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Cloning and characterization of the ecto-nucleotidase NTPDase3 from rat brain: Predicted secondary structure and relation to other members of the E-NTPDase family and actin

机译:来自大鼠脑的外切核苷酸酶NTPDase3的克隆和表征:预测的二级结构及其与E-NTPDase家族和肌动蛋白其他成员的关系

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摘要

The protein family of ecto-nucleoside triphosphate diphosphohydrolases (E-NTPDase family) contains multiple members that hydrolyze nucleoside 5’-triphosphates and nucleoside 5’-diphosphates with varying preference for the individual type of nucleotide. We report the cloning and functional expression of rat NTPDase3. The rat brain-derived cDNA has an open reading frame of 1590 bp encoding 529 amino acid residues, a calculated molecular mass of 59.1 kDa and predicted N- and C-terminal hydrophobic sequences. It shares 94.3% and 81.7% amino acid identity with the mouse and human NTPDase3, respectively, and is more closely related to cell surface-located than to the intracellularly located members of the enzyme family. The NTPDase3 gene is allocated to chromosome 8q32 and organized into 11 exons. Rat NTPDase3 expressed in CHO cells hydrolyzed both nucleoside triphosphates and nucleoside diphosphates with hydrolysis ratios of ATP:ADP of 5:1 and UTP:UDP of 8:1. After addition of ATP, ADP is formed as an intermediate product that is further hydrolyzed to AMP. The enzyme is preferentially activated by Ca2+ over Mg2+ and reveals an alkaline pH optimum. Immunocytochemistry confirmed expression of heterologously expressed NTPDase3 to the surface of CHO cells. PC12 cells express endogenous surface-located NTPDase3. An immunoblot analysis detects NTPDase3 in all rat brain regions investigated. An alignment of the secondary structure domains of actin conserved within the actin/HSP70/sugar kinase superfamily to those of all members of the NTPDase family reveals apparent similarity. It infers that NTPDases share the two-domain structure with members of this enzyme superfamily.
机译:胞外核苷三磷酸二磷酸水解酶的蛋白质家族(E-NTPDase家族)包含多个成员,它们水解核苷5'-三磷酸和核苷5'-二磷酸,对单个核苷酸类型的偏好不同。我们报告了大鼠NTPDase3的克隆和功能表达。大鼠大脑衍生的cDNA具有1590bp的开放阅读框,编码529个氨基酸残基,计算的分子量为59.1kDa,并预测了N和C端疏水序列。它与小鼠和人NTPDase3分别具有94.3%和81.7%的氨基酸同一性,并且与细胞表面定位的密切相关,而不是与酶家族的细胞内定位的密切相关。 NTPDase3基因被分配到染色体8q32,并组织为11个外显子。在CHO细胞中表达的大鼠NTPDase3水解了三磷酸核苷和二磷酸核苷,ATP:ADP的水解比为5:1,UTP:UDP的水解比为8:1。加入ATP后,形成ADP作为中间产物,其进一步水解成AMP。相对于Mg 2 + ,该酶被Ca 2 + 优先激活,并显示出最适的碱性pH。免疫细胞化学证实了异源表达的NTPDase3在CHO细胞表面的表达。 PC12细胞表达内源性表面定位的NTPDase3。免疫印迹分析在所有研究的大鼠脑区域中检测到NTPDase3。肌动蛋白/ HSP70 /糖激酶超家族中保守的肌动蛋白二级结构域与NTPDase家族所有成员的结构域比对揭示了明显的相似性。它推断NTPDase与该酶超家族成员共享两个结构域的结构。

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