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恶性疟原虫中的6-磷酸葡糖胺脱氨酶

Glucosamine 6-phosphate deaminase in Plasmodium falciparum.

作者信息

Weidanz J A, Campbell P, Moore D, DeLucas L J, Rodén L, Vezza A C

机构信息

Department of Microbiology, School of Medicine, University of Alabama at Birmingham, USA.

出版信息

Br J Haematol. 1995 Nov;91(3):578-86. doi: 10.1111/j.1365-2141.1995.tb05351.x.

DOI:10.1111/j.1365-2141.1995.tb05351.x
PMID:8555058
Abstract

The pathways of glucose utilization for energy production in the malaria parasite, Plasmodium falciparum, have been studied extensively. Little is known, however, about the reactions by which glucose is converted into complex carbohydrates in the parasite, and knowledge of the catabolism of these substances is likewise scanty. The present investigation was undertaken to determine whether the parasites possess a key enzyme of glucosamine catabolism, i.e. glucosamine 6-phosphate deaminase (EC 5.3.1.40), which catalyses the conversion of the sugar phosphate to fructose 6-phosphate and ammonia. Lysates of Plasmodium-infected erythrocytes had substantially higher deaminase activity than control samples from normal erythrocytes, and an even higher specific activity was observed in extracts of isolated parasites, amounting to 20-40 times that of uninfected cells. Anion exchange chromatography indicated that the parasite deaminase eluted in a retarded position when compared to the elution profile of the erythrocyte enzyme. The charge difference suggested by these findings was established more directly by chromatofocusing, which indicated pI values of 6.85 and 8.55 for the parasite and erythrocyte deaminases, respectively. Other differences were also observed, notably a greater thermolability on the part of the parasite enzyme. These results indicated that the parasites synthesize a specific deaminase that is distinct from the normal erythrocyte enzyme. Studies on synchronized parasite cultures further indicated that the parasite deaminase is developmentally regulated, because a dramatic increase in activity levels occurred during the later stages of parasite development.

摘要

疟原虫(恶性疟原虫)利用葡萄糖产生能量的途径已得到广泛研究。然而,对于疟原虫中葡萄糖转化为复合碳水化合物的反应却知之甚少,而且对这些物质分解代谢的了解同样匮乏。本研究旨在确定疟原虫是否拥有氨基葡萄糖分解代谢的关键酶,即6-磷酸氨基葡萄糖脱氨酶(EC 5.3.1.40),该酶催化磷酸糖转化为6-磷酸果糖和氨。感染疟原虫的红细胞裂解物的脱氨酶活性明显高于正常红细胞的对照样本,在分离出的疟原虫提取物中观察到的比活性甚至更高,达到未感染细胞的20至40倍。阴离子交换色谱表明,与红细胞酶的洗脱图谱相比,疟原虫脱氨酶在一个延迟的位置洗脱。这些发现所暗示的电荷差异通过聚焦色谱更直接地得以证实,聚焦色谱表明疟原虫脱氨酶和红细胞脱氨酶的等电点分别为6.85和8.55。还观察到了其他差异,特别是疟原虫酶的热稳定性较差。这些结果表明,疟原虫合成了一种与正常红细胞酶不同的特异性脱氨酶。对同步化疟原虫培养物的研究进一步表明,疟原虫脱氨酶受到发育调控,因为在疟原虫发育后期活性水平出现了显著增加。

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