Human leukocyte phagocytosis of zymosan particles measured by flow cytometry.

R Bjerknes, C F Bassøe
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Abstract

Human leukocyte phagocytosis of fluorescein-isothiocyanate (FITC)-labelled zymosan particles was studied by a flow cytometric (FCM) assay allowing discrimination of adhered and ingested zymosan particles. Free zymosan particles, non-phagocytes and phagocytes could be discriminated and quantified by simultaneous registration of fluorescence and light scatter. All leukocytes capable of phagocytosis were phagocytosing, and within 15 min 80% of the zymosan particles were adhered or ingested. Compared to the FITC-fluorescence of free zymosan particles, the mean fluorescence of phagocyte-associated zymosan particles was reduced by about 35%, indicating ingestion and processing of zymosan particles. Abolishing the FITC-fluorescence of extracellular zymosan particles by crystal violet, the number of zymosan particles adhered and ingested could be calculated from FCM measurements of phagocyte fluorescence. This showed that in 15 min 83% of the phagocyte-associated zymosan particles were actually ingested.

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流式细胞术测定人白细胞吞噬酶解颗粒。
用流式细胞术(FCM)研究了人白细胞对异硫氰酸荧光素(FITC)标记的酶酶颗粒的吞噬作用,从而区分粘附和摄入的酶酶颗粒。通过荧光和光散射同时记录,可以对游离酶颗粒、非吞噬细胞和吞噬细胞进行区分和定量。所有能吞噬的白细胞都被吞噬,在15分钟内80%的酶酶颗粒被粘附或摄入。与游离酶聚糖颗粒的fitc荧光相比,吞噬细胞相关酶聚糖颗粒的平均荧光降低了约35%,表明酶聚糖颗粒被摄入和加工。晶体紫去除胞外酶酶颗粒的fitc荧光,通过流式细胞仪测量吞噬细胞的荧光,可以计算粘附和摄入酶酶颗粒的数量。这表明,在15分钟内,83%的吞噬细胞相关酶原颗粒被实际摄入。
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