Hsieh Ming-Lung, Tseng Min-Jen, Tseng Ming-Chung, Chu Yen-Ho
Department of Chemistry and Biochemistry, National Chung Cheng University, Chia-Yi, Taiwan 621, Republic of China.
Anal Biochem. 2006 Jul 1;354(1):104-10. doi: 10.1016/j.ab.2006.03.054. Epub 2006 Apr 27.
As one of key bacterial proteins involved in vancomycin resistance, VanX is a D,D-dipeptidase that impedes bacterial cell wall biosynthesis by hydrolyzing the essential D-Ala-D-Ala dipeptide. Based on a report by Crowder and co-workers that L-alanine-p-nitroanilide (L-Ala-pNA) was a useful substrate for continuous assay of VanX, we constructed a library of 35 L- and D-amino acid p-nitroanilides to provide the needed diversity to discover new substrates that are more specific than L-Ala-pNA. We report here that, among all compounds tested, D-leucine-p-nitroanilide (D-Leu-pNA) was found to be the best substrate for VanX enzyme (KM=8.9+/-1.2 mM, kcat=0.0102+/-0.0016 s(-1), kcat/KM=0.0012 mM(-1)s(-1)). Although it is catalytically inefficient, this new VanX substrate needs essentially no sophisticated synthetic chemistry for preparation and therefore offers a convenient means for routine analysis of enzyme catalysis and the screening of potential inhibitors. Moreover, because it is the uncommon leucine in its D form in D-Leu-pNA, enzymatic activities due to other contaminated species in Escherichia coli used for VanX overproduction should be greatly reduced.
作为参与万古霉素耐药性的关键细菌蛋白之一,VanX是一种D,D-二肽酶,通过水解必需的D-丙氨酰-D-丙氨酸二肽来阻碍细菌细胞壁的生物合成。基于Crowder及其同事的一份报告,即L-丙氨酸对硝基苯胺(L-Ala-pNA)是连续测定VanX的有用底物,我们构建了一个包含35种L-和D-氨基酸对硝基苯胺的文库,以提供所需的多样性,从而发现比L-Ala-pNA更具特异性的新底物。我们在此报告,在所有测试的化合物中,发现D-亮氨酸对硝基苯胺(D-Leu-pNA)是VanX酶的最佳底物(KM = 8.9±1.2 mM,kcat = 0.0102±0.0016 s(-1),kcat/KM = 0.0012 mM(-1)s(-1))。尽管其催化效率不高,但这种新的VanX底物在制备时基本上不需要复杂的合成化学方法,因此为酶催化的常规分析和潜在抑制剂的筛选提供了一种便捷的手段。此外,由于D-Leu-pNA中其D形式的亮氨酸不常见,用于过量生产VanX的大肠杆菌中其他污染物种引起的酶活性应会大大降低。
