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DNA Methylation Changes in Valproic Acid-Treated HeLa Cells as Assessed by Image Analysis Immunofluorescence and Vibrational Microspectroscopy

机译:丙戊酸处理过的HeLa细胞中DNA甲基化变化的图像分析免疫荧光和振动显微光谱法进行了评估。

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摘要

Valproic acid (VPA), a well-known histone deacetylase inhibitor, has been reported to affect the DNA methylation status in addition to inducing histone hyperacetylation in several cell types. In HeLa cells, VPA promotes histone acetylation and chromatin remodeling. However, DNA demethylation was not checked in this cell model for standing effects longer than those provided by histone acetylation, which is a rapid and transient phenomenon. Demonstration of VPA-induced DNA demethylation in HeLa cells would contribute to understanding the effect of VPA on an aggressive tumor cell line. In the present work, DNA demethylation in VPA-treated HeLa cells was assessed by image analysis of chromatin texture, the abundance of 5-methylcytosine (5mC) immunofluorescence signals and Fourier transform-infrared (FT-IR) microspectroscopy centered on spectral regions related to the vibration of–CH3 groups. Image analysis indicated that increased chromatin unpacking promoted by a 4-h-treatment with 1.0 mM VPA persisted for 24 h in the absence of the drug, suggesting the occurrence of DNA demethylation that was confirmed by decreased 5mC immunofluorescence signals. FT-IR spectra of DNA samples from 1 mM or 20 mM VPA-treated cells subjected to a peak fitting analysis of the spectral window for–CH3 stretching vibrations showed decreased vibrations and energy of these groups as a function of the decreased abundance of 5mC induced by increased VPA concentrations. Only the 20 mM-VPA treatment caused an increase in the ratio of -CH3 bending vibrations evaluated at 1375 cm-1 in relation to in-plane vibrations of overall cytosines evaluated at 1492 cm-1. CH3 stretching vibrations showed to be more sensitive than–CH3 bending vibrations, as detected with FT-IR microspectroscopy, for studies aiming to associate vibrational spectroscopy and changes in DNA 5mC abundance.
机译:据报道,丙戊酸(VPA)是一种著名的组蛋白脱乙酰基酶抑制剂,除了在几种细胞类型中诱导组蛋白超乙酰化外,还影响DNA甲基化状态。在HeLa细胞中,VPA促进组蛋白乙酰化和染色质重塑。但是,在该细胞模型中,未检查DNA脱甲基化的持续作用时间长于组蛋白乙酰化所产生的持续作用,后者是一种快速且短暂的现象。在HeLa细胞中VPA诱导的DNA去甲基化的证明将有助于理解VPA对侵袭性肿瘤细胞系的影响。在目前的工作中,通过染色质构象,5-甲基胞嘧啶(5mC)免疫荧光信号的丰度和傅立叶变换红外(FT-IR)显微光谱的图像分析来评估VPA处理的HeLa细胞中的DNA去甲基化,该光谱集中于与CH3基团的振动。图像分析表明,在不存在药物的情况下,用1.0 mM VPA进行4 h处理后,染色质解包增加的现象持续了24 h,这表明DNA脱甲基现象的发生已被5mC免疫荧光信号降低所证实。从1 mM或20 mM VPA处理的细胞中进行了–CH3拉伸振动的光谱窗口的峰拟合分析的DNA样品的FT-IR光谱显示,这些组的振动和能量降低是5mC诱导的丰度降低的函数通过增加VPA浓度。只有20 mM-VPA处理导致在1375 cm -1 评估的-CH3弯曲振动的比例相对于在1492 cm -1评估的总胞嘧啶的平面内振动增加。 FT-IR显微光谱法检测到的CH3拉伸振动比–CH3弯曲振动更敏感,旨在进行振动光谱和DNA 5mC丰度变化的研究。

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