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1、1血小板单采样品中残留白细胞计数两种方法的评价作者:王拥军,沈卓岚,徐健,黄伯里,胡庆丰,冯武威【摘要】 为评价流式细胞计数法和 Nageotte 血细胞计数法计数单采血小板中残留白细胞,应用系列的稀释实验研究其准确性;对已知白细胞浓度的同一样本,反复检测 14 次,研究其重复性;分别用流式细胞计数法和 Nageotte 血细胞计数法检测 102 份去白细胞的单采血小板样本,对其结果进行比较。结果发现,当白细胞浓度为 0.8WBC/l10 时,两方法无显著差异(P0.05) 。结论: 两种方法均可用于少白细胞成分的质量控制。 【关键词】 血小板单采Evaluation of Two Metho
2、ds for Counting Residual White Blood Cells in Thrombocytaphoresis ConcentratesAbstract To evaluate flow-cytometry and Nageotte method for counting residual WBC in thrombocytaphoresis concentrates, their accuracies were determined by dilution studies separately;the repeatability was determined by mea
3、su-ring the interassay coefficient of variation for 14 replicates of a sample with known leukocyte concentration. 102 samples of leukocyte-depleted thrombocytaphoresis concentrates were detected by the above mentioned two methods,andthe results were compared each other. The results showed that no di
4、fference was observed between two methods over a range of leukocyte concentrations from 0.8 to 10 WBC/l(P0.05). In conclusion,flow-cytometry and Nageotte methods can be used for quality control of WBC-reduced blood components.Key words thrombocytapheresis; platelet; WBC; flow-cytometry method; Nageo
5、tte method近年来,大力提倡和开展成分献(输)血,尤其是单采血小板。近代医学研究表明,血液中非治疗性成分如白细胞等是一种“污染物” ,去除单采血小板样品中白细胞的污染不仅可以降低非溶血性输血反应1 、巨细胞病毒等嗜白细胞病毒的传播2 ,还可以减少 HLA 同种异体免疫反应3 (血小板输注无效、移植物抗宿主病等) 。国际上,已将引起 HLA 同种异体免疫反应的白细胞污染量控制在 5106 以下4 。这已远远超出了现有传统计数方法的检测限。近几年,已经报道了很多种低浓度白细胞的计数方法5 ,其中 Nageotte 血细胞计数法和流式细胞计数法应用最广6-8 。我们对这两种低浓度白细胞污染的
6、计数方法进行了应用和评价。现将结果报告如下。2材料和方法仪器与试剂流式细胞计数:FACSCalibur 流式细胞仪(BDIS 产品) 、LeucoCOUNT 试剂(BDIS 产品) 和 TruCOUNT 磁珠管(BDIS 产品) 。Nageotte 计数盘(Hausser Scientific Horsham,USA 产品)。血小板单采机:MCS+ Haemonetics 与Spectra,COBE Laboratories。白细胞定值样本:由浙江大学医学院与浙江省人民医院提供。样本收集浙江省血液中心无偿献血者去白细胞单采血小板,共 102 份,留样后 24 小时内检测。流式细胞计数将 100
7、 l 样品加入到已知数量的 TruCOUNT 磁珠管中,再加入 400 l 试剂,轻摇,室温暗置 30 分钟,混匀后计数 1.0104 磁珠中 PI 染色的白细胞数。利用以下公式计算白细胞浓度: WBC/l=(白细胞数/104)TruCOUNT 总磁珠数/ 样品体积(100 l)Nageotte 血细胞计数样品 5 倍稀释,充池后加盖静置 30 分钟,普通光学显微镜计数 1 个大方格(50 l)内白细胞总数(n) 。利用以下公式计算白细胞浓度:WBC/l= (n/50)5=n/10统计学分析实验结果以均数标准差(XD)表示,统计处理采用 Microsoft Excel 软件,P0.05 认为有
8、统计学意义。结 果准确性评价已知白细胞浓度的样品通过 1/10 系列稀释(0.1-10.0 WBC/l) ,每份标本分别用流式细胞计数法(A)和 Nageotte 血细胞计数法(B)平行检测。将测定值与预期值配对回归分析,得到相关系数(r) 、斜率和截距。当0.1WBC/l0.7 时,流式细胞计数法的测定值和预期值呈直线相关,y=0.99x+0.01,r=0.99(P0.001) ,Nageotte 血细胞计数法测定值比预期值持续偏低,y=1.07x-0.21,相关性差,r=0.90(图 1) ;当 0.8WBC/l10.0 时,两方法的直线回归分别为 A:y=1.01x-0.02,B:y=0
9、.99x-0.07,测定值和预期值呈直线相关 r=0.99(P0.001) ,准确性高(图 2) 。3重复性评价白细胞浓度为 4.0/l 的同一样本,分别用两种方法重复检测 14 次,流式细胞计数法白细胞均值为 4.07 /l,95%可信区间为 3.51-4.63/l;Nageotte血细胞计数法白细胞均值为 3.91/l,95%可信区间为 3.27-4.55/l。两方法的 14 次检测结果均在 95%可信区间内,重复性高(CV10%) (表 1) 。Table 1. Interassay coefficient of variation for 14 replications of a sa
10、mple with a mean leukocyte concentration of 4/l(略)应用性评价分别用两种方法同时检测 102 份去除白细胞的单采血小板样品,流式细胞计数法检测白细胞均值为 1.12/l ;Nageotte 血细胞计数法检测白细胞均值为1.10/l,所有检测结果均在 95%可信区间内。经统计分析,发现两方法无显著差异(P0.05) ,结果见表 2。Table 2. Comparison of results obtained byflow cytometry and Nageotte method (略)讨论由于白细胞去除技术的不断发展,低浓度白细胞检测也面临更新
11、的挑战,传统的全自动血细胞计数仪检测精度100/l9,10 ;Neubauer 计数池精度为2.8-5.6/l;Nageotte 计数池与流式仪的精度均可达到 0.05-0.1/l,当白细胞数0.8/l,Nageotte 血细胞计数法和流式细胞计数法一样,其测定值和预期值呈直线相关(图 2),准确度高、重复性好(CV10%) ,检测 102 份样本,两者并无显著差异。基于以上结果,本研究肯定了 Nageotte 血细胞计数法和流式细胞计数法在相应检测限内高度的准确性和可重复性。Wenz10与 Kao 等11也发现,Nageotte 血细胞计数明显比传统方法准确可靠,与流式细胞计数相比,具有不需
12、要特殊的仪器和试剂、简单、快速、经济等优点,适合于血站系统血液成分白细胞污染的常规质量控制12 。【参考文献】1Wenz B,Gurtlinger KF,O Toole AM,et al. Preparation of gra- nulocyte-poor red cells by microaggregate filtration:a simplified method to minimize febrile transfusion reaction. Vox Sang,1980; 39: 282-2872Gilbert GL,Hayes K,Hudson IL,et al. Prevent
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14、pro- ducts. Blood,1988; 71: 1402-14074Fisher M,Chapman JR,Ting A,et al. Alloimmunization to HLA antigens following transfusion with leukocyte-poor and purified platelet suspensions. Vox Sang,1985; 49: 331-3355Dzik S. Principles of counting low numbers of leukocytes in leuko reduced blood components.
15、Transfus Med Rev,1997; 11: 44-556Lutz P,Dzik WH. Large volume hemocytometer chamber for accurate counting of white cells(WBCs) in WBC-reduced platelets:validation and application for quality control of WBC- reduced platelets prepared by apheresis and filtration. Transfusion,1993; 33: 409-4127Masse M
16、,Naegelen C,Pellegrini N,et al. Validation of a simple method to count very low white cell concentrations in filtered RBCs or platelets,Transfusion,1992; 32: 565-5718Vengelen-Tyler V. Technical manual. Bethesda: American Association of Blood Banks. 1996: 722-7259Kjeldsberg CR,Knight JA. Body fluids: laboratory examination of amnionic,cerebrospinal,seminal,serous,and synovial fluids. In Laboratory methods. Chicago
