2ZMA
Crystal Structure of 6-Aminohexanoate-dimer Hydrolase S112A/G181D/H266N/D370Y Mutant with Substrate
Summary for 2ZMA
| Entry DOI | 10.2210/pdb2zma/pdb |
| Related | 1WYB 1WYC 2DCF 2E8I 2ZM7 2ZM8 2ZM9 |
| Descriptor | 6-aminohexanoate-dimer hydrolase, SULFATE ION, 6-AMINOHEXANOIC ACID, ... (6 entities in total) |
| Functional Keywords | hydrolase, nylon degradation |
| Biological source | Flavobacterium sp. More |
| Total number of polymer chains | 1 |
| Total formula weight | 44303.94 |
| Authors | Ohki, T.,Shibata, N.,Higuchi, Y.,Takeo, M.,Negoro, S. (deposition date: 2008-04-14, release date: 2009-04-07, Last modification date: 2023-11-15) |
| Primary citation | Kawashima, Y.,Ohki, T.,Shibata, N.,Higuchi, Y.,Wakitani, Y.,Matsuura, Y.,Nakata, Y.,Takeo, M.,Kato, D.,Negoro, S. Molecular design of a nylon-6 byproduct-degrading enzyme from a carboxylesterase with a beta-lactamase fold Febs J., 276:2547-2556, 2009 Cited by PubMed Abstract: A carboxylesterase with a beta-lactamase fold from Arthrobacter possesses a low level of hydrolytic activity (0.023 mumol.min(-1).mg(-1)) when acting on a 6-aminohexanoate linear dimer byproduct of the nylon-6 industry (Ald). G181D/H266N/D370Y triple mutations in the parental esterase increased the Ald-hydrolytic activity 160-fold. Kinetic studies showed that the triple mutant possesses higher affinity for the substrate Ald (K(m) = 2.0 mm) than the wild-type Ald hydrolase from Arthrobacter (K(m) = 21 mm). In addition, the k(cat)/K(m) of the mutant (1.58 s(-1).mm(-1)) was superior to that of the wild-type enzyme (0.43 s(-1).mm(-1)), demonstrating that the mutant efficiently converts the unnatural amide compounds even at low substrate concentrations, and potentially possesses an advantage for biotechnological applications. X-ray crystallographic analyses of the G181D/H266N/D370Y enzyme and the inactive S112A-mutant-Ald complex revealed that Ald binding induces rotation of Tyr370/His375, movement of the loop region (N167-V177), and flip-flop of Tyr170, resulting in the transition from open to closed forms. From the comparison of the three-dimensional structures of various mutant enzymes and site-directed mutagenesis at positions 266 and 370, we now conclude that Asn266 makes suitable contacts with Ald and improves the electrostatic environment at the N-terminal region of Ald cooperatively with Asp181, and that Tyr370 stabilizes Ald binding by hydrogen-bonding/hydrophobic interactions at the C-terminal region of Ald. PubMed: 19476493DOI: 10.1111/j.1742-4658.2009.06978.x PDB entries with the same primary citation |
| Experimental method | X-RAY DIFFRACTION (1.51 Å) |
Structure validation
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