新型检查点激酶 1 抑制剂 SRA737 在肿瘤蛋白 53 基因状态不同的非小细胞肺癌和结直肠癌细胞中的应用研究

Q3 Medicine

Exploration of targeted anti-tumor therapy Pub Date : 2023-12-21 DOI:10.37349/etat.2023.00193

Ali Duabil, Christian R Cooper, E. Aldujaily, Sarah ER Halford, Sandra Hirschberg, Sidath D Katugampola, George DD Jones

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引用次数: 0

摘要

目的：DNA损伤时，丝氨酸/苏氨酸特异性蛋白激酶检查点激酶1（CHK1）被激活，使细胞进入S期（S）和G2期（G2）细胞周期停滞。CHK1抑制剂有望阻止细胞进入这种停滞期，从而增强DNA损伤诱导的细胞毒性。与此相反，共济失调性脊髓侧索硬化症突变体（ATM）、CHK2和肿瘤抑制蛋白53（P53）信号完好的正常细胞仍能利用正常的G1/S检查点进入细胞周期停滞期，从而从增强的细胞毒性中解救出来。这项工作的主要目的是研究新型 CHK1 抑制剂 SRA737 对非小细胞肺癌（NSCLC）和结直肠癌（CRC）细胞系的体外效应，这些细胞系都存在基因畸变，易受复制应激影响，但肿瘤蛋白 53（TP53）基因状态各不相同，重点是 DNA 损伤诱导以及随后对细胞增殖和活力的影响：方法：将 NSCLC 细胞株 H23 [TP53 突变体 (MUT)] 和 A549 [TP53 野生型 (WT)]，以及 CRC 细胞株 HT29 (TP53 突变体) 和 HCT116 (TP53 野生型) 与不同微摩尔浓度的 SRA737 培养 24 小时，然后使用碱性彗星和磷酸化 H2A.X 变异组蛋白 (γH2AX) - 病灶分析法分别评估大部分 DNA 单链断裂和双链断裂损伤。此外，还进行了细胞计数/特里潘蓝染色，以评估细胞的增殖/存活能力：结果：TP53 MUT 细胞的彗星形成率和γH2AX-病灶/细胞数明显增加，而相应的 TP53 WT 细胞则没有增加或增加较少。此外，与 TP53 WT 细胞相比，TP53 MUT 细胞具有更强的抗增殖和细胞杀伤作用：本研究的数据表明，P53 状态/功能是决定 NSCLC 和 CRC 癌细胞对 CHK1 抑制敏感性的关键因素，即使在有利于高复制应激的情况下也是如此。

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Investigations of the novel checkpoint kinase 1 inhibitor SRA737 in non-small cell lung cancer and colorectal cancer cells of differing tumour protein 53 gene status

Aim: In response to DNA damage the serine/threonine-specific protein kinase checkpoint kinase 1 (CHK1) is activated allowing cells to enter S phase (S) and G2 phase (G2) cell-cycle arrest. CHK1 inhibitors are expected to prevent cells from entering such arrest, thereby enhancing DNA damage-induced cytotoxicity. In contrast, normal cells with intact ataxia–telangiectasia mutated (ATM), CHK2 and tumour suppressor protein 53 (P53) signalling are still able to enter cell-cycle arrest using the functioning G1/S checkpoint, thereby being rescued from enhanced cytotoxicity. The main objective of this work is to investigate the in vitro effects of the novel CHK1 inhibitor SRA737 on pairs of non-small cell lung cancer (NSCLC) and colorectal cancer (CRC) cell lines, all with genetic aberrations rendering them susceptible to replication stress but of differing tumour protein 53 (TP53) gene status, focusing on DNA damage induction and the subsequent effects on cell proliferation and viability. Methods: NSCLC cell lines H23 [TP53 mutant (MUT)] and A549 [TP53 wild-type (WT)] and CRC cell lines HT29 (TP53 MUT) and HCT116 (TP53 WT) were incubated with differing micromolar concentrations of SRA737 for 24 h and then analysed using alkaline comet and phosphorylated H2A.X variant histone (γH2AX)-foci assays to assess mostly DNA single strand break and double strand break damage, respectively. Cell-counting/trypan blue staining was also performed to assess cell proliferation/viability. Results: Clear concentration-dependent increases in comet formation and γH2AX-foci/cell were noted for the TP53 MUT cells with no or lower increases being noted in the corresponding TP53 WT cells. Also, greater anti-proliferative and cell killing effects were noted in the TP53 MUT cells than in the TP53 WT cells. Conclusions: This study’s data suggests that P53 status/functioning is a key factor in determining the sensitivity of NSCLC and CRC cancer cells towards CHK1 inhibition, even in circumstances conducive to high replicative stress.

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Exploration of targeted anti-tumor therapy

CiteScore

2.80

自引率

0.00%

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审稿时长

13 weeks