Nder extreme acidic conditions (pH 4.0) all enzymes experienced a significant loss of activity (greater than 60 ). All the nitrilases investigated displayed less than 50 of their optimal activity under alkaline conditions. The temperature-dependent studies of nitrilase hydrolysis 307538-42-7 showed that AkN, ApN, BgN, KpN, and RjN all had optimal temperatures at 40uC (Figure S5). GpN, RkN and TpN had slightly higher optimal activities at 50uC. At 60uC AcN, GpN and KpN retained more than 50 of their activity at 40uC. AkN, ApN, BgN, RjN, RkN, and TpN demonstrated less thermal stability with a greater than 50 loss in activity at 60uC. At 70uC all nitrilases investigated in this study demonstrated less than 10 activity.Protein Homology Modeling and Docking AnalysisHomology modeling of these nitrilases was performed to determine the active site conformation of these proteins (Figure S8). Models were generated from Pyrococcus abyssi nitrilase (PDB accession code 3IVZ), hypothetical protein from Pyrococcus horikoshii (PDB accession code 1J31) [31,33], AmiF formamidase from Helicobacter pylori (PDB accession code 2E2L), and Mus musculus nitrilase (PDB accession code 2W1V) [34]. Comparative modeling was used to generate the most probable structure of the AcN by the alignment with template sequences, while simultaneously satisfying spatial restraints and local molecular geometry (Figure 5A). Despite varying sequence identity, all nitrilase models demonstrated a characteristic monomer fold and the E, K, and C residues of the catalytic triad presented similar geometry (Figure S9). Finally, the best quality models were chosen for further calculations, molecular modeling, and docking studies. These studies were performed to demonstrate the in silico interactions ?between the enzyme and IDAN. A 60 A3 area around the catalytic triad pocket was defined as the active site [31,34]. The docking of IDAN to the active site of AcN (Figure 5B), indicated a hydrogen ?bond (bond length 2.2 A) between N1 of IDAN and the -SH ?moiety group of C164. A second hydrogen bond (1.8 A) was identified between N1 of IDAN and K130. Docking experiments were also performed with the CCA intermediate (Figure 5C). This ?data revealed a hydrogen bond between CCA and C164 (2.5 A). A second hydrogen bond was observed between the 23148522 nitrogen atom of ?CCA and K130 (2.4 A). These results demonstrate that geometry of the AcN active site can accommodate both IDAN and CCA. To identify structural features which affect IDAN activity, the AcN model was superimposed on models representing other nitrilase families: aromatic nitrilase (RjN) [35], aliphatic nitrilase (RkN) [33], and arylacetonitrilase (AkN) (Table S6) [36], Positions A/B/ C displayed distinct structural conformations in AcN as compared to the other nitrilases (Figure 6A). Sequence analysis of these regions showed several non-conserved and semi-conserved substitutions in these regions (Figure 6B). This data is suggestive that residues in A/B/C position may influence the ITI 007 web substrate specify of these enzymes.IDAN ActivityIDAN activity was assessed to identify nitrilase sequences that were active towards this substrate. Reactions were performed in 10 mL 50 mM potassium phosphate (pH 7.5) containing 0.1 g/L purified nitrilase at 35uC, reactions were initiated upon the addition of 105 mM IDAN. HPLC reference peaks for IDAN, CCA, and IDA were established at 3.2, 4.2, and 8.1 min, respectively. After 2 hours the reaction mixtures were subjected to H.Nder extreme acidic conditions (pH 4.0) all enzymes experienced a significant loss of activity (greater than 60 ). All the nitrilases investigated displayed less than 50 of their optimal activity under alkaline conditions. The temperature-dependent studies of nitrilase hydrolysis showed that AkN, ApN, BgN, KpN, and RjN all had optimal temperatures at 40uC (Figure S5). GpN, RkN and TpN had slightly higher optimal activities at 50uC. At 60uC AcN, GpN and KpN retained more than 50 of their activity at 40uC. AkN, ApN, BgN, RjN, RkN, and TpN demonstrated less thermal stability with a greater than 50 loss in activity at 60uC. At 70uC all nitrilases investigated in this study demonstrated less than 10 activity.Protein Homology Modeling and Docking AnalysisHomology modeling of these nitrilases was performed to determine the active site conformation of these proteins (Figure S8). Models were generated from Pyrococcus abyssi nitrilase (PDB accession code 3IVZ), hypothetical protein from Pyrococcus horikoshii (PDB accession code 1J31) [31,33], AmiF formamidase from Helicobacter pylori (PDB accession code 2E2L), and Mus musculus nitrilase (PDB accession code 2W1V) [34]. Comparative modeling was used to generate the most probable structure of the AcN by the alignment with template sequences, while simultaneously satisfying spatial restraints and local molecular geometry (Figure 5A). Despite varying sequence identity, all nitrilase models demonstrated a characteristic monomer fold and the E, K, and C residues of the catalytic triad presented similar geometry (Figure S9). Finally, the best quality models were chosen for further calculations, molecular modeling, and docking studies. These studies were performed to demonstrate the in silico interactions ?between the enzyme and IDAN. A 60 A3 area around the catalytic triad pocket was defined as the active site [31,34]. The docking of IDAN to the active site of AcN (Figure 5B), indicated a hydrogen ?bond (bond length 2.2 A) between N1 of IDAN and the -SH ?moiety group of C164. A second hydrogen bond (1.8 A) was identified between N1 of IDAN and K130. Docking experiments were also performed with the CCA intermediate (Figure 5C). This ?data revealed a hydrogen bond between CCA and C164 (2.5 A). A second hydrogen bond was observed between the 23148522 nitrogen atom of ?CCA and K130 (2.4 A). These results demonstrate that geometry of the AcN active site can accommodate both IDAN and CCA. To identify structural features which affect IDAN activity, the AcN model was superimposed on models representing other nitrilase families: aromatic nitrilase (RjN) [35], aliphatic nitrilase (RkN) [33], and arylacetonitrilase (AkN) (Table S6) [36], Positions A/B/ C displayed distinct structural conformations in AcN as compared to the other nitrilases (Figure 6A). Sequence analysis of these regions showed several non-conserved and semi-conserved substitutions in these regions (Figure 6B). This data is suggestive that residues in A/B/C position may influence the substrate specify of these enzymes.IDAN ActivityIDAN activity was assessed to identify nitrilase sequences that were active towards this substrate. Reactions were performed in 10 mL 50 mM potassium phosphate (pH 7.5) containing 0.1 g/L purified nitrilase at 35uC, reactions were initiated upon the addition of 105 mM IDAN. HPLC reference peaks for IDAN, CCA, and IDA were established at 3.2, 4.2, and 8.1 min, respectively. After 2 hours the reaction mixtures were subjected to H.