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用血液荧光计测量接近正常浓度的红细胞原卟啉:血浆对“前表面照明”检测的影响。

Measurement of near-normal concentrations of erythrocyte protoporphyrin with the hematofluorometer: influence of plasma on "front-surface illumination" assay.

作者信息

Schifman R B, Finley P R

出版信息

Clin Chem. 1981 Jan;27(1):153-6.

PMID:7449099
Abstract

Zinc protoporphyrin in erythrocytes increases in iron depletion. Because the hematofluorometer directly measures zinc protoporphyrin in whole blood, it may therefore be a useful screening instrument for detecting iron deficiency. We evaluated its performance with normal to slightly above-normal zinc protoporphyrin concentrations (0.2 to 2.0 mg/L) in erythrocytes, because this is a critical range for differentiating normal and iron-deficient individuals. There was excellent correlation (r2 = 0.900) between erythrocyte protoporphyrin as measured by an extraction procedure and as measured directly with the hematofluorometer. However, at these concentrations, plasma caused hematofluorometer readings to be spuriously high, by 2.4 to 89.4%, an effect due to the instrument's optical design. The effect can be eliminated by washing the cells free of plasma or by allowing erythrocytes to displace plasma by settling to the illuminated surface before the measurement. The interference does not affect the hematofluorometer's sensitivity, but abnormal results obtained for whole blood should be confirmed with more-specific tests, and interlaboratory precision may be influenced if whole-blood samples are used. A 1-min delay from sample placement to measurement decreased zinc protoporphyrin values by 2.6 to 36.9%. We also describe the use of cryopreserved control erythrocytes, for which the CV is 2.3% for a concentration of 0.96 mg per liter of erythrocytes, which are not affected by time of measurement, and which are stable for three months.

摘要

缺铁时红细胞中的锌原卟啉会增加。由于血液荧光计可直接测量全血中的锌原卟啉,因此它可能是检测缺铁的一种有用的筛查工具。我们评估了其在红细胞锌原卟啉浓度正常至略高于正常(0.2至2.0mg/L)时的性能,因为这是区分正常人和缺铁个体的关键范围。通过萃取法测量的红细胞原卟啉与用血液荧光计直接测量的结果之间存在极好的相关性(r2 = 0.900)。然而,在这些浓度下,血浆会导致血液荧光计读数出现高达2.4%至89.4%的假性升高,这是由于仪器的光学设计所致。通过洗涤细胞去除血浆或在测量前让红细胞沉降到光照表面以取代血浆,可消除这种影响。这种干扰不会影响血液荧光计的灵敏度,但全血获得的异常结果应通过更特异的检测进行确认,如果使用全血样本,实验室间的精密度可能会受到影响。从放置样本到测量的1分钟延迟会使锌原卟啉值降低2.6%至36.9%。我们还描述了冷冻保存的对照红细胞的使用,对于每升红细胞浓度为0.96mg的情况,其CV为2.3%,不受测量时间影响,且在三个月内稳定。

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