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首页> 外文期刊>Cytometry: The Journal of the Society for Analytical Cytology >Proposed flow cytometric reference method for the determination of erythroid F-cell counts
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Proposed flow cytometric reference method for the determination of erythroid F-cell counts

机译:拟议的流式细胞仪参考方法,用于测定红血球F细胞计数

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Background: Quantitation of adult erythrocytes (RBC) containing fetal hemoglobin (F cells) is of potential clinical utility in evaluating erythropoietic disorders, such as myelodysplasia and hemoglobinopathies, and in monitoring F-cell augmenting therapy. F-cell counting methodologies include fluorescence microscopy and flow cytometry, Previous flow cytometric methods have employed an isotype antibody control to distinguish F cells from non-F cells. We investigated the feasibility of using the orange autofluorescence signal (FL2) in glutaraldehyde-fixed RBC to substitute for fluorescein isothiocyanate (FITC)-labeled isotype control antibody use in F-cell quantitation. Methods: Our previously published method for fetal red cell detection in fetomaternal hemorrhage was used, employing a FITC-labeled anti-hemoglobin F (HbF) monoclonal antibody reagent. Blood samples with varying F-cell counts were quantitated for F cells using both immunofluorescence microscopy and flow cytometry comparing FITC-labeled isotype to FL1 thresholding defined by FL2 autofluorescence. Results: F cell percentages obtained by using an FL2 defined threshold for FL1 gating correlated well with expected values in diluted blood samples (r(2) = 0.994, slope = 1.019, intercept = 0.24), values obtained using an isotype control (r(2) = 0.996, slope = 1.012, intercept = -0.17), and microscopic immunofluorescence counts (r(2) = 0.989, slope = 0.999, intercept = -0.72). F-cell quantitation by the isotype control and FL2 autofluorescence methods was also comparable in 40 blood samples (r(2) = 0.994, slope = 1.014, intercept = 0.03). Intra-assay, interobserver, and interinstrument precision with this autofluorescence gating method exhibited low imprecision (coefficient of variation <14%). Conclusion: This novel method is a more objective and less laborious alternative for F-cell quantitation by flow cytometry compared to using an isotype control or microscopy, thereby providing a more robust methodology for clinical studies and consideration as a laboratory reference method for F-cell counting, Cytometry (Comm, Clin, Cytometry) 42:239-246, 2000, (C) 2000 Wiley-Liss, Inc. [References: 16]
机译:背景:定量含有胎儿血红蛋白(F细胞)的成年红细胞(RBC)在评估红细胞生成疾病(如骨髓增生异常和血红蛋白病)以及监测F细胞增强疗法方面具有潜在的临床应用价值。 F细胞计数方法包括荧光显微镜和流式细胞术。以前的流式细胞术方法已采用同种型抗体对照来区分F细胞和非F细胞。我们研究了在戊二醛固定的RBC中使用橙色自发荧光信号(FL2)替代荧光素异硫氰酸酯(FITC)标记的同种型对照抗体在F细胞定量分析中的可行性。方法:使用我们先前发表的胎儿红细胞检测胎儿母细胞性出血的方法,采用FITC标记的抗血红蛋白F(HbF)单克隆抗体试剂。使用免疫荧光显微镜和流式细胞术对F细胞计数变化的F细胞计数的血样进行定量,将FITC标记的同种型与FL2自发荧光定义的FL1阈值进行比较。结果:通过使用FL2门限的FL2定义阈值获得的F细胞百分比与稀释血样中的预期值(r(2)= 0.994,斜率= 1.019,截距= 0.24)很好相关,而通过同型对照获得的值(r( 2)= 0.996,斜率= 1.012,截距= -0.17)和显微免疫荧光计数(r(2)= 0.989,斜率= 0.999,截距= -0.72)。通过同型对照和FL2自发荧光方法进行的F细胞定量在40个血液样本中也具有可比性(r(2)= 0.994,斜率= 1.014,截距= 0.03)。使用这种自发荧光门控方法的测定内,观察员间和仪器间的精密度均显示出较低的不准确性(变异系数<14%)。结论:与使用同型对照或显微镜检查相比,这种新方法是流式细胞术定量F细胞的一种更客观,更省力的替代方法,从而为临床研究和作为F细胞的实验室参考方法提供了更可靠的方法计数,细胞计数法(Comm,Clin,Cytometry)42:239-246,2000,(C)2000 Wiley-Liss,Inc. [参考:16]

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