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Development of On-Chip Multi-Imaging Flow Cytometry for Identification of Imaging Biomarkers of Clustered Circulating Tumor Cells

机译:片上多重成像流式细胞仪的发展用于鉴定簇状循环肿瘤细胞的成像生物标志物

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摘要

An on-chip multi-imaging flow cytometry system has been developed to obtain morphometric parameters of cell clusters such as cell number, perimeter, total cross-sectional area, number of nuclei and size of clusters as “imaging biomarkers”, with simultaneous acquisition and analysis of both bright-field (BF) and fluorescent (FL) images at 200 frames per second (fps); by using this system, we examined the effectiveness of using imaging biomarkers for the identification of clustered circulating tumor cells (CTCs). Sample blood of rats in which a prostate cancer cell line (MAT-LyLu) had been pre-implanted was applied to a microchannel on a disposable microchip after staining the nuclei using fluorescent dye for their visualization, and the acquired images were measured and compared with those of healthy rats. In terms of the results, clustered cells having (1) cell area larger than 200 µm2 and (2) nucleus area larger than 90 µm2 were specifically observed in cancer cell-implanted blood, but were not observed in healthy rats. In addition, (3) clusters having more than 3 nuclei were specific for cancer-implanted blood and (4) a ratio between the actual perimeter and the perimeter calculated from the obtained area, which reflects a shape distorted from ideal roundness, of less than 0.90 was specific for all clusters having more than 3 nuclei and was also specific for cancer-implanted blood. The collected clusters larger than 300 µm2 were examined by quantitative gene copy number assay, and were identified as being CTCs. These results indicate the usefulness of the imaging biomarkers for characterizing clusters, and all of the four examined imaging biomarkers—cluster area, nuclei area, nuclei number, and ratio of perimeter—can identify clustered CTCs in blood with the same level of preciseness using multi-imaging cytometry.
机译:已开发了片上多成像流式细胞仪系统,以获取细胞簇的形态参数,例如细胞数量,周长,总横截面积,核数目和簇的大小,作为“成像生物标记物”,同时采集和以每秒200帧(fps)的速度分析亮场(BF)和荧光(FL)图像;通过使用该系统,我们检查了使用成像生物标志物鉴定簇状循环肿瘤细胞(CTC)的有效性。使用荧光染料将核染色后,将预先植入了前列腺癌细胞系(MAT-LyLu)的大鼠的样本血涂在一次性微芯片上的微通道上,并对其进行测量和比较。健康大鼠的那些。根据结果​​,在癌细胞中特别观察到具有(1)细胞面积大于200μm 2 和(2)细胞核面积大于90μm 2 的簇状细胞。 -植入的血液,但在健康大鼠中未观察到。此外,(3)核数多于3个的簇对植入癌的血液具有特异性,并且(4)实际周长与从所获得的面积计算出的周长之比(小于理想圆度的形状)小于0.90对所有具有3个以上核的簇都具有特异性,对癌症植入的血液也具有0.90的特异性。通过定量基因拷贝数分析检查收集到的大于300 µm 2 的簇,并将其鉴定为CTC。这些结果表明,成像生物标记物可用于表征簇,并且所检查的四个成像生物标记物(簇面积,细胞核面积,细胞核数目和周长比)全部可以使用多准确度鉴定相同水平的血液中的簇状CTC。 -成像细胞术。

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