Department of Pharmacology and the Vanderbilt Institute of Chemical Biology, Vanderbilt University School of Medicine, Nashville, Tennessee 37232, USA.
J Biol Chem. 2010 Dec 17;285(51):39866-75. doi: 10.1074/jbc.M110.155374. Epub 2010 Oct 4.
Epidermal lipoxygenase-3 (eLOX3) exhibits hydroperoxide isomerase activity implicated in epidermal barrier formation, but its potential dioxygenase activity has remained elusive. We identified herein a synthetic fatty acid, 9E,11Z,14Z-20:3ω6, that was oxygenated by eLOX3 specifically to the 9S-hydroperoxide. Reaction showed a pronounced lag phase, which suggested that eLOX3 is deficient in its activation step. Indeed, we found that high concentrations of hydroperoxide activator (e.g. 65 μM) overcame a prolonged lag phase (>1 h) and unveiled a dioxygenase activity with arachidonic acid; the main products were the 5-, 9-, and 7-hydroperoxyeicosatetraenoic acids (HPETEs). These were R/S mixtures (ranging from ∼50:50 to 73:27), and as the bis-allylic 7-HPETE can be formed only inside the enzyme active site, the results indicate there is oxygen availability along either face of the reacting fatty acid radical. That the active site oxygen supply is limited is implied from the need for continuous re-activation, as carbon radical leakage leaves the enzyme in the unactivated ferrous state. An Ala-to-Gly mutation, known to affect the positioning of O(2) in the active site of other lipoxygenase enzymes, led to more readily activated reaction and a significant increase in the 9R- over the 5-HPETE. Activation and cycling of the ferric enzyme are thus promoted using the 9E,11Z,14Z-20:3ω6 substrate, by continuous hydroperoxide activation, or by the Ala-to-Gly mutation. We suggest that eLOX3 represents one end of a spectrum among lipoxygenases where activation is inefficient, favoring hydroperoxide isomerase cycling, with the opposite end represented by readily activated enzymes in which dioxygenase activity is prominent.
表皮脂氧合酶-3(eLOX3)具有过氧化物异构酶活性,与表皮屏障形成有关,但它潜在的双加氧酶活性仍难以捉摸。我们在此鉴定出一种合成脂肪酸,9E,11Z,14Z-20:3ω6,它可被 eLOX3 特异性氧化生成 9S-过氧化物。反应显示出明显的迟滞期,这表明 eLOX3 在其激活步骤中存在缺陷。事实上,我们发现高浓度的过氧化物激活剂(例如 65 μM)可以克服长时间的迟滞期(>1 h),并揭示出具有花生四烯酸的双加氧酶活性;主要产物是 5-、9-和 7-羟过氧二十碳四烯酸(HPETEs)。这些都是 R/S 混合物(范围从约 50:50 到 73:27),由于双烯丙基 7-HPETE 只能在酶活性中心内部形成,因此结果表明在反应脂肪酸自由基的任一侧都有氧气供应。由于自由基泄漏会使酶处于未激活的亚铁状态,需要不断重新激活,这表明活性中心的氧气供应是有限的。已知 Ala-to-Gly 突变会影响其他脂氧合酶酶活性中心的 O(2)定位,它导致反应更容易激活,并使 9R-与 5-HPETE 的比值显著增加。通过连续的过氧化物激活,或通过 Ala-to-Gly 突变,促进了 ferric 酶的激活和循环。因此,我们认为 eLOX3 代表了脂氧合酶中一端的谱,在这一端,激活效率低下,有利于过氧化物异构酶循环,而另一端则是易于激活的酶,其中双加氧酶活性很突出。