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Shedding New Light on the Molecular Architecture of Oocytes Using a Combination of Synchrotron Fourier Transform-Infrared and Raman Spectroscopic Mapping

机译:同步加速器傅里叶变换红外和拉曼光谱映射相结合为卵母细胞的分子结构提供了新的思路

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Synchrotron Fourier transform-infrared (FT-IR) and Raman microspectroscopy were applied to investigate changes in the molecular architecture of mouse oocytes and demonstrate the overall morphology of the maturing oocyte. Here we show that differences were identified between immature mouse oocytes at the germinal vesicle (GV) and mature metaphase II (MII) stage when using this technology, without the introduction of any extrinsic markers, labels, or dyes. GV mouse oocytes were found to have a small, centrally located lipid deposit and another larger polar deposit of similar composition. MII oocytes have very large, centrally located lipid deposits. Each lipid deposit for both cell types contains an inner and outer lipid environment that differs in composition. To assess interoocyte variability, line scans were recorded across the diameter of the oocytes and compared from three independent trials (GV, n velence 91; MII, n velence 172), and the data were analyzed with principal component analysis (PCA). The average spectra and PCA loading plots show distinct and reproducible changes in the CH stretching region that can be used as molecular maturation markers. The method paves the way for developing an independent assay to assess oocyte status during maturation providing new insights into lipid distribution at the single cell level.
机译:同步加速傅立叶变换红外(FT-IR)和拉曼光谱技术用于研究小鼠卵母细胞分子结构的变化,并证明了成熟卵母细胞的整体形态。在这里,我们显示了使用此技术时,在未引入任何外部标记,标记或染料的情况下,已确定在生小泡(GV)和成熟中期II(MII)阶段的未成熟小鼠卵母细胞之间存在差异。发现GV小鼠卵母细胞有一个小的,位于中心的脂质沉积物和另一个较大的极性沉积物,具有相似的组成。 MII卵母细胞具有非常大的位于中央的脂质沉积物。两种细胞类型的每种脂质沉积物都包含内部和外部脂质环境,它们的组成各不相同。为了评估卵母细胞间的变异性,在整个卵母细胞直径上记录线扫描,并与三个独立试验(GV,nvelence 91; MII,nvelence 172)进行比较,并使用主成分分析(PCA)分析数据。平均光谱和PCA载荷图显示了CH拉伸区域中明显且可重现的变化,可用作分子成熟标记。该方法为开发独立的方法以评估成熟过程中的卵母细胞状态铺平了道路,从而为单细胞水平的脂质分布提供了新的见识。

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