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外文期刊>The biochemical journal
>Expression, purification and kinetic characterization of wild-type human ornithine transcarbamylase and a recurrent mutant that produces ‘late onset’ hyperammonaemia
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Expression, purification and kinetic characterization of wild-type human ornithine transcarbamylase and a recurrent mutant that produces ‘late onset’ hyperammonaemia
pOrnithine Transcarbamylase Deficiency, an X-linked disorder, is the most common cause of inherited urea cycle disorders. Approx. 90 mutations that produce reduced levels of ornithine transcarbamylase (OTCase) activity have been identified in patients [Tuchman (1993) Hum. Mutat. b2/b, 174–178; Tuchman and Plante (1995) Hum. Mutat. b5/b, 293–295]. A model of the three-dimensional structure of OTCase, developed on the basis of its homology to the catalytic subunit of iEscherichia coli/i aspartate transcarbamylase (ATCase) [Tuchman, Morizono, Reish, Yuan and Allewell (1995) J. Med. Genet. b32/b, 680–688], and in good agreement with the crystal structure of iPseudomonas aeruginosa/i OTCase [Villeret, Tricot, Stalon and Dideberg (1995) Proc. Natl. Acad. Sci. U.S.A. b92/b, 10762–10766], indicates that many mutations that produce severe clinical symptoms are at the active site or buried in the interior of the protein. However, one of the few recurrent mutations, R277W, an alteration that produces a milder phenotype of ornithine transcarbamylase deficiency, is located in the model in a loop remote from the active site that is analogous to a similar loop (the 2409s loop, a flexible loop of the catalytic chain of iEscherichia coli/iaspartate transcarbamylase, comprised of residues 230–250) of ATCase. Human wild-type OTCase and the R277W mutant have been cloned and overexpressed in iE. coli/i and a rapid and efficient purification method utilizing the bisubstrate analogue, iN/isupΔ/sup-(phosphonacetyl)-l-ornithine, has been developed and used to purify both proteins. Gel chromatography indicates both are trimeric. The pH dependence of the kinetic parameters of the wild-type enzyme is similar to that of iE. coli/i OTCase [Kuo, Herzberg and Lipscomb (1985) Biochemistry b24/b, 4754–4761], suggesting that its catalytic mechanism is similar, although its maximal activity is approx. 10-fold less. Compared with the wild-type, the R277W mutant has nearly 70-fold lower affinity for l-ornithine, shows no substrate inhibition, and its thermal stability is reduced by 5 °C. Its reduced affinity for l-ornithine, which in turn results in lower activity at physiological concentrations of ornithine, as well as its reduced stability, may contribute to the clinical effects that it produces./p
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机译:>鸟氨酸转氨甲酰酶缺乏症(一种与X连锁的疾病)是遗传性尿素循环疾病的最常见原因。大约在患者中已经鉴定出产生降低水平的鸟氨酸转氨甲酰酶(OTCase)活性的90种突变[Tuchman(1993)Hum.Biol.215:403-10。笨蛋 2 ,174-178; Tuchman and Plante(1995)哼。笨蛋 5 ,293-295]。基于OTCase的三维结构模型,该模型基于其与大肠杆菌i。天门冬氨酸转氨甲酰酶(ATCase)催化亚基的同源性而开发[Tuchman,Morizono,Reish,Yuan和Allewell(1995) J. Med。基因 32 ,680–688],并且与铜绿假单胞菌(Pseudomonas aeruginosa )OTCase的晶体结构非常吻合[Villeret,Tricot,Stalon和Dideberg(1995)Proc.Natl.Acad.Sci.USA,95:5873-5877。 Natl。学院科学美国, 92 ,10762–10766],表明产生严重临床症状的许多突变都位于蛋白质的活性位点或内部。但是,少数复发突变之一R277W(一种产生较弱表型鸟氨酸转氨甲酰酶缺乏症的表型的改变)位于模型中远离活动位点的环中,类似于类似的环(2409s环,大肠杆菌天冬氨酸转氨酶的催化链环,由ATCase残基230-250组成。人野生型OTCase和R277W突变体已被克隆并在大肠杆菌中过表达。大肠杆菌和利用双底物类似物 N Δ-(膦酰基乙酰基)-1-鸟氨酸的快速高效纯化方法已被开发并用于纯化这两种蛋白质。凝胶色谱表明两者均为三聚体。野生型酶的动力学参数的pH依赖性与E相似。大肠杆菌OTCase [Kuo,Herzberg and Lipscomb(1985)Biochemistry 24 ,4754–4761],表明其催化机理是相似的,尽管其最大活性约为。少十倍。与野生型相比,R277W突变体对L-鸟氨酸的亲和力低近70倍,没有底物抑制,其热稳定性降低了5°C。它对左旋鸟氨酸的亲和力降低,进而导致在鸟氨酸的生理浓度下活性降低,稳定性降低,可能有助于其产生的临床效果。
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