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首页> 外文期刊>Cytometry, Part A: the journal of the International Society for Analytical Cytology >Flow cytometric quantitation of opsonophagocytosis and intracellular killing of Candida albicans using a whole blood microassay
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Flow cytometric quantitation of opsonophagocytosis and intracellular killing of Candida albicans using a whole blood microassay

机译:使用全血微量测定法对白细胞念珠菌的调理吞噬作用和细胞内杀伤进行流式细胞术定量

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Flow cytometric assays for quantifying polymorphonuclear leucocyte (PMN) function involve peripheral blood fractionation methods. However, most are of limited use for conditions like pediatrics and thalassemia, as they may require large blood volumes or complicated by red blood cefl contamination. in whole blood assay, 500-mu l aliquots of normal or thalassemic whole blood were incubated with bis-carboxyethyl-carboxyfluorescein pentaacetoxymethylester (BCECF-AM)-labeled Candida albicans cells and phycoerythrin-conjugated anti-CD13 monoclonal antibody for PMNs. Phagocytosis was quantitated by gating on CD13 label PMNs and determining the frequency of phagocytosed yeast using flow cytometry. The killing activity was quantitated by estimating the number of viable fluorescence retaining yeast cells liberated following lysis of PMNs. In normal control or thalassemia samples, nonphagocytosed yeast and PMNs with or without phagocytosed yeast were readily distinguished by two-color dot plot, permitting phagocytosis estimates. Viable and nonviable yeast killed by whole blood PMNs were distinguished by side scatter and fluorescence, permitting killing estimates. The patterns seen using whole blood was similar to that seen with fractionated PMNs. Data from thalassemia patients showed similar opsonophagocytosis but slightly decreased intracellular killing of yeast cells when compared with normal subjects. This assay provides an alternative method to assess PMN function in small blood samples, which could be especially useful in conditions like thalassemia and pediatric patients. (c) 2007 Interoational society for Artalytical Cytology.
机译:用于定量多形核白细胞(PMN)功能的流式细胞术涉及外周血分级方法。然而,由于它们可能需要大量的血液或因红血球污染而复杂化,因此大多数在诸如儿科和地中海贫血等疾病中用途有限。在全血测定中,将500毫升等分的正常或地中海贫血全血与双羧乙基-羧基荧光素五乙酰氧基甲基酯(BCECF-AM)标记的白色念珠菌细胞和藻红蛋白偶联的抗CD13单克隆抗体一起温育。通过在CD13标记PMN上进行门控并使用流式细胞仪确定吞噬酵母的频率来定量吞噬作用。通过估计PMN裂解后释放的存活荧光的酵母细胞的数量来定量杀伤活性。在正常对照或地中海贫血样品中,非吞噬酵母和带有或不带有吞噬酵母的PMN可以通过两色点图来区分,从而可以估计吞噬作用。全血PMN杀死的活酵母和不活酵母通过侧向散射和荧光进行区分,从而可以估算杀伤力。使用全血观察到的模式类似于使用分级PMN观察到的模式。地中海贫血患者的数据显示相似的调理吞噬作用,但是与正常受试者相比,酵母细胞的细胞内杀伤力略有降低。该测定法提供了另一种方法来评估小血样中的PMN功能,这在地中海贫血和小儿患者等疾病中尤其有用。 (c)2007年国际细胞学细胞学会。

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