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Quantification of Relative Chromatin Content in Flow Cytometry Standards using 3D OPTM Imaging Technique

机译:使用3D OPTM成像技术对流式细胞仪标准品中的相对染色质含量进行定量

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A potential biomarker for early diagnosis of cancer is assessment of high nuclear DNA content. Conventional hematoxylin staining is neither stoichiometric nor reproducible. Although feulgen stain is stoichiometric, it is time consuming and destroys nuclear morphology. We used acidic thionin stain, which can be stoichiometric and also preserve the nuclear morphology used in conventional cytology. Fifty chicken erythrocyte nuclei singlets (CENs), diploid trout erythrocyte nuclei (TENs) and Triploid TENs were stained for 15 and 30 minutes each. After imaging with optical projection tomography microscope (OPTM), 3D reconstructions of the nuclei were processed to calculate chromatin content. The mean of ratios of individual observations was compared with standard ratios of DNA indices of the flow cytometry standards. Mean error, standard deviation and 97% confidence interval (CI) was computed for the ratios of these standards. At 15 and 30 minutes, the ratio of Triploid TEN to TEN was 1.72 and 1.76, TEN to CEN was 1.27 and 2.01 and Triploid TEN to CEN was 2.11 and 3.39 respectively. Estimates of DNA indices for all 3 types of nuclei had less mean error at 30 minutes of staining; Triploid TEN to TEN 0.349±0.04, TEN to CEN 0.36±0.04 and Triploid TEN to CEN 0.64 ± 0.07. In conclusion, imaging of cells with thionin staining at 30 minutes and 3D reconstruction provides quantitative assessment of cell chromatin content. The addition of this quantitative feature of aneuploidy is expected to add greater accuracy to a classifier for early diagnosis of cancer based on 3D cytological imaging.
机译:早期诊断癌症的潜在生物标志物是高核DNA含量的评估。传统的苏木精染色既不是化学计量的也不是可重复的。尽管富尔根染料是化学计量的,但它很耗时并且破坏了核的形态。我们使用了酸性硫蛋白染色剂,该染色剂可以是化学计量的,也可以保留常规细胞学中使用的核形态。五十只鸡红细胞核单峰(CEN),二倍体鳟鱼红细胞核(TENs)和三倍体TENs分别染色15分钟和30分钟。用光学投影断层扫描显微镜(OPTM)成像后,对核的3D重建进行处理以计算染色质含量。将各个观察值的平均值与流式细胞仪标准品的DNA指标的标准比例进行比较。计算这些标准物的比例的平均误差,标准偏差和97%置信区间(CI)。在15和30分钟时,三倍体TEN与TEN的比例分别为1.72和1.76,TEN与CEN的比例分别为1.27和2.01,三倍体TEN与CEN的比例分别为2.11和3.39。在染色30分钟时,所有3种细胞核的DNA指数估算值均值误差较小;三倍体TEN至TEN 0.349±0.04,TEN至CEN 0.36±0.04和三倍体TEN至CEN 0.64±0.07。总之,在30分钟时用硫蛋白染色和3D重建对细胞进行成像可对细胞染色质含量进行定量评估。这种非整倍性的定量特征的添加有望为基于3D细胞学成像的早期诊断癌症的分类器增加更高的准确性。

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