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功能性人谷氨酰胺酶在杆状病毒系统中的表达:亲和纯化、动力学及分子特征分析

Expression of functional human glutaminase in baculovirus system: affinity purification, kinetic and molecular characterization.

作者信息

Campos-Sandoval José A, López de la Oliva Amada R, Lobo Carolina, Segura Juan A, Matés José M, Alonso Francisco J, Márquez Javier

机构信息

Departamento de Biología Molecular y Bioquímica, Laboratorio de Química de Proteínas, Facultad de Ciencias, Universidad de Málaga, 29071 Málaga, Spain.

出版信息

Int J Biochem Cell Biol. 2007;39(4):765-73. doi: 10.1016/j.biocel.2006.12.002. Epub 2006 Dec 21.

DOI:10.1016/j.biocel.2006.12.002
PMID:17267261
Abstract

Glutaminase catalyzes the hydrolysis of glutamine yielding stoichiometric amounts of glutamate plus ammonium ions. In mammals, there are two different genes encoding for glutaminase, known as liver (L) and kidney (K) types. The human L-type isoform expressed in baculovirus yielded functional recombinant enzyme in Sf9 insect cells. A novel affinity chromatography method, based on its specific interaction with a PDZ protein, was developed for purification. Kinetic constants were determined for the purified human isozyme, which showed an allosteric behaviour for glutamine, with a Hill index of 2.7 and S(0.5) values of 32 and 64 mM for high and low P(i) concentrations, respectively. Whereas the protein showed a low P(i) dependence typical for L-type glutaminases, the enzyme was unexpectedly inhibited by glutamate, a kinetic characteristic exclusive of K-type isozymes, and was slightly activated by ammonia, unlike the classical liver enzymes which show an absolute dependence on ammonia. Subcellular fractionation demonstrates that recombinant human glutaminase was targeted to both mitochondria and nucleus, and in both locations the protein was catalytically active. This is the first report of the expression of a functional L-type mammalian glutaminase enzyme. The study also provides a simple and efficient method for affinity purification of the recombinant enzyme. Moreover, the data imply that this human enzyme may represent a new isoform different from classical kidney and liver isozymes.

摘要

谷氨酰胺酶催化谷氨酰胺水解,生成化学计量的谷氨酸和铵离子。在哺乳动物中,有两种不同的基因编码谷氨酰胺酶,即肝型(L)和肾型(K)。在杆状病毒中表达的人L型同工酶在Sf9昆虫细胞中产生了功能性重组酶。基于其与一种PDZ蛋白的特异性相互作用,开发了一种新型亲和层析方法用于纯化。测定了纯化的人同工酶的动力学常数,该同工酶对谷氨酰胺表现出别构行为,高、低无机磷酸(P(i))浓度下的希尔系数为2.7,S(0.5)值分别为32 mM和64 mM。虽然该蛋白表现出典型的L型谷氨酰胺酶对低P(i)的依赖性,但该酶出人意料地受到谷氨酸的抑制,这是K型同工酶独有的动力学特征,并且与绝对依赖氨的经典肝酶不同,该酶受到氨的轻微激活。亚细胞分级分离表明,重组人谷氨酰胺酶定位于线粒体和细胞核,且在这两个位置该蛋白均具有催化活性。这是关于功能性L型哺乳动物谷氨酰胺酶表达的首次报道。该研究还提供了一种简单有效的重组酶亲和纯化方法。此外,数据表明这种人酶可能代表一种不同于经典肾型和肝型同工酶的新同工型。

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