首页> 外文会议>Conference on photonic therapeutics and diagnostics IX >Could the differences in the biochemistry of prostate carcinoma compared to benign prostate tissue biopsy fragments be evaluated through Raman spectroscopy?
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Could the differences in the biochemistry of prostate carcinoma compared to benign prostate tissue biopsy fragments be evaluated through Raman spectroscopy?

机译:可以通过拉曼光谱评估与良性前列腺组织活检片段相比前列腺癌生物化学的差异吗?

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It has been proposed a spectral model to evaluate the biochemical differences between prostate carcinoma and benign fragments using dispersive Raman spectroscopy. We have examined 51 prostate fragments from surgically removed PrCa; each fragment was snap-frozen and stored (-80°C) prior spectral analysis. Raman spectrum was measured using a Raman spectrometer (830 nm excitation) coupled to a fiber-optic probe. Integration time and laser power were set to 50 s and 300 mW, respectively. It has been collected triplicate spectra from each fragment (total 153 spectra). Some samples exhibited a strong fluorescence, which was removed by a 7th order polynomial fitting. It has been developed a spectral model based on the least-squares fitting of the spectra of pure biochemicals (actin, collagen, elastin, carotene, glycogen, phosphatidylcholine, hemoglobin, and water) with the spectra of tissues, where the fitting parameters are the relative contribution of the compounds to the tissue spectrum. The spectra (600-1800 cm~(-1) range) are dominated by bands of proteins; it has been found a small difference in the mean spectra of PrCa compared to the benign tissue, mainly in the 1000-1400 cm~(-1) region, indicating similar biochemical constitution. The spectral fitting model revealed that elastin and phosphatidylcholine were increased in PrCa, whereas blood and water were reduced in malignant lesions (p < 0.05). A discrimination of PrCa from benign tissue using Mahalanobis distance applied to the contribution of elastin, hemoglobin and phosphatidylcholine resulted in sensitivity of 72% and specificity of 70%.
机译:已经提出了一种光谱模型,以评估前列腺癌和良性碎片之间使用分散拉曼光谱的生化差异。我们已经检查了来自手术删除的51个前列腺片段;每种片段都是卡扣 - 冷冻并储存(-80°C)之前的光谱分析。使用耦合到光纤探针的拉曼光谱仪(830 nm激发)测量拉曼光谱。集成时间和激光功率分别设定为50秒和300 mW。它已从每个片段收集三份光谱(总共153个光谱)。一些样品表现出强烈的荧光,通过第七阶多项式拟合除去。它已经开发了一种基于纯化生物化学型光谱的最小二乘拟合(肌动蛋白,胶原,弹性蛋白,胡萝卜素,糖原,磷脂酰胆碱,血红蛋白和水)的光谱模型,其中包含组织的光谱,其中拟合参数是化合物对组织谱的相对贡献。光谱(600-1800cm〜(-1)范围)由蛋白质带主导;已经发现与良性组织相比,PRCA的平均光谱差异,主要是在1000-1400cm〜(-1)区域,表明类似的生化构成。光谱拟合模型表明,PRCA中的弹性蛋白和磷脂酰胆碱增加,而恶性病变减少了血液和水(P <0.05)。使用应用于弹性蛋白,血红蛋白和磷脂酰胆碱的贡献的Mahalanobis距离的PRCA辨别PRCA,导致敏感性为72%和70%的特异性。

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