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自动血小板计数技术的持续发展。

Continuing developments with the automated platelet count.

作者信息

Briggs C, Harrison P, Machin S J

机构信息

Department of Haematology, University College London Hospitals, London, UK.

出版信息

Int J Lab Hematol. 2007 Apr;29(2):77-91. doi: 10.1111/j.1751-553X.2007.00909.x.

Abstract

The four main procedures for platelet counting are: manual phase contrast microscopy, impedance, optical light scatter/fluorescence and flow cytometry. Early methods to enumerate platelets were inaccurate and irreproducible. The manual count is still recognized as the gold standard or reference method, and until very recently the calibration of platelet counts by the manufacturers of automated cell counters and quality control material was performed by this method. However, it is time-consuming and results in high levels of imprecision. The introduction of automated full blood counters using impedance technology resulted in a dramatic improvement in precision. However, impedance counts still have limitations as cell size analysis cannot discriminate platelets from other similar-sized particles. More recently, light scatter or fluorescence methods have been introduced for automated platelet counting, but there are still occasional cases where an accurate platelet count remains a challenge. Thus, there has been interest in the development of an improved reference procedure to enable optimization of automated platelet counting. This method utilizes monoclonal antibodies to platelet cell surface antigens conjugated to a suitable fluorophore. This permits the possible implementation of a new reference method to calibrate cell counters, assign values to calibrators, and to obtain a direct platelet count on a variety of pathological samples. In future, analysers may introduce additional platelet parameters; a reliable method to quantify immature or reticulated platelets would be useful.

摘要

血小板计数的四种主要方法是

手工相差显微镜检查法、阻抗法、光学光散射/荧光法和流式细胞术。早期的血小板计数方法不准确且不可重复。手工计数仍被视为金标准或参考方法,直到最近,自动血细胞计数器和质量控制材料制造商对血小板计数的校准仍采用这种方法。然而,它耗时且导致高度不精确。采用阻抗技术的自动全血细胞计数器的引入使精密度有了显著提高。然而,阻抗计数仍有局限性,因为细胞大小分析无法将血小板与其他大小相似的颗粒区分开来。最近,光散射或荧光方法已被引入用于自动血小板计数,但仍有偶尔的情况,准确的血小板计数仍是一项挑战。因此,人们对开发一种改进的参考程序以优化自动血小板计数产生了兴趣。该方法利用与合适荧光团偶联的针对血小板细胞表面抗原的单克隆抗体。这使得有可能实施一种新的参考方法来校准血细胞计数器、为校准物赋值,并在各种病理样本上获得直接的血小板计数。未来,分析仪可能会引入额外的血小板参数;一种可靠的量化未成熟或网织血小板的方法将很有用。

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