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通过使用二聚体甄别策略,提高血小板-单核细胞复合物计数的准确性和可重复性。

Improved accuracy and reproducibility of enumeration of platelet-monocyte complexes through use of doublet-discriminator strategy.

机构信息

Department of Haematology, University College London, Royal Free Hospital Campus, London NW3 2PF, United Kingdom.

出版信息

Cytometry B Clin Cytom. 2012 Nov;82(6):353-9. doi: 10.1002/cyto.b.21040. Epub 2012 Aug 22.

DOI:10.1002/cyto.b.21040
PMID:22915375
Abstract

BACKGROUND

Platelet-monocyte complex (PMC) formation is a marker of in vivo platelet activation and may be readily measured by flow cytometry. Due to the high frequency of free platelets relative to monocytes and PMCs, false-positive identification through coincidence remains a significant technical problem.To overcome this problem, we evaluated the use of a doublet-discriminator strategy (DDM) to allow faster sample acquisition whilst significantly reducing aberrant coincidence.

METHODS

Fourteen healthy volunteers and 20 patients with coronary artery disease (CAD) gave arterial and/or peripheral venous blood samples (NaCit). Whole blood was labelled in duplicate with anti-CD61 and anti-CD14 using a standard lyse/wash protocol. One of each paired sample was serially diluted before analysis; the second was analyzed at full concentration but using FL1-width to exclude co-incident platelet and monocyte events. Control experiments were performed with ex vivo thrombin activated samples.

RESULTS

With the DDM use PMC frequencies in the peripheral blood of healthy individuals and in CAD patients fell significantly [6.27% ± 1.77 (mean ± sd) to 2.57% ± 0.99 (P = 0.02)] and from 16.04% (± 11.26) to 7.66% (± 5.18) (P < 0.01), respectively. DDM use significantly reduced the percentage of PMCs in the ex vivo thrombin activated samples (P < 0.05).

CONCLUSIONS

Use of DDM effectively reduces the coincidence and enumerates true PMC in the samples of normal individuals and in patients with CAD and in ex vivo thrombin activated samples.

摘要

背景

血小板-单核细胞复合物(PMC)的形成是体内血小板活化的标志物,可通过流式细胞术进行测量。由于游离血小板与单核细胞和 PMCs 的频率相比非常高,因此通过巧合进行假阳性识别仍然是一个重大的技术问题。为了解决这个问题,我们评估了使用双区分策略(DDM)的方法,该方法允许更快地采集样本,同时显著减少异常巧合。

方法

14 名健康志愿者和 20 名冠心病(CAD)患者采集动脉和/或外周静脉血样(NaCit)。全血用抗 CD61 和抗 CD14 双重标记,使用标准的裂解/洗涤方案。每个配对样本的一份进行连续稀释后进行分析;另一份则在全浓度下进行分析,但使用 FL1 宽度排除血小板和单核细胞事件的偶然重合。用体外凝血酶激活的样本进行对照实验。

结果

使用 DDM 后,健康个体和 CAD 患者外周血中的 PMC 频率显著降低[6.27%±1.77(均值±标准差)至 2.57%±0.99(P=0.02)],分别从 16.04%(±11.26)降至 7.66%(±5.18)(P<0.01)。DDM 的使用显著降低了体外凝血酶激活样本中 PMC 的百分比(P<0.05)。

结论

DDM 的使用可有效减少巧合,并对正常个体和 CAD 患者以及体外凝血酶激活样本中的真正 PMC 进行计数。

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