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首页> 外文期刊>The Japanese Journal of Veterinary Research >Flow cytometry to evaluate the level of Babesia gibsoni parasitemia in vivo and in vitro by using the fluorescent nucleic acid stain SYTO16
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Flow cytometry to evaluate the level of Babesia gibsoni parasitemia in vivo and in vitro by using the fluorescent nucleic acid stain SYTO16

机译:流式细胞术通过使用荧光核酸染色剂SYTO16在体内和体外评估长柄拟南芥的寄生虫病水平

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摘要

In the present study, we employed flow cytometry to evaluate the level of parasitemia of Babesia gibsoni infecting canine erythrocytes in vivo and in vitro by using fluorescent nucleic acid staining. Peripheral blood samples from a R gibsoni-infected dog and cultured B. gibsoni parasitizing in canine erythrocytes were stained with a membrane-permeable fluorescent nucleic acid stain, SYTO16. In this study, we utilized normal canine erythrocytes (LK erythrocytes) and canine erythrocytes containing high concentrations of potassium, reduced glutathione, and some free amino acids (HK erythrocytes) as host cells for culture. Parasitized cells in vivo were discriminated completely from unparasitized cells and a correlation (r = 0.998) between the percentage of SYTO16-positive cells and parasitemia in vivo was observed. On the other hand, erythrocytes in vitro could not be divided clearly into parasitized and unparasitized cells. However, when LK erythrocytes were used as host cells, the percentage of SYTO16-positive cells was almost the same as, and was well correlated (r = 0.932) with, the level of parasitemia. When HK erythrocytes were used as host cells, the percentage of SYTO16-positive cells was almost half of, but was correlated (r = 0.982) with, the level of parasitemia. Therefore, we attempted to observe the changes in the percentage of parasitized cells after treatment with antiprotozoal drug or mitochondria. inhibitors by using flow cytometry. The changes in the percentage of SYTO16-positive cells corresponded well with the changes of the level of parasitemia when the parasites in HK erythrocytes were cultured with each compound. The present results suggest that flow cytometric detection using SYTO16 is a rapid and reliable method for monitoring parasitemia both in vivo and in vitro.
机译:在本研究中,我们使用流式细胞仪通过荧光核酸染色在体内和体外评估长柄拟南芥感染犬红细胞的寄生虫病水平。用膜透性荧光核酸染料SYTO16对来自R gibsoni感染的狗和寄生在犬红细胞中的培养的B. gibsoni的外周血样品进行染色。在这项研究中,我们利用正常的犬红细胞(LK红细胞)和含有高浓度钾,还原型谷胱甘肽和一些游离氨基酸(HK红细胞)的犬红细胞作为宿主细胞进行培养。将体内的寄生虫细胞与未寄生虫的细胞完全区分开,并观察到SYTO16阳性细胞百分比与体内寄生虫血症之间的相关性(r = 0.998)。另一方面,不能将体外的红细胞清楚地分为寄生的和未寄生的细胞。但是,当将LK红细胞用作宿主细胞时,SYTO16阳性细胞的百分比与寄生虫血症的水平几乎相同,并且高度相关(r = 0.932)。当HK红细胞用作宿主细胞时,SYTO16阳性细胞的百分比几乎是寄生虫血症水平的一半,但与寄生虫血症水平相关(r = 0.982)。因此,我们试图观察用抗原生动物药物或线粒体治疗后被寄生的细胞百分比的变化。通过使用流式细胞仪检测抑制剂。当用每种化合物培养HK红细胞中的寄生虫时,SYTO16阳性细胞百分比的变化与寄生虫血症水平的变化非常吻合。目前的结果表明使用SYTO16的流式细胞仪检测是一种在体内和体外监测寄生虫病的快速,可靠的方法。

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