazole (Cayman) or 10 µM flavopiridol (Cayman) for 30 min, or 2 µM FK506 for 2 h before activation. Primary B cells were treated with 2 µM FK506 (Cayman) for 2 h before activation. Inhibitors were kept in culture during activation time course. Acute degradation was induced by treating the cells with 0.5 µM dTAG-13 (Tocris) before activation. dTAG-13 was kept in culture during activation time course. The time series degradation experiments were performed by inducing protein degradation at the beginning of the time course and harvesting the samples at different time points. RPMI-1640 (Gibco) contains 0.42 mM calcium. Additional CaCl2 was supplied to the medium before activation to a final concentration of 1 mM. A23187 was purchased from Sigma and Cayman. Neutrophils were activated either using fast activation conditions (20 µM A23187 for 15 min), or using slow activation conditions (5 µM A23187 for 4 h). These two activation conditions were used throughout the manuscript unless otherwise mentioned.
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Neutrophil Nuclear Architecture Modulation
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A23187
B cells
Benzimidazole
Calcium
Cayman
Fk506
Flavopiridol
Inhibitors
Model system
Neutrophils
Protein degradation
Triptolide
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- Inhibitors used: 10 µM Triptolide, 100 µM 5,6-dichloro-1-β-D-ribofuranosyl-1H-benzimidazole, 10 µM flavopiridol, 2 µM FK506
- Acute degradation induced by 0.5 µM dTAG-13
- Calcium concentration in the medium: 1 mM (additional CaCl2 added)
- Activation conditions: 20 µM A23187 for 15 min (fast), 5 µM A23187 for 4 h (slow)
- Nuclear architecture in response to calcium influx in neutrophils
- RPMI-1640 medium contains 0.42 mM calcium
- ECOMG cells were cultured and differentiated as previously described (Zhu et al. 2017)
- Primary B cells treated with 2 µM FK506 for 2 h before activation
- Not explicitly mentioned
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