麻疯树可以降低Hsp70的表达,从而减少蛋白折叠错误,促进正常蛋白在增殖和凋亡中的功能

A. Prayitno, M. S. Fitria, Elm, O. P. Astirin
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引用次数: 2

摘要

背景:麻疯树(jj . curcas)作为一种地方植物,具有抗炎和细胞毒性等植物化学成分。近十年来关于癌症的研究表明,热休克蛋白70 (Hsp70)的过度表达会导致错误折叠,并继续引发增殖和抑制细胞凋亡。Hsp70的表达增加导致蛋白质的错误折叠,并涉及导致疼痛发病的功能,包括癌症的发生。本研究检测了麻瓜处理Raji细胞后Hsp70、pRb和caspase3的表达。方法:先测定其含量。该植物是灌木状的,木质的,许多在热带地区被发现,命名为J.curcas sp.(大戟科)。第二步,从麻瓜中提取新鲜叶子,洗净,风干,切成小片,最后在65°C的烤箱中干燥48小时。第三,建立了Raji细胞培养(一种癌症模型)系统,并用麻瓜叶提取物处理细胞。四是免疫组化分析Hsp70、pRb和caspase-3的表达。光镜下采集半定量(低、中、强)数据。结果:我们的研究结果表明,麻叶提取物处理后的Raji细胞中Hsp70的表达较对照(14:46.60%)低9%(30.00%)。与对照(9:30.00%)相比,麻叶分体处理后pRb的表达量高15倍(50.00%)。caspase-3在Raji细胞中的表达比对照(9:30.00%)高13个百分点(43.3%)。结论:我们的研究结果表明,麻疯树叶可以降低Hsp70的表达,表明麻疯树叶也可以减少蛋白质折叠错误,促进正常的蛋白质功能,如增殖(通过抑制pRb蛋白表达)和凋亡(通过增强caspase-3蛋白表达)。
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Jatropha Curcas Linn can Reduce the Expression of Hsp70 that will Result in Reduced Errors in Protein Folding and Promotion of Normal Protein Function in Proliferation and Apoptosis
Background: Jatropha curcas (J. curcas) as a local plant have phytochemical contents like phenolic that effect as anti-inflammatory and cytotoxicity properties. Research in the last decade about cancers showed that over expression of heat shock protein 70 (Hsp70) does to mis-folding and continues to triggering proliferation and suppressing apoptosis. Increased expression of Hsp70 is responsible for mis-folding of proteins and implicated in functions that lead and play a role in the pathogenesis of pain including cancer incidence. In this study, we examined the expression of Hsp70, pRb and caspase3 in Raji cells after treatment with J. curcas. Methods: We first to determinethe plant. The plant is shrubby, woody and many are found in the tropics, names J.curcas sp. (Euphorbiaceae family). Second, to extraction of fresh leaves taken from J. curcas, washed clean, dried by the wind, sliced into small pieces and end dried by an oven at a temperature 65°C for 48 hours. And third, To developed a Raji cell culture (a cancer model) system and treated cells with fractionated extracts of J. curcas leaf. Fourth are evaluating the expression of Hsp70, pRb and caspase-3 that do by immuno histochemical analysis. A semi quantitative (devided into catagories: low, medium and strong) data was collected under light microscope view. Results: Our results showed that the expression of Hsp70 in Raji cells after treatment with fractionation J. curcas leaf was strong as much as 9(30.00%) lower than control (14:46.60%). The expression of pRb after treatment with fractionation J. curcas leaf was strong as much as 15(50.00%) higher than control (9:30.00%). And the expression of caspase-3 in Raji cells after treatment with fractionation J. curcas leaf was strong as much as 13(43.3%) higher than control (9:30.00%). Conclusion: Our results show that J. curcas leaf can reduce the expression of Hsp70, suggesting it can also reduce errors in protein folding and promotion of normal protein function in proliferation (by inhibit pRb protein expression) and apoptosis (by enhance caspase-3 protein expression).
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