高效液相色谱和流式细胞术分析单层细胞和多细胞球体对阿霉素和甲诺加瑞的摄取。

T J Bichay, E G Adams, W R Inch, W J Adams, J E Brewer, B K Bhuyan
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引用次数: 5

摘要

我们使用高效液相色谱和流式细胞术测量并比较了两种蒽环类药物,甲诺加利(MEN)和阿霉素(ADR),在V79中国地鼠肺成纤维细胞中生长为单层和650微米的多细胞球体。为了比较两种方法测量的球形细胞内药物积累,我们使用标准曲线将流式细胞仪的平均通道荧光转换为以ng/10(6)细胞表示的药物摄取。暴露于任一药物的单层细胞的流式细胞仪平均通道荧光与HPLC测定的细胞内药物蓄积的关系曲线。然后使用该标准曲线将药物暴露球体细胞的平均通道荧光转换为ng/10(6)细胞。我们的研究结果表明,在球体和单层细胞中,相同的细胞内药物积累(通过高效液相色谱测定)并不导致这两种细胞群的细胞荧光发射(通过流式细胞术测定)相等。例如,通过流式细胞术测量,细胞内MEN积累量为650 ng/10(6)个细胞的单层细胞可发出40个单位的荧光。然而,具有相同细胞内聚积的球形细胞发出约80个单位的荧光。这导致通过流式细胞术测量的球体的细胞内MEN摄取比HPLC测量的高2- 3倍。流式细胞术测定的细胞内ADR积累量也高于HPLC法。尽管两种方法在数量上存在差异,但在质量上两种方法都给出了相似的结果。因此,两种技术都表明,在中等药物浓度下,单层药物摄取比球体大得多。(摘要删节250字)
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HPLC and flow cytometric analyses of uptake of adriamycin and menogaril by monolayers and multicell spheroids.

We have used both HPLC and flow cytometry to measure and compare the uptake of two anthracyclines, menogaril (MEN) and Adriamycin (ADR), in V79 Chinese hamster lung fibroblasts grown as monolayers and as 650 microns multicell spheroids. In order to compare intracellular drug accumulation in spheroid cells measured by the two methods, we converted mean channel fluorescence of the flow cytometer to drug uptake expressed as ng/10(6) cells by using a standard curve. The standard curve related the flow cytometric mean channel fluorescence, of monolayer cells exposed to either drug, to the intracellular drug accumulation determined by HPLC. This standard curve was then used to convert the mean channel fluorescence of cells from drug-exposed spheroids to ng/10(6) cells. Our results show that equal intracellular drug accumulation (determined by HPLC) in spheroids and monolayers does not result in equal cellular fluorescence emission (determined by flow cytometry) by these 2 cell populations. For example, monolayer cells with an intracellular MEN accumulation of 650 ng/10(6) cells, emit 40 units of fluorescence as measured by flow cytometry. However, spheroid cells with the same intracellular accumulation emit about 80 units of fluorescence. This results in the intracellular MEN uptake in spheroids measured by flow cytometry being as much as 2- to 3-fold higher than that measured by HPLC. Intracellular ADR accumulation measured by flow cytometry was also higher than that obtained by HPLC. In spite of the quantitative difference between the two methods, qualitatively both methods gave similar results. Thus, both techniques showed that at equal drug concentration in medium drug uptake in monolayers was much greater than in spheroids.(ABSTRACT TRUNCATED AT 250 WORDS)

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