定制扫描细胞仪对胎儿nrbc模型制备的超罕见事件检测性能。

Cytometry Pub Date : 2000-04-01
S Bajaj, J B Welsh, R C Leif, J H Price
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引用次数: 0

摘要

背景:利用母体循环中的胎儿有核红细胞(fnrbc)模型,对全自动扫描细胞仪的性能进行了评估,该扫描细胞仪结合了先前报道的高精度自动聚焦和精确图像分割,用于检测“超罕见”细胞。这些独特的扫描细胞术技术有望显著提高灵敏度和特异性。方法:用异硫氰酸荧光素偶联抗胎儿血红蛋白和核染料4,6-二氨基-2-苯基吲哚对正常成人血液和胎儿红细胞进行染色。将成人细胞与胎儿细胞加尖,形成10(7)个有核细胞中约1个fnRBC的比例,并使用离心细胞学方法将其单层沉积在载玻片上。对罕见事件性能参数进行了审查、形式化,并应用于使用该单元模型测试新仪器。结果:对15张载玻片进行分析,以确定其与人工检测的性能,并对4组载玻片进行扫描,每组扫描4张载玻片,以探索检测的极限。结果平均灵敏度为91%,平均特异性误差为每百万细胞12.3个假阳性,在862 Hz的细胞分析率下重复性为100%。随着扫描后快速互动步骤的增加,假阳性率在15个实验中下降到总共只有一个伪影。该仪器成功地在2000万个成年细胞中定位了1个fnRBC,这是检测的最低限度。结论:这种持续的高性能,加上扫描任意数量细胞的能力,验证了用于超罕见事件检测的精确高速自动对焦和精确实时图像分割的巨大潜力。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
Ultra-rare-event detection performance of a custom scanning cytometer on a model preparation of fetal nRBCs.

Background: The performance of a fully automated scanning cytometer incorporating previously reported high-precision autofocus and accurate image segmentation was evaluated for the detection of "ultra-rare" cells using a model of fetal nucleated red blood cells (fnRBCs) in the maternal circulation. These distinctive scanning cytometry techniques were expected to markedly improve sensitivity and specificity.

Methods: Normal adult blood and fetal red blood cells were stained with fluorescein isothiocyanate-conjugated anti-fetal hemoglobin and 4,6-diamidino-2-phenylindole, a nuclear dye. Adult cells were spiked with fetal cells to create ratios of about 1 fnRBC in 10(7) nucleated cells and deposited in monolayers on slides using centrifugal cytology. Rare-event performance parameters were reviewed, formalized, and applied to test the new instrument using this cell model.

Results: Fifteen slides were analyzed to establish performance by comparison with manual detection, and four sets of four slides each were then scanned to explore the limit of detection. Results were an average sensitivity of 91%, an average specificity error of 12.3 false-positives per million cells, and repeatability of 100% at a cell analysis rate of 862 Hz. With addition of a quick interactive step subsequent to scanning, the false-positive rate dropped to a total of only one artifact over the 15 experiments. The instrument succeeded at locating 1 fnRBC in 20 million adult cells, the lowest limit of detection tested.

Conclusion: This consistently high performance, coupled with the capability of scanning arbitrarily large numbers of cells, validates the considerable potential of precise high-speed autofocus and accurate real-time image segmentation for ultra-rare event detection.

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