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Laboratory evaluation of a flow cytometric BCR-ABL immunobead assay

机译:流式细胞仪BCR-ABL免疫珠测定的实验室评估

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摘要

Background: A new flow cytometric (FC) BCR-ABL immunobead assay has been developed recently. Here we present the laboratory evaluation of the commercially available kit. Methods: Mononuclear cells were isolated, lysed and processed according to the instructions of the manufacturer. Anti-BCR antibodies adsorbed to capture beads bind the BCR-ABL fusion proteins of the lysed cells, a phycoerythrin (PE)-conjugated anti-ABL antibody is the detector reagent and mean fluorescence intensity (MFI) signals were recorded by flow cytometry. Detection of t(9;22)(q34;q11) translocation was carried out with a quantitative PCR assay. Results: MFI results of 20 normal peripheral blood samples were 88±8 (mean±SD), CV 9. K562 cells were used as positive control. Within-batch imprecision was excellent (3.7 in the normal and 10 in the pathological range). Cut-off was chosen at MFI 112, where both sensitivity and specificity were 100. Altogether 17 chronic myeloid leukemia (CML) and 16 acute leukemia samples were analyzed. All PCR positive samples (n14) were positive with the FC method and negative results were also concordant (n15). Frozen cell lysates can be stored up to 4 weeks without significant decrease of MFI signal. Conclusions: The FC BCR-ABL assay is a fast, reproducible and reliable method that may be incorporated into standard flow cytometric protocols to help clinical decision-making.
机译:背景:最近开发了一种新的流式细胞术(FC)BCR-ABL免疫珠测定法。在这里,我们介绍了市售套件的实验室评估。方法:按照制造商的说明分离,裂解和处理单核细胞。吸附到捕获珠上的抗BCR抗体与裂解细胞的BCR-ABL融合蛋白结合,结合了藻红蛋白(PE)的抗ABL抗体是检测试剂,并且通过流式细胞术记录了平均荧光强度(MFI)信号。用定量PCR测定法检测t(9; 22)(q34; q11)易位。结果:20例正常外周血样本的MFI结果为88±8(平均值±SD),CV9。将K562细胞用作阳性对照。批内不精确度极好(正常情况下为3.7,病理范围内为10)。在MFI 112处选择了临界值,其敏感性和特异性均为100。共分析了17种慢性髓样白血病(CML)和16种急性白血病样本。所有PCR阳性样品(n14)在FC方法中均为阳性,阴性结果也一致(n15)。冷冻的细胞裂解液最多可保存4周,而MFI信号不会明显降低。结论:FC BCR-ABL检测是一种快速,可重复且可靠的方法,可将其纳入标准流式细胞术方案以帮助临床决策。

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