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恶性疟原虫和人类红细胞的标记酶作为寄生虫纯度的指标。

Marker enzymes of Plasmodium falciparum and human erythrocytes as indicators of parasite purity.

作者信息

Vander Jagt D L, Intress C, Heidrich J E, Mrema J E, Rieckmann K H, Heidrich H G

出版信息

J Parasitol. 1982 Dec;68(6):1068-71.

PMID:6757398
Abstract

Plasmodium falciparum trophozoites, isolated by mechanical rupture of infected human erythrocytes, were analyzed for purity by determination of the specific activities of a number of marker enzymes selected for high activity, stability, and convenience of assay procedures. The specific activities of the soluble enzymes lactate dehydrogenase and malate dehydrogenase were much higher in the parasite than in the erythrocyte. The soluble enzyme glutamate dehydrogenase (NADP+) was specific for the parasite. Samples of 100,000 g supernate obtained from parasites that appeared to be free from contaminating erythrocytes consistently showed specific activities of about 4, 3 and 0.1 mumole/min/mg for lactate dehydrogenase, malate dehydrogenase and glutamate dehydrogenase, respectively. Moreover, preparations of parasites that exhibit these specific activities showed low acetylcholine esterase activity in the membrane fractions. The specific activities of these soluble marker enzymes did not appear to be strain dependent. A preparation of highly purified trophozoites obtained by free flow electrophoresis and analyzed for purity by electron microscopy exhibited the same specific activities for these marker enzymes. The use of specific activities of selected marker enzymes should be very useful for determining the purity of preparation of parasites when used in conjunction with other methods.

摘要

通过机械破碎感染的人类红细胞分离得到的恶性疟原虫滋养体,通过测定多种因活性高、稳定性好且检测程序简便而挑选出的标记酶的比活性来分析其纯度。寄生虫中可溶性酶乳酸脱氢酶和苹果酸脱氢酶的比活性远高于红细胞中的比活性。可溶性酶谷氨酸脱氢酶(NADP+)是寄生虫特有的。从看似无红细胞污染的寄生虫中获得的100,000g上清液样本,乳酸脱氢酶、苹果酸脱氢酶和谷氨酸脱氢酶的比活性分别始终约为4、3和0.1微摩尔/分钟/毫克。此外,表现出这些比活性的寄生虫制剂在膜部分显示出低乙酰胆碱酯酶活性。这些可溶性标记酶的比活性似乎不依赖于菌株类型。通过自由流动电泳获得的高度纯化滋养体制剂,并通过电子显微镜分析其纯度,这些标记酶表现出相同的比活性。当与其他方法结合使用时,所选标记酶的比活性对于确定寄生虫制剂的纯度应该非常有用。

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