Evdokimov Alexey A, Zinoviev Victor V, Malygin Ernst G, Schlagman Samuel L, Hattman Stanley
Institute of Molecular Biology, State Research Center of Virology and Biotechnology Vector, Novosibirsk 630559, Russia.
J Biol Chem. 2002 Jan 4;277(1):279-86. doi: 10.1074/jbc.M108864200. Epub 2001 Oct 30.
We carried out a steady state kinetic analysis of the bacteriophage T4 DNA-[N6-adenine]methyltransferase (T4 Dam) mediated methyl group transfer reaction from S-adenosyl-l-methionine (AdoMet) to Ade in the palindromic recognition sequence, GATC, of a 20-mer oligonucleotide duplex. Product inhibition patterns were consistent with a steady state-ordered bi-bi mechanism in which the order of substrate binding and product (methylated DNA, DNA(Me) and S-adenosyl-l-homocysteine, AdoHcy) release was AdoMet downward arrow DNA downward arrow DNA(Me) upward arrow AdoHcy upward arrow. A strong reduction in the rate of methylation was observed at high concentrations of the substrate 20-mer DNA duplex. In contrast, increasing substrate AdoMet concentration led to stimulation in the reaction rate with no evidence of saturation. We propose the following model. Free T4 Dam (initially in conformational form E) randomly interacts with substrates AdoMet and DNA to form a ternary T4 Dam-AdoMet-DNA complex in which T4 Dam has isomerized to conformational state F, which is specifically adapted for catalysis. After the chemical step of methyl group transfer from AdoMet to DNA, product DNA(Me) dissociates relatively rapidly (k(off) = 1.7 x s(-1)) from the complex. In contrast, dissociation of product AdoHcy proceeds relatively slowly (k(off) = 0.018 x s(-1)), indicating that its release is the rate-limiting step, consistent with kcat = 0.015 x s(-1). After AdoHcy release, the enzyme remains in the F conformational form and is able to preferentially bind AdoMet (unlike form E, which randomly binds AdoMet and DNA), and the AdoMet-F binary complex then binds DNA to start another methylation cycle. We also propose an alternative pathway in which the release of AdoHcy is coordinated with the binding of AdoMet in a single concerted event, while T4 Dam remains in the isomerized form F. The resulting AdoMet-F binary complex then binds DNA, and another methylation reaction ensues. This route is preferred at high AdoMet concentrations.
我们对噬菌体T4 DNA - [N6 - 腺嘌呤]甲基转移酶(T4 Dam)介导的甲基基团从S - 腺苷 - L - 甲硫氨酸(AdoMet)转移至20聚体寡核苷酸双链体回文识别序列GATC中的腺嘌呤(Ade)的反应进行了稳态动力学分析。产物抑制模式符合稳态有序双底物双产物机制,其中底物结合和产物(甲基化DNA,DNA(Me)和S - 腺苷 - L - 高半胱氨酸,AdoHcy)释放的顺序为AdoMet→DNA→DNA(Me)→AdoHcy→。在高浓度的底物20聚体DNA双链体存在下,观察到甲基化速率大幅降低。相反,增加底物AdoMet浓度会导致反应速率增加,且无饱和迹象。我们提出以下模型。游离的T4 Dam(最初处于构象形式E)随机与底物AdoMet和DNA相互作用,形成三元T4 Dam - AdoMet - DNA复合物,其中T4 Dam已异构化为构象状态F,该状态特别适合催化作用。在甲基基团从AdoMet转移至DNA的化学步骤之后,产物DNA(Me)相对快速地(k(off) = 1.7×s(-1))从复合物中解离。相反,产物AdoHcy的解离相对较慢(k(off) = 0.018×s(-1)),表明其释放是限速步骤,这与kcat = 0.015×s(-1)一致。AdoHcy释放后,酶保持在F构象形式,并且能够优先结合AdoMet(与随机结合AdoMet和DNA的E形式不同),然后AdoMet - F二元复合物结合DNA以开始另一个甲基化循环。我们还提出了另一种途径,其中AdoHcy的释放与AdoMet的结合在单个协同事件中协调进行,而T4 Dam保持异构化形式F。由此产生的AdoMet - F二元复合物然后结合DNA,并发生另一个甲基化反应。在高AdoMet浓度下,这条途径更受青睐。
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