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. 2020 Mar 16;295(18):6165–6176. doi: 10.1074/jbc.RA120.012793

Figure 3.

Figure 3.

The AbNadE2 activity is down-regulated by NAD+ and GlnZ relives AbNadE2 from NAD+ inhibition. NadE2 discontinuous assays were performed to measure the formation of PPi in the presence of 4 mm l-glutamine, 4 mm ATP, and 2 mm NaAD. Data were plotted as relative percent activity considering the reaction without NAD+ as 100% activity. A, effect of redox metabolites, when indicated 2.5 mm NAD+ or 1 mm of NADH, NADP+ or NADPH were added. An asterisk indicates statistically significant difference (t test, p < 0.01), n = 3. B, reactions were carried out in the presence of 100 nm NadE2Ab (monomer), GlnZ was added at 2 μm (trimer) when indicated. Reactions without GlnZ were contained 2 μm BSA. The calculated AbNadE2 NAD+ Ki was 1 mm and 2.5 mm in the absence and presence of GlnZ, respectively. Data were analyzed and the IC50 were calculated by nonlinear regression in GraphPad Prism 7. S. D. from triplicate experiments are indicated by error bars.