不同浓度的含氯水溶性 C60 富勒烯衍生物对人胚胎肺成纤维细胞 (HELF) 基因表达选择性调控的剂量-反应效应。

IF 3.3 Q2 BIOCHEMISTRY & MOLECULAR BIOLOGY Frontiers in bioscience (Landmark edition) Pub Date : 2024-10-12 DOI:10.31083/j.fbl2910352
Svetlana V Kostyuk, Elena M Malinovskaya, Pavel E Umriukhin, Elena N Mikheeva, Elizaveta S Ershova, Ekaterina A Savinova, Larisa V Kameneva, Pavel A Troshin, Olga A Kraevaya, Ivan V Rodionov, Svetlana E Kostyuk, Tatyana A Salimova, Sergey I Kutsev, Natalia N Veiko
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引用次数: 0

摘要

背景:新合成的 C60 富勒烯水溶性衍生物引起了研究人员的极大兴趣,因为它们有可能成为药物输送、生物成像、生物降解和组织工程方面的理想材料。富勒烯衍生物的表面官能化改变了它们的化学和物理特性,增加了它们的溶解度,使其更适合不同的生物系统应用,然而,官能化富勒烯的任何变化都会改变它们的细胞毒性和抗氧化特性。富勒烯衍生物对细胞的毒性或保护作用是通过激活或抑制细胞中负责调节细胞活性氧(ROS)水平、增殖和凋亡的关键信号通路的基因和蛋白质来实现的:方法:采用 3-[4,5-二甲基噻唑-2-基]-2,5-二苯基溴化四氮唑(MTT)检测法评估细胞活力。流式细胞仪分析法用于测量人胚胎肺成纤维细胞(HELF)中的蛋白质水平。HELF 是一种标准、稳定和描述良好的人类细胞系,可以多次传代。使用 H2DCFH-DA 对 ROS 定量进行评估。荧光图像通过显微镜获得。使用实时聚合酶链反应(PCR)分析了 BCL2、CCND1、CDKN2A、BRCA1、BAX、NFKB1、NOX4、NRF2 和 TBP(参考基因)的表达:我们发现,高浓度和低浓度的富勒烯 C60 衍生物与 6-(3-苯基丙酰胺基)己酸钾盐(F1)或 6-(2-(噻吩-2-基)乙酰胺基)己酸钾盐(F2)的五个残基以及直接连接在笼子上的一个氯原子,会对 HELF 中调节氧化应激和细胞凋亡水平的关键信号通路的基因和蛋白质产生截然相反的激活作用。高浓度的 F1 和 F2 具有基因毒性作用,可在 24-72 小时内导致 NADPH 氧化酶 4(NOX4)表达激活(增加 2-4 倍)、ROS 合成诱导(增加 30-40%)、DNA 损伤和断裂(8-oxodG 水平增加 2-2.在 NF-E2 相关因子 2(NRF2)表达减少(20-45%)的背景下,活化 B 细胞的核因子卡巴轻链增强子(NF-κB)被激活(40-80%)。低浓度的 F1 和 F2 能产生细胞保护作用:在 24-72 小时内,它们能减少 DNA 的氧化损伤(20-40%),减少 DNA 双链断裂的数量(20-30%),提高抗凋亡蛋白的水平,增强激活 NRF2 表达的抗氧化反应(NRF2 基因表达增加 1.5-2.3 倍,NRF2 蛋白的磷酸化形式增加 2-3 倍):结论:研究结果表明,在低剂量情况下,所研究的富勒烯可作为 DNA 保护剂,抵御基因毒性因素的破坏。
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Dose-Response Effect of Various Concentrations of Cl-Containing Water-Soluble Derivatives of C60 Fullerenes on a Selective Regulation of Gene Expression in Human Embryonic Lung Fibroblasts (HELF).

Background: The new synthesized water-soluble derivatives of C60 fullerenes are of a great interest to researchers since they can potentially be promising materials for drug delivery, bioimaging, biosonding, and tissue engineering. Surface functionalization of fullerene derivatives changes their chemical and physical characteristics, increasing their solubility and suitability for different biological systems applications, however, any changes in functionalized fullerenes can modulate their cytotoxicity and antioxidant properties. The toxic or protective effect of fullerene derivatives on cells is realized through the activation or inhibition of genes and proteins of key signaling pathways in cells responsible for regulation of cellular reactive oxygen species (ROS) level, proliferation, and apoptosis.

Methods: The 3-[4,5-dimethylthiazol-2-yl]-2,5 diphenyl tetrazolium bromide (MTT) assay was used to assess cells viability. Flow cytometry analyses was applied to measure proteins levels in human embryonic lung fibroblasts (HELF) cells. HELF is a standard, stable and well described human cell line that can be passaged many times. Quantitation of ROS was assessed using H2DCFH-DA. Fluorescence images were obtained using microscopy. Expression of BCL2, CCND1, CDKN2A, BRCA1, BAX, NFKB1, NOX4, NRF2, TBP (reference gene) was analyzed using real-time Polymerase chain reaction (PCR).

Results: We found that high and low concentrations of fullerene C60 derivatives with the five residues of potassium salt of 6-(3-phenylpropanamido)hexanoic (F1) or 6-(2-(thiophen-2-yl)acetamido)hexanoic (F2) acid and a chlorine atom attached directly to the cage cause diametrically opposite activation of genes and proteins of key signaling pathways regulating the level of oxidative stress and apoptosis in HELF. High concentrations of F1 and F2 have a genotoxic effect, causing NADPH oxidase 4 (NOX4) expression activation in 24-72 hours (2-4 fold increase), ROS synthesis induction (increase by 30-40%), DNA damage and breaks (2-2.5 fold 8-oxodG level increases), and activation of nuclear factor kappa-light-chain-enhancer of activated B cells (NF-κB) (by 40-80%) against the background of reduced NF-E2-related factor 2 (NRF2) expression (by 20-45%). Low concentrations of F1 and F2 produced a cytoprotective effect: in 24-72 hours they reduce the oxidative DNA damage (by 20-40%), decrease the number of double-strand DNA breaks (by 20-30%), increase the level of anti-apoptotic proteins and enhance the antioxidant response activating the NRF2 expression (NRF2 gene expression increases 1.5-2.3 fold, phosphorylated form of the NRF2 protein increases 2-3 fold).

Conclusions: Obtained results show that in low doses studied fullrens may serve as perspective DNA protectors against the damaging genotoxic factors.

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