使用近场光热显微光谱法监测MCF-7细胞中的细胞周期分布。
Monitoring cell cycle distributions in MCF-7 cells using near-field photothermal microspectroscopy.
作者信息
Hammiche Azzedine, German Matthew J, Hewitt Rebecca, Pollock Hubert M, Martin Francis L
机构信息
Department of Physics, Institute of Environmental and Natural Sciences, Lancaster University, Lancaster, United Kingdom.
出版信息
Biophys J. 2005 May;88(5):3699-706. doi: 10.1529/biophysj.104.053926. Epub 2005 Feb 18.
Microspectroscopic techniques such as Fourier transform infrared (FTIR) have played an important role in "fingerprinting" the biochemical composition of cellular components. Based on structure and function, complex biomolecules absorb energy in the mid-infrared (lambda = 2-20 microm) yielding characteristic vibrational infrared (IR) spectra. However, optical detection FTIR microspectroscopy may not be suitable for IR-absorbing sample materials. Photothermal microspectroscopy (PTMS) permits the direct measurement of heat generated as a result of sample material absorbing radiation. This approach generates true absorption spectra and is implemented by interfacing a scanning probe microscope and an FTIR spectrometer. Detection is performed using a near-field ultra-miniaturized temperature sensor. Employing PTMS, IR spectra of MCF-7 cells were examined in spectral regions (900-2000 cm(-1)) corresponding to proteins, DNA, RNA, glycoproteins, carbohydrates, lipids, and levels of protein phosphorylation. As a cell passes through the cell cycle, its nuclear material decondenses and condenses and this has led to ambiguity as to whether the intensity of such spectral regions may be associated with the G(1)-, S- or G(2)-phases of the cell cycle. Cultured cells were tracked over a time course known to correspond to marked alterations in cell-cycle distributions, as determined using flow cytometry. Experiments were carried out in the absence or presence of lindane, a pesticide known to induce G(1)-arrest in MCF-7 cells. Significant (P < 0.05) elevations in spectral intensities were associated with exponentially growing cell populations, predominantly in S-phase or G(2)-phase, compared to more quiescent populations predominantly in G(1)-phase. Increases in the absorption band at 970 cm(-1), associated with elevated protein phosphorylation, were observed in vibrational spectra of exponentially growing cell populations compared to those exhibiting a slowing in their growth kinetics. These results seem to suggest that intracellular bulk changes, associated with transit through the cell cycle, can be tracked using PTMS.
傅里叶变换红外光谱(FTIR)等显微光谱技术在对细胞成分的生化组成进行“指纹识别”方面发挥了重要作用。基于结构和功能,复杂生物分子在中红外区域(波长λ = 2 - 20微米)吸收能量,产生特征性的振动红外(IR)光谱。然而,光学检测FTIR显微光谱法可能不适用于红外吸收性样品材料。光热显微光谱法(PTMS)允许直接测量样品材料吸收辐射产生的热量。这种方法可生成真实的吸收光谱,通过将扫描探针显微镜与FTIR光谱仪连接来实现。使用近场超小型温度传感器进行检测。采用PTMS,在对应于蛋白质、DNA、RNA、糖蛋白、碳水化合物、脂质以及蛋白质磷酸化水平的光谱区域(900 - 2000 cm⁻¹)对MCF - 7细胞的红外光谱进行了检测。随着细胞通过细胞周期,其核物质会发生解聚和凝聚,这导致关于此类光谱区域的强度是否可能与细胞周期的G₁期、S期或G₂期相关存在模糊性。在已知对应于细胞周期分布显著变化的时间进程中对培养细胞进行跟踪,这是通过流式细胞术确定的。在存在或不存在林丹(一种已知可诱导MCF - 7细胞G₁期阻滞的农药)的情况下进行实验。与主要处于G₁期的较为静止的细胞群体相比,光谱强度的显著升高(P < 0.05)与指数生长的细胞群体相关,这些细胞群体主要处于S期或G₂期。与生长动力学减缓的细胞群体相比,在指数生长的细胞群体的振动光谱中观察到970 cm⁻¹处吸收带增加,这与蛋白质磷酸化水平升高有关。这些结果似乎表明,使用PTMS可以跟踪与细胞周期进程相关的细胞内整体变化。
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