Schumacher Maria A, Bashor Caleb J, Song Minsun Hong, Otsu Kanao, Zhu Shuren, Parry Ronald J, Ullman Buddy, Brennan Richard G
Department of Biochemistry and Molecular Biology, Oregon Health and Science University, 3181 Southwest Sam Jackson Park Road, Portland, OR 97201-3098, USA.
Proc Natl Acad Sci U S A. 2002 Jan 8;99(1):78-83. doi: 10.1073/pnas.012399599. Epub 2002 Jan 2.
Uracil phosphoribosyltransferase (UPRT) is a member of a large family of salvage and biosynthetic enzymes, the phosphoribosyltransferases, and catalyzes the transfer of ribose 5-phosphate from alpha-d-5-phosphoribosyl-1-pyrophosphate (PRPP) to the N1 nitrogen of uracil. The UPRT from the opportunistic pathogen Toxoplasma gondii represents a promising target for rational drug design, because it can create intracellular, lethal nucleotides from subversive substrates. However, the development of such compounds requires a detailed understanding of the catalytic mechanism. Toward this end we determined the crystal structure of the T. gondii UPRT bound to uracil and cPRPP, a nonhydrolyzable PRPP analogue, to 2.5-A resolution. The structure suggests that the catalytic mechanism is substrate-assisted, and a tetramer would be the more active oligomeric form of the enzyme. Subsequent biochemical studies revealed that GTP binding, which has been suggested to play a role in catalysis by other UPRTs, causes a 6-fold activation of the T. gondii enzyme and strikingly stabilizes the tetramer form. The basis for stabilization was revealed in the 2.45-A resolution structure of the UPRT-GTP complex, whereby residues from three subunits contributed to GTP binding. Thus, our studies reveal an allosteric mechanism involving nucleotide stabilization of a more active, higher order oligomer. Such regulation of UPRT could play a role in the balance of purine and pyrimidine nucleotide pools in the cell.
尿嘧啶磷酸核糖转移酶(UPRT)是补救和生物合成酶大家族——磷酸核糖转移酶家族的一员,它催化5-磷酸核糖从α-d-5-磷酸核糖-1-焦磷酸(PRPP)转移至尿嘧啶的N1氮原子上。机会性致病原刚地弓形虫的UPRT是合理药物设计的一个有前景的靶点,因为它能利用颠覆性底物生成细胞内致死性核苷酸。然而,开发此类化合物需要详细了解其催化机制。为此,我们测定了与尿嘧啶和cPRPP(一种不可水解的PRPP类似物)结合的刚地弓形虫UPRT的晶体结构,分辨率达到2.5埃。该结构表明其催化机制是底物辅助型的,并且四聚体可能是该酶更具活性的寡聚形式。随后的生化研究表明,GTP结合(已表明它在其他UPRT的催化中起作用)会使刚地弓形虫酶激活6倍,并显著稳定四聚体形式。在UPRT-GTP复合物2.45埃分辨率的结构中揭示了稳定化的基础,即来自三个亚基的残基参与了GTP结合。因此,我们的研究揭示了一种变构机制,涉及更具活性的高阶寡聚体的核苷酸稳定作用。UPRT的这种调节可能在细胞嘌呤和嘧啶核苷酸库的平衡中发挥作用。