Molecular Mechanisms of Improvement of Hydrolytic Antibody 6D9 by Site-Directed Mutagenesis

doi:10.1093/jb/mvj179

Journal of Biochemistry Advance Access originally published online on August 18, 2006
Journal of Biochemistry 2006 140(4):509-515; doi:10.1093/jb/mvj179

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Molecular Mechanisms of Improvement of Hydrolytic Antibody 6D9 by Site-Directed Mutagenesis

Naoko Takahashi-Ando¹^,*^,, Kazuko Shimazaki¹^,*, Hiroyuki Kakinuma¹^,*, Ikuo Fujii²^,* and Yoshisuke Nishi¹^,*^,

¹ Laboratory of Life Science & Biomolecular Engineering, Japan Tobacco, Inc. 6-2, Umegaoka, Aoba-ku, Yokohama, Kanagawa 227-8512; and ² Department of Biological Science, Graduate School of Science, Osaka Prefecture University, 1-2, Gakuen-cho, Sakai, Osaka 599-8570

^* Present addresses: Naoko Takahashi-Ando, Plant & Microbial Metabolic Engineering Research Unit, RIKEN, 2-1, Hirosawa, Wako, Saitama 351-0198; Kazuko Shimazaki, Nippon Veterinary and Life Science University, Department of Veterinary, Laboratory of Structural Bioinformatics, 1-7-1, Kyonan-cho, Musashino, Tokyo 180-8602; Hiroyuki Kakinuma, Medicinal Chemistry Laboratory, Taisho Pharmaceutical CO., LTD., 1-403, Yoshino-cho, Saitama, Saitama 330-8530; Yoshisuke Nishi, Faculty of Bioscience, Nagahama Institute of Bio-Science and Technology, 1266 Tamura-cho, Nagahama, Shiga 526-0829.

We performed a series of site-directed mutagenesis experimentsof catalytic antibody, 6D9, which hydrolyzes a prodrug of chloramphenicol,based on our previous directed evolution study [Takahashi etal. (2001) Nat. Biotechnol. 19, 563–567]. Since we previouslyfound that the variants with a mutation of Ser(L27e)Tyr affordeda one order of magnitude increase in catalytic rate, we createda site-directed mutant containing this mutation. The resultingmutant, 6D9-Ser(L27e)Tyr, had 6.5-fold higher k_cat/k_uncat and9.8-fold higher k_cat/K_m than wild-type 6D9. We also created6D9-Thr(L27a)Pro, since this mutation occurred frequently inthe previous directed evolution, and it had 2.1-fold higherk_cat/k_uncat and k_cat/K_m than 6D9. Kinetic and computationalanalyses suggest that Tyr at L27e contributes to transition-statestabilization, while Pro at L27a does not interact with thetransition-state structure directly, but obviously contributesto enhanced catalytic activity. Including double mutants thatcombined favourable substitutions, we created seven site-directedmutants. However, none of them had higher catalytic activitiesthan some of highly improved variants obtained in the previousdirected evolution. The present study gives direct evidencethat not only a specific amino acid residue which obviouslycontributes to transition-state stabilization, but also a groupof amino acid residues working in concert is important for efficientcatalysis of a given transformation.

To whom correspondence should be addressed. Naoko Takahashi-Ando,Tel: +81-48-467-9796, E-mail: ntando{at}postman.riken.jp; YoshisukeNishi, Tel: +81-749-64-8122 (direct line)/+81-749-64-8100 (mainline), Fax: +81-749-64-8140, E-mail: y_nishi{at}nagahama-i-bio.ac.jp

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Journal of Biochemistry

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Molecular Mechanisms of Improvement of Hydrolytic Antibody 6D9 by Site-Directed Mutagenesis