Sullivan Sarah M, Holyoak Todd
Department of Biochemistry and Molecular Biology, The University of Kansas Medical Center, Kansas City, Kansas 66160, USA.
Biochemistry. 2007 Sep 4;46(35):10078-88. doi: 10.1021/bi701038x. Epub 2007 Aug 9.
The structures of the rat cytosolic isoform of phosphoenolpyruvate carboxykinase (PEPCK) reported in the PEPCK-Mn2+, -Mn2+-oxaloacetic acid (OAA), -Mn2+-OAA-Mn2+-guanosine-5'-diphosphate (GDP), and -Mn2+-Mn2+-guanosine-5'-tri-phosphate (GTP) complexes provide insight into the mechanism of phosphoryl transfer and decarboxylation mediated by this enzyme. OAA is observed to bind in a number of different orientations coordinating directly to the active site metal. The Mn2+-OAA and Mn2+-OAA-Mn2+GDP structures illustrate inner-sphere coordination of OAA to the manganese ion through the displacement of two of the three water molecules coordinated to the metal in the holo-enzyme by the C3 and C4 carbonyl oxygens. In the PEPCK-Mn2+-OAA complex, an alternate bound conformation of OAA is present. In this conformation, in addition to the previous interactions, the C1 carboxylate is directly coordinated to the active site Mn2+, displacing all of the waters coordinated to the metal in the holo-enzyme. In the PEPCK-Mn2+-GTP structure, the same water molecule displaced by the C1 carboxylate of OAA is displaced by one of the gamma-phosphate oxygens of the triphosphate nucleotide. The structures are consistent with a mechanism of direct in-line phosphoryl transfer, supported by the observed stereochemistry of the reaction. In the catalytically competent binding mode, the C1 carboxylate of OAA is sandwiched between R87 and R405 in an environment that would serve to facilitate decarboxylation. In the reverse reaction, these two arginines would form the CO2 binding site. Comparison of the Mn2+-OAA-Mn2+GDP and Mn2+-Mn2+GTP structures illustrates a marked difference in the bound conformations of the nucleotide substrates in which the GTP nucleotide is bound in a high-energy state resulting from the eclipsing of all three of the phosphoryl groups along the triphosphate chain. This contrasts a previously determined structure of PEPCK in complex with a triphosphate nucleotide analogue in which the analogue mirrors the conformation of GDP as opposed to GTP. Last, the structures illustrate a correlation between conformational changes in the P-loop, the nucleotide binding site, and the active site lid that are important for catalysis.
磷酸烯醇丙酮酸羧激酶(PEPCK)大鼠胞质同工型在PEPCK-Mn2+、-Mn2+-草酰乙酸(OAA)、-Mn2+-OAA-Mn2+-鸟苷-5'-二磷酸(GDP)和-Mn2+-Mn2+-鸟苷-5'-三磷酸(GTP)复合物中的结构,为深入了解该酶介导的磷酸基转移和脱羧机制提供了线索。观察到OAA以多种不同取向结合,直接与活性位点金属配位。Mn2+-OAA和Mn2+-OAA-Mn2+GDP结构表明,通过C3和C4羰基氧取代全酶中与金属配位的三个水分子中的两个,OAA与锰离子形成内球配位。在PEPCK-Mn2+-OAA复合物中,存在OAA的另一种结合构象。在这种构象中,除了先前的相互作用外,C1羧酸盐直接与活性位点Mn2+配位,取代了全酶中与金属配位的所有水分子。在PEPCK-Mn2+-GTP结构中,被OAA的C1羧酸盐取代的同一个水分子被三磷酸核苷酸的γ-磷酸氧之一取代。这些结构与直接串联磷酸基转移机制一致,该机制得到了观察到的反应立体化学的支持。在催化活性结合模式中,OAA的C1羧酸盐夹在R87和R405之间,所处环境有助于促进脱羧反应。在逆反应中,这两个精氨酸将形成CO2结合位点。Mn2+-OAA-Mn2+GDP和Mn2+-Mn2+GTP结构的比较表明,核苷酸底物的结合构象存在显著差异,其中GTP核苷酸以高能状态结合,这是由于三磷酸链上所有三个磷酸基团相互重叠所致。这与先前确定的PEPCK与三磷酸核苷酸类似物复合物的结构形成对比,在该结构中,类似物反映的是GDP而非GTP的构象。最后,这些结构说明了对催化作用很重要的P环、核苷酸结合位点和活性位点盖子的构象变化之间的相关性。
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