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SpiD3 modifies transcriptional profiles and subverts oncogenic pathways in CLL cells. A–D, RNA sequencing of OSU-CLL cells treated with SpiD3 (1, 2 µmol/L; 4 hours) or equivalent DMSO vehicle (VEH; n = 3 independent experiments). A, Hierarchical clustering of the top 500 differentially expressed genes (DEG) in SpiD3-treated cells (FDR B, GSEA of the top 500 DEGs in 2 µmol/L SpiD3-treated cells. C, Heat map of correlation between WGCNA module and the indicated treatment conditions. Each heat map cell displays the correlation coefficient (top) and corresponding P value (bottom). D, Volcano plot of SpiD3-treated cells (2 µmol/L) with select CLL-relevant genes labeled. Genes meeting both the statistical significance (FDR 2 FC| > 1) were used for downstream analysis (red). Genes meeting only statistical significance (blue), only fold-change (green), or neither threshold (gray) are shown for comparison. E, Representative immunoblots (n = 3 independent experiments) of the indicated proteins in SpiD3-treated OSU-CLL cells (4 hours). F, Cell cycle analysis of OSU-CLL cells treated with increasing amounts of SpiD3 (48 hours). BET inhibitor, JQ-1 (1 µmol/L), served as a positive control for cell cycle arrest (n = 5 independent experiments). Insert depicts a representative immunoblot for p21 expression following SpiD3 treatment (24 hours; n = 3 independent experiments). β-ACTIN served as the loading control. G, OSU-CLL cells were pretreated with 5 mmol/L N-acetylcysteine (NAC, 1 hour) followed by SpiD3 or VEH (24 hours). Pyocyanin (PYO, 1 mmol/L) served as a control ROS inducer (n = 3 independent experiments). Percent viability per condition is denoted below. Data are represented as mean ± SEM. Asterisks denote significance versus VEH: *, P P P
Eiken et al. (Wed,) studied this question.
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