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Acute effect of lactic acid on tumor-endothelial cell metabolic coupling in the tumor microenvironment

机译:乳酸对肿瘤微环境中肿瘤-内皮细胞代谢偶联的急性影响

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摘要

The present study aimed to systematically analyze alterations in the expression of mitochondrial-associated proteins in human bladder cancer T24 cells co-cultured with tumor-associated human umbilical vein endothelial cells (HUVECs), and to investigate the characteristics of bladder cancer cell energy metabolism. The present study used the following techniques: A co-culture system of T24 cells and HUVECs was constructed using a microfluidic chip as a 3D co-culture system; the concentration of lactic acid in the medium of the cells was determined using an automatic microplate reader; a qualitative analysis of mitochondria-associated protein expression was performed by immunofluorescent staining; and a quantitative analysis of mitochondrial-associated protein expression was conducted using western blotting. The present results revealed that between the control groups (monoculture of T24 cells or HUVECs), the mitochondrial-associated protein fluorescence intensity was increased in the HUVECs compared with the T24 cells. The fluorescence intensity of mitochondrial-associated proteins in the HUVEC control group was increased compared with the HUVECs in the experimental co-culture group. In the T24 cells, the protein fluorescence intensity was increased in the experimental co-culture group compared with the control group. In addition, the expression of mitochondria-associated proteins was increased in HUVECs compared with T24 cells in the control groups, while T24 cells in the experimental co-culture group had an increased expression compared with HUVECs in the experimental group (P<0.05). For T24 cells, the expression of mitochondrial-associated proteins was increased in the experimental group compared with the control group, and contrasting results were observed for the HUVECs (P<0.05). Determination of lactic acid concentration demonstrated that lactic acid concentration was highest in the experimental co-culture group, followed by the T24 control group and the HUVEC control group. In conclusion, the present study demonstrated that energy metabolism of the bladder tumor cells does not parallel the ‘Warburg effect’, since even under sufficient oxygen conditions the tumor cells still undergo glycolysis. Additionally, bladder tumor cells have an efficient oxidative phosphorylation process, wherein tumor cells promote glycolysis in adjacent interstitial cells, thereby causing increased formation of nutritional precursors. These high-energy metabolites are transferred to adjacent tumor cells in a specified direction and enter the Krebs Cycle. Ultimately, oxidative phosphorylation increases, and sufficient ATP is produced.
机译:本研究旨在系统分析线粒体相关蛋白在与肿瘤相关人脐静脉内皮细胞(HUVEC)共培养的人膀胱癌T24细胞中的表达变化,并研究膀胱癌细胞能量代谢的特征。本研究使用以下技术:使用微流体芯片作为3D共培养系统,构建T24细胞和HUVEC的共培养系统;用自动酶标仪测定细胞培养基中乳酸的浓度。通过免疫荧光染色对线粒体相关蛋白表达进行定性分析。使用蛋白质印迹法对线粒体相关蛋白的表达进行定量分析。本结果表明,在对照组之间(T24细胞或HUVEC的单培养),与T24细胞相比,HUVEC中线粒体相关蛋白的荧光强度增加。与实验共培养组的HUVEC相比,HUVEC对照组的线粒体相关蛋白的荧光强度增加。在T24细胞中,与对照组相比,实验共培养组的蛋白质荧光强度增加。另外,与对照组的T24细胞相比,HUVECs中的线粒体相关蛋白表达增加,而实验共培养组的T24细胞与HUVECs相比,表达水平增加(P <0.05)。对于T24细胞,与对照组相比,实验组中线粒体相关蛋白的表达增加,并且观察到HUVEC的对比结果(P <0.05)。乳酸浓度的测定表明,在实验共培养组中乳酸浓度最高,其次是T24对照组和HUVEC对照组。总之,本研究表明,膀胱肿瘤细胞的能量代谢与“ Warburg效应”不相符,因为即使在充足的氧气条件下,肿瘤细胞仍会发生糖酵解。另外,膀胱肿瘤细胞具有有效的氧化磷酸化过程,其中肿瘤细胞促进相邻间质细胞中的糖酵解,从而导致营养前体的形成增加。这些高能代谢物沿指定方向转移到相邻的肿瘤细胞,并进入克雷布斯循环。最终,氧化磷酸化增加,并产生足够的ATP。

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