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Non-invasive detection of DNA methylation states in carcinoma and pluripotent stem cells using Raman microspectroscopy and imaging

机译:使用拉曼微斑透视和成像的癌和多能干细胞中DNA甲基化状态的非侵入性检测

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DNA methylation plays a critical role in the regulation of gene expression. Global DNA methylation changes occur in carcinogenesis as well as early embryonic development. However, the current methods for studying global DNA methylation levels are invasive and require sample preparation. The present study was designed to investigate the potential of Raman microspectroscopy and Raman imaging?as non-invasive, marker-independent and non-destructive tools for the detection of DNA methylation in living cells. To investigate global DNA methylation changes, human colon carcinoma HCT116 cells, which were hypomorphic for DNA methyltransferase 1, therefore showing a lower global DNA methylation (DNMT1sup-/-/sup cells), were compared to HCT116 wildtype cells. As a model system for early embryogenesis, murine embryonic stem cells were adapted to serum-free 2i medium, leading to a significant decrease in DNA methylation. Subsequently, 2i?medium?-adapted cells were compared to cells cultured in serum-containing medium. Raman microspectroscopy and imaging revealed significant differences between high- and low-methylated cell types. Higher methylated cells demonstrated higher relative intensities of Raman peaks, which can be assigned to the nucleobases and 5-methylcytosine. Principal component analysis detected distinguishable populations of high- and low-methylated samples. Based on the provided data we conclude that Raman microspectroscopy and imaging are suitable tools for the real-time, marker-independent and artefact-free investigation of the DNA methylation states in living cells.
机译:DNA甲基化在基因表达的调节中起着关键作用。全局DNA甲基化变化发生在癌发生中以及早期胚胎发育中。然而,研究全球DNA甲基化水平的目前的方法是侵入性的并且需要样品制备。本研究旨在调查拉曼微型光谱和拉曼成像的潜力?作为无侵入性,标记无关和无损性的工具,用于检测活细胞中的DNA甲基化。为了研究全局DNA甲基化变化,将DNA甲基转移酶1的低晶体的人结肠癌HCT116细胞,因此显示与HCT116野生型细胞进行下全局DNA甲基化(DNMT1 - / -COM>细胞)。作为早期胚胎发生的模型系统,鼠胚胎干细胞适应无血清2I培养基,导致​​DNA甲基化的显着降低。随后,将2Iα-培养基细胞与在含血清培养基中培养的细胞进行比较。拉曼微穴位检查和成像显示出高甲基化细胞类型之间的显着差异。较高的甲基化细胞显示出拉曼峰的相对相对性,可以将其分配给核碱基和5-甲基胞嘧啶。主要成分分析检测到的高甲基化样品的可区分群体。基于所提供的数据,我们得出结论,拉曼微型光谱学和成像是用于实时,标记无关的和无遗体对活细胞中DNA甲基化状态的可自由制品的工具。

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