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Effects of multipurpose solutions on the viability and encystment of acanthamoeba determined by flow cytometry

机译:流式细胞仪测定多功能溶液对棘阿米巴活力和包囊的影响

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摘要

Purpose: To evaluate simultaneously the effects of multipurpose contact lens care solution (MPS) on the viability and encystment of Acanthamoeba using flow cytometry. Methods: Viability and encystment rate were evaluated using Acanthamoeba castellanii (ATCC 50514 and ATCC 50370) and three clinical strains of Acanthamoeba spp. isolated from patients with Acanthamoeba keratitis. Acanthamoeba trophozoites (1.0 × 10 cells/mL) were exposed to four kinds of commercially available MPSs for 24 hours. After dispensing the cell suspension into two portions, one portion was stained with 0.004% Congo Red (CR), a fluorescence dye to stain the inner cell wall of cysts, and the other portion was stained with a mixture of Congo Red and 3% sarkosyl (CRS), a detergent to lyse the trophozoites and pseudocysts. Flow cytometric analysis of the treated portions was then carried out on an EPICS ALTRA flow cytometer. The encystment rate and disinfecting efficacies (percentage of rounded trophozoites, "pseudocyst") were calculated by the rates of CR-stained, CR-nonstained, and CRS-stained populations, respectively. Ultrastructural features of resistant (mature or immature) cysts and pseudocysts were observed by transmission electron microscopy. Results: Resistant cysts and rounded trophozoites (pseudocysts) were stained with CR, whereas native (unrounded) trophozoites were not. Resistant cysts were also stained with CRS unlike pseudocysts. Three clinical isolates showed higher resistance and higher encystment rates than two ATCC strains when treated with encystment-positive control solution. Disinfecting efficacy of each MPS was not directly related to each encystment rate. Transmission electron microscopy observations showed basic differences in the ultrastructure of pseudocysts produced by MPSs and resistant cysts. Conclusions: These results suggest that viability and encystment of Acanthamoeba are independent phenomena, and therefore disinfecting efficacy of MPS and encystment rates of Acanthamoeba should be evaluated, respectively. Thus, it is important to evaluate simultaneously the disinfecting efficacies and encystment rates of newly developed premarket MPS using the authors' novel flow cytometric methods.
机译:目的:使用流式细胞仪同时评估多功能隐形眼镜护理液(MPS)对棘阿米巴的生存力和包囊的影响。方法:使用卡氏棘阿米巴(ATCC 50514和ATCC 50370)和三株棘阿米巴属菌株评估活力和包囊率。分离自棘阿米巴角膜炎患者。将棘阿米巴滋养体(1.0×10细胞/ mL)暴露于四种市售MPS 24小时。将细胞悬液分为两部分后,一部分用0.004%刚果红(CR)染色,一种荧光染料可染色囊肿的内壁,另一部分则用刚果红和3%沙克糖基的混合物染色(CRS),用于溶解滋养体和假性囊肿的洗涤剂。然后在EPICS ALTRA流式细胞仪上进行处理部分的流式细胞仪分析。包囊率和消毒效率(圆形滋养体的百分比,“假囊肿”)分别通过CR染色,CR未染色和CRS染色的种群比率来计算。通过透射电子显微镜观察到了耐药性(成熟或未成熟)囊肿和假性囊肿的超微结构特征。结果:抗性囊肿和圆形滋养体(假囊肿)被CR染色,而天然(非圆形)滋养体则没有。与假性囊肿不同,抗性囊肿也用CRS染色。当用包囊阳性对照溶液处理时,三个临床分离株显示出比两个ATCC菌株更高的耐药性和更高的包囊率。每个MPS的消毒效果与每个包囊率没有直接关系。透射电子显微镜观察显示,MPSs和耐药性囊肿产生的假性囊肿的超微结构存在基本差异。结论:这些结果表明棘阿米巴的生存力和包囊是独立的现象,因此应分别评估MPS的消毒效果和棘阿米巴的包囊率。因此,使用作者新颖的流式细胞仪方法同时评估新开发的上市MPS的消毒效果和包囊率非常重要。

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