Jin Yi, Cooper William C, Penning Trevor M
Department of Pharmacology, University of Pennsylvania School of Medicine, 3620 Hamilton Walk, Philadelphia, PA 19104-6084, USA.
Chem Biol Interact. 2003 Feb 1;143-144:383-92. doi: 10.1016/s0009-2797(02)00207-7.
Human 3alpha-hydroxysteroid dehydrogenases (HSDs) are potential drug targets since they regulate the occupancy and trans-activation of steroid hormone receptors by interconverting potent hormones with their cognate inactive metabolites. The human isoforms (AKR1C1-4) are all members of the aldo-keto reductase superfamily and display distinctive differences in steroid specificity and catalytic efficiency when compared with the closely related and more extensively studied rat 3alpha-HSD (AKR1C9). Specifically, AKR1C1-4 display 3alpha-, 17beta- and 20alpha-HSD activities to varying degrees whereas AKR1C9 is positional- and stereo-specific for the 3alpha-HSD reaction. In addition, AKR1C1-4 isoforms have significantly lower catalytic efficiencies (k(cat)/K(m)) than AKR1C9 and this is largely due to a lower k(cat). To understand these functional differences, human type 3 3alpha-HSD (AKR1C2) was studied as a representative human 3alpha-HSD. Comparison of the crystal structure of AKR1C2-NADP(+)-ursodeoxycholate ternary complex (3.0 A) with that of the AKR1C9-NADP(+)-testosterone ternary complex (2.8 A) demonstrates the expected conservancy in overall structure and active site topology. More interestingly, it reveals striking differences in the structure of the steroid binding pockets of the two enzymes and shows how ursodeoxycholate binds 'backwards' and 'upside-down' with respect to testosterone. This difference in steroid binding provides a structural basis for the broad positional specificity of AKR1C2 and the exquisite stereospecificity of AKR1C9. To determine why AKR1C2 has a much lower k(cat) than AKR1C9, the events associated with the binding of cofactor to both enzymes were studied by steady state fluorescence titration and stopped-flow experiments. Comparable K(d) values for E-NADP(H) and k(obs) values for the fluorescence transients were obtained for the two enzymes. These data are consistent with both enzymes binding NADP(H) in a conserved manner which is supported by the available crystal structures. The results suggest that cofactor binding or release for the human and rat 3alpha-HSDs are similar and do not account for the observed differences in k(cat).
人类3α-羟基类固醇脱氢酶(HSDs)是潜在的药物靶点,因为它们通过将强效激素与其相应的无活性代谢物相互转化,来调节类固醇激素受体的占有率和反式激活。人类同工型(AKR1C1 - 4)均为醛糖还原酶超家族的成员,与密切相关且研究更为广泛的大鼠3α-HSD(AKR1C9)相比,它们在类固醇特异性和催化效率上表现出显著差异。具体而言,AKR1C1 - 4在不同程度上表现出3α-、17β-和20α-HSD活性,而AKR1C9对3α-HSD反应具有位置特异性和立体特异性。此外,AKR1C1 - 4同工型的催化效率(k(cat)/K(m))明显低于AKR1C9,这主要是由于k(cat)较低。为了解这些功能差异,以人类3型3α-HSD(AKR1C2)作为代表性的人类3α-HSD进行了研究。将AKR1C2 - NADP(+) - 熊去氧胆酸盐三元复合物(3.0 Å)的晶体结构与AKR1C9 - NADP(+) - 睾酮三元复合物(2.8 Å)的晶体结构进行比较,结果表明在整体结构和活性位点拓扑结构上存在预期的保守性。更有趣的是,它揭示了两种酶的类固醇结合口袋结构存在显著差异,并展示了熊去氧胆酸盐相对于睾酮是如何“反向”和“颠倒”结合的。这种类固醇结合的差异为AKR1C2广泛的位置特异性和AKR1C9精确的立体特异性提供了结构基础。为了确定为什么AKR1C2的k(cat)比AKR1C9低得多,通过稳态荧光滴定和停流实验研究了与辅因子结合到两种酶上相关的事件。两种酶获得了可比的E - NADP(H)的K(d)值和荧光瞬变的k(obs)值。这些数据与两种酶以保守方式结合NADP(H)一致,现有晶体结构也支持这一点。结果表明,人类和大鼠3α-HSD的辅因子结合或释放相似,无法解释观察到的k(cat)差异。
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