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Nudix家族的哺乳动物NADH二磷酸酶:人类过氧化物酶体NUDT12蛋白的克隆与特性分析

Mammalian NADH diphosphatases of the Nudix family: cloning and characterization of the human peroxisomal NUDT12 protein.

作者信息

Abdelraheim Salama R, Spiller David G, McLennan Alexander G

机构信息

Cell Regulation and Signalling Group, School of Biological Sciences, University of Liverpool, Liverpool L69 7ZB, UK.

出版信息

Biochem J. 2003 Sep 1;374(Pt 2):329-35. doi: 10.1042/BJ20030441.

Abstract

The human NUDT12 Nudix hydrolase has been expressed in insect cells from a baculovirus vector as a His-tagged recombinant protein. In vitro, it efficiently hydrolyses NAD(P)H to NMNH and AMP (2',5'-ADP), and diadenosine diphosphate to AMP. It also has activity towards NAD(P)(+), ADP-ribose and diadenosine triphosphate. K (m) values for NADH, NADPH and NAD(+) are 11, 16 and 190 microM and k (cat) values are 11, 16 and 10.5 s(-1) respectively. Thus, like other NADH diphosphatases of the Nudix family, NUDT12 has a marked substrate preference for the reduced nicotinamide nucleotides. Optimal activity was supported by 50 microM Mn(2+) ions in vitro, with 3-fold lower activity at 0.4 mM Mg(2+). Expression of NUDT12 as a C-terminal fusion to green fluorescent protein revealed that it was targeted to peroxisomes by the C-terminal tripeptide PNL acting as a novel type 1 peroxisomal targeting signal. Deletion of PNL resulted in diffuse cellular fluorescence. In addition, C-terminal, but not N-terminal, fusions with or without the PNL signal accumulated in large, unidentified cytoplasmic structures. NUDT12 may act to regulate the concentration of peroxisomal nicotinamide nucleotide cofactors required for oxidative metabolism in this organelle.

摘要

人NUDT12 Nudix水解酶已通过杆状病毒载体在昆虫细胞中表达为带有His标签的重组蛋白。在体外,它能有效地将NAD(P)H水解为NMNH和AMP(2',5'-ADP),并将二腺苷二磷酸水解为AMP。它对NAD(P)(+)、ADP-核糖和二腺苷三磷酸也有活性。NADH、NADPH和NAD(+)的K(m)值分别为11、16和190 microM,k(cat)值分别为11、16和10.5 s(-1)。因此,与Nudix家族的其他NADH二磷酸酶一样,NUDT12对还原型烟酰胺核苷酸有明显的底物偏好。体外50 microM Mn(2+)离子可支持最佳活性,在0.4 mM Mg(2+)时活性低3倍。NUDT12作为绿色荧光蛋白的C末端融合蛋白表达表明,它通过C末端三肽PNL作为新型1型过氧化物酶体靶向信号靶向过氧化物酶体。删除PNL会导致细胞荧光弥漫。此外,带有或不带有PNL信号的C末端融合蛋白(而非N末端融合蛋白)会在大型未识别的细胞质结构中积累。NUDT12可能起到调节该细胞器氧化代谢所需的过氧化物酶体烟酰胺核苷酸辅因子浓度的作用。

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本文引用的文献

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