chk1 抑制物可强烈阻断人多发性骨髓瘤细胞中 stat3 酪氨酸 705 的磷酸化、dna 结合活性和下游靶基因的激活。
Chk1 Inhibition Potently Blocks STAT3 Tyrosine705 Phosphorylation, DNA-Binding Activity, and Activation of Downstream Targets in Human Multiple Myeloma Cells.
机构信息
Division of Hematology/Oncology, Department of Medicine, Virginia Commonwealth University, Richmond, Virginia.
Division of Molecular Diagnostics, Department of Pathology, Virginia Commonwealth University, Richmond, Virginia.
出版信息
Mol Cancer Res. 2022 Mar 1;20(3):456-467. doi: 10.1158/1541-7786.MCR-21-0366.
UNLABELLED
The relationship between the checkpoint kinase Chk1 and the STAT3 pathway was examined in multiple myeloma cells. Gene expression profiling of U266 cells exposed to low (nmol/L) Chk1 inhibitor [PF-477736 (PF)] concentrations revealed STAT3 pathway-related gene downregulation (e.g., BCL-XL, MCL-1, c-Myc), findings confirmed by RT-PCR. This was associated with marked inhibition of STAT3 Tyr705 (but not Ser727) phosphorylation, dimerization, nuclear localization, DNA binding, STAT3 promoter activity by chromatin immunoprecipitation assay, and downregulation of STAT-3-dependent proteins. Similar findings were obtained in other multiple myeloma cells and with alternative Chk1 inhibitors (e.g., prexasertib, CEP3891). While PF did not reduce GP130 expression or modify SOCS or PRL-3 phosphorylation, the phosphatase inhibitor pervanadate antagonized PF-mediated Tyr705 dephosphorylation. Significantly, PF attenuated Chk1-mediated STAT3 phosphorylation in in vitro assays. Surface plasmon resonance analysis suggested Chk1/STAT3 interactions and PF reduced Chk1/STAT3 co-immunoprecipitation. Chk1 CRISPR knockout or short hairpin RNA knockdown cells also displayed STAT3 inactivation and STAT3-dependent protein downregulation. Constitutively active STAT3 diminished PF-mediated STAT3 inactivation and downregulate STAT3-dependent proteins while significantly reducing PF-induced DNA damage (γH2A.X formation) and apoptosis. Exposure of cells with low basal phospho-STAT3 expression to IL6 or human stromal cell conditioned medium activated STAT3, an event attenuated by Chk1 inhibitors. PF also inactivated STAT3 in primary human CD138+ multiple myeloma cells and tumors extracted from an NSG multiple myeloma xenograft model while inhibiting tumor growth.
IMPLICATIONS
These findings identify a heretofore unrecognized link between the Chk1 and STAT3 pathways and suggest that Chk1 pathway inhibitors warrant attention as novel and potent candidate STAT3 antagonists in myeloma.
未加标签
研究人员在多发性骨髓瘤细胞中检查了检查点激酶 Chk1 和 STAT3 通路之间的关系。对暴露于低浓度(nmol/L)Chk1 抑制剂[PF-477736(PF)]的 U266 细胞进行基因表达谱分析,揭示了 STAT3 通路相关基因下调(例如,BCL-XL、MCL-1、c-Myc),这一发现通过 RT-PCR 得到证实。这与 STAT3 Tyr705(而非 Ser727)磷酸化的显著抑制、二聚化、核定位、DNA 结合、染色质免疫沉淀测定中的 STAT3 启动子活性以及 STAT-3 依赖性蛋白的下调有关。在其他多发性骨髓瘤细胞和替代 Chk1 抑制剂(例如,prexasertib、CEP3891)中也获得了类似的发现。虽然 PF 不会降低 GP130 表达或改变 SOCS 或 PRL-3 磷酸化,但磷酸酶抑制剂过钒酸钠拮抗 PF 介导的 Tyr705 去磷酸化。重要的是,PF 在体外测定中减弱了 Chk1 介导的 STAT3 磷酸化。表面等离子体共振分析表明 Chk1/STAT3 相互作用,PF 减少了 Chk1/STAT3 共免疫沉淀。Chk1 CRISPR 敲除或短发夹 RNA 敲低细胞也显示出 STAT3 失活和 STAT3 依赖性蛋白下调。组成性激活的 STAT3 减弱了 PF 介导的 STAT3 失活和下调 STAT3 依赖性蛋白,同时显著减少 PF 诱导的 DNA 损伤(γH2A.X 形成)和凋亡。将低基础磷酸化 STAT3 表达的细胞暴露于 IL6 或人基质细胞条件培养基中激活了 STAT3,这一事件被 Chk1 抑制剂减弱。PF 还在原发性人 CD138+多发性骨髓瘤细胞和从 NSG 多发性骨髓瘤异种移植模型中提取的肿瘤中失活了 STAT3,同时抑制了肿瘤生长。
意义
这些发现确定了 Chk1 和 STAT3 通路之间以前未被识别的联系,并表明 Chk1 途径抑制剂值得关注,作为骨髓瘤中新型和有效的候选 STAT3 拮抗剂。
Zotero 插件