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A Cytometric Dual-Bead Array for Analyzing PML-RARalpha Fusion Protein

机译:用于分析PML-Raralpha融合蛋白的细胞计量双珠阵列

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This study investigated a cytometric dual-bead array used to analyze PML-RARalpha fusion protein. The carboxylated and aminated polystyrene beads were prepared and barcoded with either high or low brightness using a fluorescein isothiocyanate (FITC) penetration method. Using anti-RARalpha antibody, homotype control antibody, barcoded beads and phycoerythrin (PE)-labeled antibody, the analytical capability of the cytometric dual-bead array was tested with two cell models containing a NB_4 cell line. Fusion protein levels were normalized using a PE mean fluorescence intensity (MFI) ratio (PE MFI of high brightness beads / PE MFI of low brightness beads). In flow cytometry, the cytometric dual-bead array could analyze PML(L)-RARalpha protein with high specificity, and this assay possessed analytical sensitivity of at least 0.6%. A dilution experiment also demonstrated a concordant result between the logarithm of the PE MFI ratio and the logarithm of the NB_4 cell concentration (R~2 = 0.9936). When compared with a cytometric single-bead assay, this array exhibited a lower relative standard deviation (R.S.D.) and a lower relative error (R.E.). In conclusion, using the MFI ratio can attenuate data error in fusion protein cytometric analysis, and the cytometric dual-bead array presented here may be of use in the quantification of PML-RARalpha fusion protein.
机译:本研究研究了用于分析PML-Raralpha融合蛋白的细胞计量双珠阵列。使用荧光素异硫氰酸酯(FITC)渗透法制备羧化和胺化聚苯乙烯珠粒并用高亮度或低亮度进行条形晶体。使用抗Raralpha抗体,同种型对照抗体,条形码珠和植物(PE) - 标记抗体,用含有Nb_4细胞系的细胞模型测试细胞计数双珠阵列的分析能力。使用PE平均荧光强度(MFI)比率(MFI)比率(高亮度珠/ PE MFI的PE MFI的低亮度珠子)归一化融合蛋白水平。在流式细胞术中,细胞术双珠阵列可以分析具有高特异性的PML(L)-rarpha蛋白,并且该测定具有至少0.6%的分析敏感性。稀释实验还证明了PE MFI比率与NB_4细胞浓度的对数之间的一致性结果(R〜2 = 0.9936)。与细胞计量单珠测定相比,该阵列表现出较低的相对标准偏差(R.S.D.)和较低的相对误差(R.E.)。总之,使用MFI比可以衰减融合蛋白质细胞术分析中的数据误差,并且这里呈现的细胞计量双珠阵列可以用于定量PML-Raralpha融合蛋白。

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