Campbell B J, Di Shih Y, Forrester L J, Zahler W L
Department of Biochemistry, University of Missouri, Columbia 65212.
Biochim Biophys Acta. 1988 Sep 21;956(2):110-8. doi: 10.1016/0167-4838(88)90256-7.
Purified human renal dipeptidase was shown to exhibit no detectable activity against substrates that are characteristic for other known mammalian peptidases. The enzymic activities that were assayed were: aminopeptidase A, aminopeptidase B, aminopeptidase M, aminopeptidase P, and tripeptidase. A quantitative assay for renal dipeptidase was developed which measures the rate of release of glycine from glycylpeptides by pre-column derivatization of the amino acid with phenylisothiocyanate followed by high-performance liquid chromatography. The ratio of Vmax/Km for a series of dipeptides was used as an index of the enzyme's preference for substrates. According to the data obtained, the enzyme prefers that a bulky, hydrophobic group of the dipeptide be located at the N-terminal position. This suggests that the substrate-binding site of the enzyme may provide a hydrophobic pocket to accommodate the hydrophobic moiety at the N-terminus of the dipeptide. The unsaturated dipeptide substrate, glycyldehydrophenylalanine, was employed in spectrophotometric assays to provide kinetic analyses of enzymic inhibition. The inhibitory effect of dithiothreitol was immediate, and the kinetic data indicated reversible, competitive inhibition. These results suggest that the inhibitor competes with substrate for a coordination site of zinc within the active site of the enzyme. The reaction of renal dipeptidase with the transition-state peptide analog, bestatin, was time dependent, and velocity measurements were made after the inhibitor had been incubated with the enzyme until constant rates were observed. These steady-state rate measurements, made following preincubation of enzyme with inhibitor, were employed to show that bestatin caused apparent non-competitive inhibition of the enzyme. The inhibitory effect of the beta-lactam inhibitor, cilastatin, upon the oligomeric dipeptidase was shown to be competitive. Graphical analysis of this inhibition indicated that the subunits of the enzyme react independently during enzymic catalysis and that the catalytic event is not influenced by cooperativity between sites on the subunits. The conversion of leukotriene D4 to leukotriene E4 in the presence of human renal dipeptidase was demonstrated by HPLC procedures. This bioconversion reaction was quantitated by derivatizing the glycine produced by cleavage of the cysteinylglycine bond and isolating this derivative as a function of time. The relationship between the purified enzyme concentration and enzyme activity against leukotriene D4 was shown to be linear over the enzyme concentration range of 1 ng through 69 ng in this assay.(ABSTRACT TRUNCATED AT 400 WORDS)
纯化的人肾二肽酶对其他已知哺乳动物肽酶特有的底物未表现出可检测到的活性。所检测的酶活性包括:氨肽酶A、氨肽酶B、氨肽酶M、氨肽酶P和三肽酶。开发了一种肾二肽酶的定量测定方法,该方法通过用异硫氰酸苯酯对氨基酸进行柱前衍生,然后进行高效液相色谱法来测量甘氨酰肽中甘氨酸的释放速率。一系列二肽的Vmax/Km比值用作该酶对底物偏好性的指标。根据获得的数据,该酶更倾向于二肽的一个庞大的疏水基团位于N端位置。这表明该酶的底物结合位点可能提供一个疏水口袋来容纳二肽N端的疏水部分。不饱和二肽底物甘氨酰脱氢苯丙氨酸用于分光光度测定,以提供酶抑制的动力学分析。二硫苏糖醇的抑制作用是即时的,动力学数据表明是可逆的竞争性抑制。这些结果表明,抑制剂与底物竞争酶活性位点内锌的配位位点。肾二肽酶与过渡态肽类似物贝抑素的反应是时间依赖性的,在抑制剂与酶孵育直至观察到恒定速率后进行速度测量。在酶与抑制剂预孵育后进行的这些稳态速率测量用于表明贝抑素对该酶产生明显的非竞争性抑制。β-内酰胺抑制剂西司他丁对寡聚二肽酶的抑制作用被证明是竞争性的。对这种抑制的图形分析表明,该酶的亚基在酶催化过程中独立反应,并且催化事件不受亚基位点之间协同作用的影响。通过高效液相色谱法证明了在人肾二肽酶存在下白三烯D4向白三烯E4的转化。通过对由半胱氨酰甘氨酸键裂解产生的甘氨酸进行衍生化,并将该衍生物作为时间的函数进行分离,对这种生物转化反应进行定量。在该测定中,在1 ng至69 ng的酶浓度范围内,纯化的酶浓度与针对白三烯D4的酶活性之间的关系显示为线性。(摘要截短至400字)
