Institut für Pharmakologie und Toxikologie, Medizinische Fakultät, Ruhr-Universität-Bochum, Bochum, Germany.
Br J Pharmacol. 2010 Dec;161(7):1645-60. doi: 10.1111/j.1476-5381.2010.00977.x.
By controlling intracellular cyclic nucleotide levels, phosphodiesterases (PDE) serve important functions within various signalling pathways. The PDE2 and PDE5 families are allosterically activated by their substrate cGMP via regulatory so-called GAF domains. Here, we set out to identify synthetic ligands for the GAF domains of PDE2 and PDE5.
Using fluorophore-tagged, isolated GAF domains of PDE2 and PDE5, promising cGMP analogues were selected. Subsequently, the effects of these analogues on the enzymatic activity of PDE2 and PDE5 were analysed.
The PDE2 ligands identified, 5,6-DM-cBIMP and 5,6-DCl-cBIMP, caused pronounced, up to 40-fold increases of the cAMP- and cGMP-hydrolysing activities of PDE2. The ligand for the GAF domains of PDE5, 8-Br-cGMP, elicited a 20-fold GAF-dependent activation and moreover revealed a time-dependent increase in PDE5 activity that occurred independently of a GAF ligand. Although GAF-dependent PDE5 activation was fast at high ligand concentrations, it was slow at physiologically relevant cGMP concentrations; PDE5 reached its final catalytic rates at 1µM cGMP after approximately 10min.
We conclude that the delayed activation of PDE5 is required to shape biphasic, spike-like cGMP signals. Phosphorylation of PDE5 further enhances activity and conserves PDE5 activation, thereby enabling PDE5 to act as a molecular memory balancing cGMP responses to nitric oxide or natriuretic peptide signals.
通过控制细胞内环核苷酸水平,磷酸二酯酶(PDE)在各种信号通路中发挥重要作用。PDE2 和 PDE5 家族均可通过其底物 cGMP 对调节性所谓的 GAF 结构域进行变构激活。在此,我们旨在鉴定 PDE2 和 PDE5 的 GAF 结构域的合成配体。
使用荧光标记的 PDE2 和 PDE5 的分离 GAF 结构域,选择有前景的 cGMP 类似物。随后,分析这些类似物对 PDE2 和 PDE5 的酶活性的影响。
鉴定出的 PDE2 配体 5,6-DM-cBIMP 和 5,6-DCl-cBIMP 导致 PDE2 的 cAMP 和 cGMP 水解活性显著增加,最高可达 40 倍。PDE5 的 GAF 结构域配体 8-Br-cGMP 引起 20 倍的 GAF 依赖性激活,此外还显示 PDE5 活性的时间依赖性增加,这种增加独立于 GAF 配体。虽然在高配体浓度下 GAF 依赖性 PDE5 激活很快,但在生理相关的 cGMP 浓度下较慢;PDE5 在大约 1µM cGMP 后经过 10 分钟达到其最终的催化速率。
我们得出结论,PDE5 的延迟激活对于形成双相、尖峰样 cGMP 信号是必需的。PDE5 的磷酸化进一步增强了其活性并保存了 PDE5 的激活,从而使 PDE5 能够作为一种分子记忆,平衡一氧化氮或利钠肽信号对 cGMP 反应。