AstraZeneca India Pvt. Ltd., Bangalore, India.
PLoS One. 2010 Dec 15;5(12):e14336. doi: 10.1371/journal.pone.0014336.
The enzyme Polyphosphate Kinase (PPK) catalyses the reversible transfer of the terminal γ-Pi of ATP to form a long chain Polyphosphate (PolyP). Using an IPTG inducible mycobacterial vector, the vulnerability of this gene has been evaluated by antisense knockdown experiments in M. tuberculosis. Expression profiling studies point to the fact that down regulation of PPK caused cidality during the late phase in contrast to its bacteriostatic mode immediately following antisense expression. PPK thus seems to be a suitable anti-tubercular drug target. The enzyme which is a tetramer has been cloned in E. coli and purified to homogeneity. An enzyme assay suitable for High Throughput Screening was optimized by using the statistical Taguchi protocol and the kinetic parameters determined. The enzyme displayed a strong product inhibition by ADP. In order to accurately estimate the product inhibition, progress curve analysis of the enzyme reaction was monitored. The kinetic equation describing the progress curve was suitably modified by taking into account the product inhibition. The reversible nature of the enzyme indicated a possibility of a two way ATP↔ADP switch operating in the bacteria as a response to its growth requirement.
酶多聚磷酸激酶(PPK)催化 ATP 的末端γ-Pi 的可逆转移,形成长链多聚磷酸盐(PolyP)。使用 IPTG 诱导的分枝杆菌载体,通过分枝杆菌中的反义敲低实验评估了该基因的脆弱性。表达谱研究指出,与反义表达后立即呈现的抑菌模式相反,PPK 的下调会导致晚期阶段的细胞毒性。因此,PPK 似乎是一种合适的抗结核药物靶点。该酶是一个四聚体,已在大肠杆菌中克隆并纯化至均一性。通过使用统计 Taguchi 方案优化了适合高通量筛选的酶测定法,并确定了动力学参数。该酶对 ADP 表现出强烈的产物抑制。为了准确估计产物抑制,监测了酶反应的进展曲线分析。通过考虑产物抑制,对描述进展曲线的动力学方程进行了适当修改。酶的可逆性质表明,作为对其生长需求的响应,细菌中可能存在一种双向 ATP↔ADP 转换的可能性。
