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Why do nitric oxide synthases use tetrahydrobiopterin?

机译:为什么一氧化氮合酶使用四氢生物蝶呤?

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We are combining stopped-flow, stop-quench, and rapid-freezing kinetic methods to help clarify the unique redox roles of tetrahydrobiopterin (H4B) in NO synthesis, which occurs via the consecutive oxidation Of L-arginine (Arg) and N-hydroxy-L-arginine (NOHA). In the Arg reaction, H4B radical formation is coupled to reduction of a heme (FeO2)-O-II intermediate. The tempo of this electron transfer is important for coupling (FeO2)-O-II formation to Arg hydroxylation. Because H4B provides this electron faster than can the NOS reductase domain, H4B appears to be a kinetically preferred source of the second electron for oxygen activation during Arg hydroxylation. A conserved Trp (W457 in mouse inducible NOS) has been shown to influence product formation by controlling the kinetics of H,B electron transfer to the (FeO2)-O-II intermediate. This shows that the NOS protein tunes H4B redox function. In the NOHA reaction the role of H4B is more obscure. However, existing evidence suggests that H4B may perform consecutive electron donor and acceptor functions to reduce the (FeO2)-O-II intermediate and then ensure that NO is produced from NOHA. (C) 2002 Elsevier Science Inc. All rights reserved. [References: 37]
机译:我们将停止流,停止淬火和快速冷冻动力学方法相结合,以帮助阐明四氢生物蝶呤(H4B)在NO合成中的独特氧化还原作用,这是通过L-精氨酸(Arg)和N-羟基的连续氧化而发生的-L-精氨酸(NOHA)。在Arg反应中,H4B自由基的形成与血红素(FeO2)-O-II中间体的还原相关。这种电子转移的速度对于将(FeO2)-O-II的形成与Arg羟基化耦合很重要。因为H4B提供此电子的速度比NOS还原酶域更快,所以H4B似乎是Arg羟基化过程中用于氧活化的第二电子的动力学优选来源。保守的Trp(小鼠诱导型NOS中的W457)已显示可通过控制H,B电子转移至(FeO2)-O-II中间体的动力学来影响产物的形成。这表明NOS蛋白调节H4B的氧化还原功能。在NOHA反应中,H4B的作用更加模糊。但是,现有证据表明,H4B可能会执行连续的电子给体和受体功能,以还原(FeO2)-O-II中间体,然后确保NOHA产生NO。 (C)2002 Elsevier Science Inc.保留所有权利。 [参考:37]

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