Cooper A J
J Biol Chem. 1976 Feb 25;251(4):1088-96.
Pulsed Fourier transform proton magnetic resonance spectroscopy was used to study the glutamate-alanine transaminase-catalyzed incorporation of deuterium from solvent deuterium oxide into the alpha and beta positions of L-alanine. It was found that the beta proton resonance signal initially disappears slightly faster than the signal due to the alpha proton, but whereas the alpha proton signal decays exponentially, that due to the beta proton signal does not. Eventually, the rate of decrease of the alpha proton signal becomes greater than that for the beta proton. This change in the relative rates is ascribed to a deuterium isotope effect upon substitution of an alpha proton by a deuteron. Furthermore, as deuterium begins to replace hydrogen, two classes of alanine become distinguishable, i.e. alanine which contains deuterium in the alpha position and hydrogen in the beta position, and alanine which contains hydrogen in the alpha position and deuterium in the beta position. Thus, removal of all 3 beta protons is not contingent upon loss of an alpha proton from the same molecule. The two classes of deuterated alanine may conceivably arise by a scrambling mechanism in which protons are transferred from the alpha to the beta position and vice versa. Present evidence excludes this scramblong mechanism and leads to the conclusion that deuterium incorporation into L-alanine involves, (a) the reversible enzymatic conversion of the classical ketimine enzymes intermediate to an enaminetype structure, and (b) considerable conservation of label during the prototropic shift from the alpha carbon of L-alanine to the C4-position of pyridoxal 5'-phosphate. It is also postulated that alanine binds at the active site in such a way as to bring the beta protons into close contact with a basic group on the enzyme surface. This group is distinct from that used in abstraction of an alpha proton. The beta protons of glutamate are not enzymatically removed; presumably glutamate binds in such a way that the beta protons cannot effectively interact with an enzyme base. Similar studies were carried out on soluble glutamate-aspartate transaminase; no evidence was found for significant enzyme-catalyzed deuterium incorporation into the beta position of L-glutamate, L-aspartate, and L-alanine.
采用脉冲傅里叶变换质子磁共振波谱法研究谷氨酸 - 丙氨酸转氨酶催化将溶剂氧化氘中的氘掺入L - 丙氨酸的α和β位。结果发现,β质子共振信号最初消失的速度略快于α质子的信号,但α质子信号呈指数衰减,而β质子信号并非如此。最终,α质子信号的下降速率变得大于β质子的下降速率。这种相对速率的变化归因于α质子被氘取代时的氘同位素效应。此外,随着氘开始取代氢,两类丙氨酸变得可区分,即α位含氘而β位含氢的丙氨酸,以及α位含氢而β位含氘的丙氨酸。因此,去除所有3个β质子并不取决于同一分子中α质子的丢失。这两类氘代丙氨酸可能通过一种质子转移机制产生,即质子从α位转移到β位,反之亦然。目前的证据排除了这种质子转移机制,并得出结论,氘掺入L - 丙氨酸涉及:(a) 经典酮亚胺酶中间体向烯胺型结构的可逆酶促转化;(b) 在从L - 丙氨酸的α碳向磷酸吡哆醛5'-磷酸的C4位的质子转移过程中,标记的大量保留。还推测丙氨酸以这样一种方式结合在活性位点上,使得β质子与酶表面的一个碱性基团紧密接触。该基团与用于夺取α质子的基团不同。谷氨酸的β质子不会被酶促去除;推测谷氨酸的结合方式使得β质子不能有效地与酶碱相互作用。对可溶性谷氨酸 - 天冬氨酸转氨酶进行了类似的研究;未发现有显著的酶催化氘掺入L - 谷氨酸、L - 天冬氨酸和L - 丙氨酸的β位的证据。
