Kuo L C, Miller A W, Lee S, Kozuma C
Department of Chemistry, Boston University, Massachusetts 02215.
Biochemistry. 1988 Nov 29;27(24):8823-32. doi: 10.1021/bi00424a021.
In the carbamoyl-transfer reaction catalyzed by ornithine transcarbamoylase, an arginine residue in the active site of the Escherichia coli enzyme has been suggested to bind the phosphate moiety of the substrate carbamoyl phosphate. With the application of site-specific mutagenesis, the most likely arginine residue among three candidates at the binding site of carbamoyl phosphate, Arg-57, has been replaced with a glycine. The resultant Gly-57 mutant enzyme is drastically inefficient in catalysis. In the synthesis of L-citrulline from carbamoyl phosphate and L-ornithine with the release of inorganic phosphate, the turnover rate of the mutant is 21,000-fold lower than that of the wild type. However, the mutation of Arg-57 affects only moderately the binding of carbamoyl phosphate; the dissociation constant of this substrate, measured under steady-state turnover condition, is increased from 0.046 to 3.2 mM by the mutation. On the other hand, ornithine binding is substantially affected as estimated by the change in the dissociation constant of its analogue L-norvaline. The dissociation constant of L-norvaline increases about 500-fold from 54 microM for the wild type to 25 mM for the mutant. Since Arg-57 is expected to be distal from the ornithine site and the amino acid (both ornithine and norvaline) binds only after carbamoyl phosphate in the wild-type reaction, the poor norvaline affinity to the mutant suggests that Arg-57 is involved in interactions essential for productive addition of the amino acid. This interpretation is supported by difference ultraviolet absorption spectra which show that the conformational changes induced in the wild type by carbamoyl phosphate upon binding are absent in the mutant. Furthermore, steady-state kinetic data reveal that the ordered binding mechanism of the wild-type enzyme is transformed into a random binding mechanism in the mutant. Thus, the presence of carbamoyl phosphate in the mutant active site is no longer a requisite for ornithine binding. In the 5-50 degrees C temperature range, transcarbamoylation catalyzed by either the wild type or the mutant observes the Arrhenius rate law with almost identical enthalpies of activation, 11 and 10 kcal/mol, respectively. The entropy of activation is -5.5 eu for the wild-type reaction and -29 eu for the mutant reaction, accounting for a loss of 6-7 kcal/mol in the rate-determining step of the enzymic reaction.(ABSTRACT TRUNCATED AT 400 WORDS)
在鸟氨酸转氨甲酰酶催化的氨甲酰基转移反应中,有人提出大肠杆菌酶活性位点中的一个精氨酸残基可结合底物氨甲酰磷酸的磷酸部分。通过位点特异性诱变,在氨甲酰磷酸结合位点的三个候选精氨酸残基中,最有可能的Arg - 57已被甘氨酸取代。所得的Gly - 57突变酶催化效率极低。在由氨甲酰磷酸和L - 鸟氨酸合成L - 瓜氨酸并释放无机磷酸的过程中,突变体的周转速率比野生型低21,000倍。然而,Arg - 57的突变仅对氨甲酰磷酸的结合有中等程度的影响;在稳态周转条件下测量的该底物的解离常数因突变从0.046 mM增加到3.2 mM。另一方面,根据其类似物L - 正缬氨酸解离常数的变化估计,鸟氨酸的结合受到显著影响。L - 正缬氨酸的解离常数从野生型的54 microM增加约500倍至突变体的25 mM。由于预计Arg - 57距离鸟氨酸位点较远,且在野生型反应中氨基酸(鸟氨酸和正缬氨酸)仅在氨甲酰磷酸之后结合,因此突变体对正缬氨酸的亲和力较差表明Arg - 57参与了氨基酸有效添加所必需的相互作用。差异紫外吸收光谱支持了这一解释,该光谱表明突变体中不存在野生型因结合氨甲酰磷酸而诱导的构象变化。此外,稳态动力学数据表明,野生型酶的有序结合机制在突变体中转变为随机结合机制。因此,突变体活性位点中氨甲酰磷酸的存在不再是鸟氨酸结合的必要条件。在5 - 50℃温度范围内,野生型或突变体催化的转氨甲酰化反应均遵循阿伦尼乌斯速率定律,活化焓几乎相同,分别为11和10 kcal/mol。野生型反应的活化熵为 - 5.5 eu,突变体反应的活化熵为 - 29 eu,这说明在酶促反应的速率决定步骤中损失了6 - 7 kcal/mol。(摘要截短至400字)
