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Influence of components of tumour microenvironment on the response of HCT-116 colorectal cancer to the ruthenium-based drug NAMI-A

机译:肿瘤微环境组分对钌基药物NAMI-A对HCT-116结直肠癌响应的影响

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摘要

Solid tumours are constituted of tumour cells, healthy cells recruited from the host tissues and soluble factors released by both these cell types. The present investigation examines the capacity of co-cultures between the HCEC colon epithelial cells and the HCT-116 colorectal cancer cells (mimicking the primary site of tumour growth) and between IHH hepatocytes and the HCT-116 colorectal cancer cells (metastatic site) to influence the effects of NAMI-A (imidazolium trans-imidazoledimethylsulphoxidetetrachloro ruthenate) on the tumour cells themselves. The growth of HCT-116 cells is significantly influenced when the cancer cells are sown on a monolayer of HCEC. The release of soluble factors by the healthy cells promotes, in HCT-116 colorectal cancer cells, the transcription of genes involved in growth, invasion and migration. NAMI-A is not cytotoxic to HCT-116 cells grown on plastics or co-cultured with HCEC or IHH cells, and maintains its ability to control the cell pseudo-metastatic ability, mimicked by the migration in the scratch test. The effects of NAMI-A on HCT-116 migration are supported by its inhibition of the transcription of the ABL-2, ATF-3 and RND-1 genes. In conclusion the study highlights the need of test systems more complex than a single cancer cell culture to study an anticancer drug in vitro and reinforces the hypothesis that NAMI-A targets the ability of the cancer cell to interact with the tumour microenvironment and with the signals that support its metastatic ability.
机译:实体肿瘤由肿瘤细胞,从宿主组织中募集的健康细胞和通过这两种细胞类型释放的可溶性因子构成。本研究中检查的共培养的HCEC结肠上皮细胞和HCT-116结肠直肠癌细胞(模拟肿瘤生长的原发部位)之间的电容和IHH肝细胞和HCT-116结肠直肠癌细胞(转移部位)之间进行影响Nami-A(Imidazolium Trans-Imidazoledimethylerphusphorphorshloxidetthloro钌酸盐)对肿瘤细胞本身的影响。当癌细胞播种在HCEC的单层播种时,HCT-116细胞的生长显着影响。通过健康细胞释放可溶性因子在HCT-116结直肠癌细胞中,参与生长,侵袭和迁移的基因的转录。 NAMI-A不是在塑料中生长的HCT-116细胞的细胞毒性,或者用HCEC或IHH细胞共同培养,并保持其控制细胞伪转移能力的能力,通过划痕试验中的迁移模仿。通过抑制ABL-2,ATF-3和RND-1基因的转录,支持Nami-A对HCT-116迁移的影响。总之,该研究突出了测试系统的需求比单一癌细胞培养物更复杂,以研究抗癌药物体外,并增强Nami-A靶向癌细胞与肿瘤微环境相互作用的能力和信号的假设支持其转移能力。

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