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find Keyword "乏氧" 2 results
  • 恶性肿瘤放射增敏机制及药物研究进展

    放射治疗是恶性肿瘤治疗的有效方式之一,几乎超过50%的恶性肿瘤患者在抗癌过程中接受过放射治疗。但是高能量的放射线在杀死肿瘤细胞的同时,不可避免会损伤肿瘤周围正常组织。所以控制肿瘤放射剂量,使肿瘤放射“局部化”,是肿瘤科医生共同的追求。放射增敏剂的使用助于获得相对低量高效的放射剂量,有效增加肿瘤局部控制率,降低放射对肿瘤周围正常组织的伤害。但是目前临床上使用的放射增敏剂,大多数存在药物自身细胞毒性大、选择性低、价格昂贵等特点,限制了临床广泛使用。所以寻找安全经济且可区分肿瘤组织和正常组织的“智能型”放射增敏物质十分迫切且必要。这篇综述主要对肿瘤放射增敏机制及相关药物研究进展进行了总结分析,并介绍一些新兴的放射增敏措施,为临床上放射增敏剂的使用和进一步研发提供方向。

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  • Effect of HIF-1α on reverse differentiation of hepatocellular carcinoma cells in hypoxic environment

    ObjectiveTo explore the effects of hypoxia inducible factor-1 alpha (HIF-1α) on the reverse differentiation of hepatocellular carcinoma cells into liver cancer stem cells, and the maintenance of malignant biological behavior in hypoxic environment.MethodsCD133-negative cells in HepG2 cells were separated by immunomagnetic beads and divided into two groups. The cells of siRNA group were transfected with siRNA-HIF-1α to silence the expression of HIF-1α gene, while cells of the blank control group did not transfect any siRNA fragments. The two groups of cells were cultured under normal and hypoxic conditions respectively. MTT, cloning and Transwell chamber experiments were used to detect the proliferation and invasion ability of cells. Western blot and real-time PCR (RT-PCR) were used to detect the expressions of HIF-1α, CD133, CD90, and CD44 protein and mRNA in cells.ResultsMTT results showed that the cell proliferation rate increased with the prolongation of hypoxia in four groups. Compared with the blank control group at 24, 32, 40, and 48 hours, the cell proliferation rate decreased significantly after siRNA-HIF-1a transfection, on both two kinds of cultured conditions (P<0.05). The results of plate cloning experiment showed that the number of cell-forming clones increased significantly after hypoxic culture (there were significant differences between the transfected normoxic group and transfected hypoxic group, blank control normoxic group and blank control hypoxic group, P<0.05); and the formation of transfected hypoxic condition group at the same time of hypoxia was also significant (P<0.05). The number of clones were significantly less than that of the blank control group at the hypoxic condition (P<0.05). Transwell lab experiment showed that after hypoxic culture, the number of cells migrated to the inferior chamber in the transfection group was significantly reduced compared with that of the blank control group (P<0.05). Western blot and RT-PCR results showed that the expression levels of HIF-1α protein and tumor stem cell markers (CD133, CD90, and CD44 protein) in the blank control hypoxic condition group were significantly higher than those in the other three groups (P<0.05); after siRNA-HIF-1a transfection, HIF-1α mRNA and tumor stem cell markers mRNA (CD133, CD90, and CD44 mRNA) in the transfected hypoxic condition group were significantly lower than those in the transfected normal condition group and the blank control normal condition group (P<0.05).ConclusionsIn hypoxia environment, HIF-1α can promote hepatocellular carcinoma cells to differentiate into liver cancer stem cells and enhance their malignant biological behavior.

    Release date:2019-01-16 10:05 Export PDF Favorites Scan
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