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Structure-Based Engineering of an Artificially Generated NADP + -Dependent d-Amino Acid Dehydrogenase
A stable NADP -dependent d-amino acid dehydrogenase (DAADH) was recently created from -diaminopimelate dehydrogenase through site-directed mutagenesis. To produce a novel DAADH mutant with different substrate specificity, the crystal structure of apo-DAADH was determined at a resolution of 1.78 Å, a...
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| Published in: | Applied and environmental microbiology 2017-06, Vol.83 (11) |
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| creator | Hayashi, Junji Seto, Tomonari Akita, Hironaga Watanabe, Masahiro Hoshino, Tamotsu Yoneda, Kazunari Ohshima, Toshihisa Sakuraba, Haruhiko |
| description | A stable NADP
-dependent d-amino acid dehydrogenase (DAADH) was recently created from
-diaminopimelate dehydrogenase through site-directed mutagenesis. To produce a novel DAADH mutant with different substrate specificity, the crystal structure of apo-DAADH was determined at a resolution of 1.78 Å, and the amino acid residues responsible for the substrate specificity were evaluated using additional site-directed mutagenesis. By introducing a single D94A mutation, the enzyme's substrate specificity was dramatically altered; the mutant utilized d-phenylalanine as the most preferable substrate for oxidative deamination and had a specific activity of 5.33 μmol/min/mg at 50°C, which was 54-fold higher than that of the parent DAADH. In addition, the specific activities of the mutant toward d-leucine, d-norleucine, d-methionine, d-isoleucine, and d-tryptophan were much higher (6 to 25 times) than those of the parent enzyme. For reductive amination, the D94A mutant exhibited extremely high specific activity with phenylpyruvate (16.1 μmol/min/mg at 50°C). The structures of the D94A-Y224F double mutant in complex with NADP
and in complex with both NADPH and 2-keto-6-aminocapronic acid (lysine oxo-analogue) were then determined at resolutions of 1.59 Å and 1.74 Å, respectively. The phenylpyruvate-binding model suggests that the D94A mutation prevents the substrate phenyl group from sterically clashing with the side chain of Asp94. A structural comparison suggests that both the enlarged substrate-binding pocket and enhanced hydrophobicity of the pocket are mainly responsible for the high reactivity of the D94A mutant toward the hydrophobic d-amino acids with bulky side chains.
In recent years, the potential uses for d-amino acids as source materials for the industrial production of medicines, seasonings, and agrochemicals have been growing. To date, several methods have been used for the production of d-amino acids, but all include tedious steps. The use of NAD(P)
-dependent d-amino acid dehydrogenase (DAADH) makes single-step production of d-amino acids from oxo-acid analogs and ammonia possible. We recently succeeded in creating a stable DAADH and demonstrated that it is applicable for one-step synthesis of d-amino acids, such as d-leucine and d-isoleucine. As the next step, the creation of an enzyme exhibiting different substrate specificity and higher catalytic efficiency is a key to the further development of d-amino acid production. In this study, we succeeded in |
| doi_str_mv | 10.1128/AEM.00491-17 |
| format | article |
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-dependent d-amino acid dehydrogenase (DAADH) was recently created from
-diaminopimelate dehydrogenase through site-directed mutagenesis. To produce a novel DAADH mutant with different substrate specificity, the crystal structure of apo-DAADH was determined at a resolution of 1.78 Å, and the amino acid residues responsible for the substrate specificity were evaluated using additional site-directed mutagenesis. By introducing a single D94A mutation, the enzyme's substrate specificity was dramatically altered; the mutant utilized d-phenylalanine as the most preferable substrate for oxidative deamination and had a specific activity of 5.33 μmol/min/mg at 50°C, which was 54-fold higher than that of the parent DAADH. In addition, the specific activities of the mutant toward d-leucine, d-norleucine, d-methionine, d-isoleucine, and d-tryptophan were much higher (6 to 25 times) than those of the parent enzyme. For reductive amination, the D94A mutant exhibited extremely high specific activity with phenylpyruvate (16.1 μmol/min/mg at 50°C). The structures of the D94A-Y224F double mutant in complex with NADP
and in complex with both NADPH and 2-keto-6-aminocapronic acid (lysine oxo-analogue) were then determined at resolutions of 1.59 Å and 1.74 Å, respectively. The phenylpyruvate-binding model suggests that the D94A mutation prevents the substrate phenyl group from sterically clashing with the side chain of Asp94. A structural comparison suggests that both the enlarged substrate-binding pocket and enhanced hydrophobicity of the pocket are mainly responsible for the high reactivity of the D94A mutant toward the hydrophobic d-amino acids with bulky side chains.
In recent years, the potential uses for d-amino acids as source materials for the industrial production of medicines, seasonings, and agrochemicals have been growing. To date, several methods have been used for the production of d-amino acids, but all include tedious steps. The use of NAD(P)
-dependent d-amino acid dehydrogenase (DAADH) makes single-step production of d-amino acids from oxo-acid analogs and ammonia possible. We recently succeeded in creating a stable DAADH and demonstrated that it is applicable for one-step synthesis of d-amino acids, such as d-leucine and d-isoleucine. As the next step, the creation of an enzyme exhibiting different substrate specificity and higher catalytic efficiency is a key to the further development of d-amino acid production. In this study, we succeeded in creating a novel mutant exhibiting extremely high catalytic activity for phenylpyruvate amination. Structural insight into the mutant will be useful for further improvement of DAADHs.</description><identifier>ISSN: 0099-2240</identifier><identifier>EISSN: 1098-5336</identifier><identifier>DOI: 10.1128/AEM.00491-17</identifier><identifier>PMID: 28363957</identifier><language>eng</language><publisher>United States: American Society for Microbiology</publisher><subject>Amino Acid Motifs ; Amino Acid Oxidoreductases - chemistry ; Amino Acid Oxidoreductases - genetics ; Amino Acid Oxidoreductases - metabolism ; Amino Acid Sequence ; Bacterial Proteins - chemistry ; Bacterial Proteins - genetics ; Bacterial Proteins - metabolism ; Binding Sites ; Enzymology and Protein Engineering ; Kinetics ; Models, Molecular ; Mutagenesis, Site-Directed ; NADP - metabolism ; Planococcaceae - chemistry ; Planococcaceae - enzymology ; Planococcaceae - genetics ; Protein Engineering ; Substrate Specificity</subject><ispartof>Applied and environmental microbiology, 2017-06, Vol.83 (11)</ispartof><rights>Copyright © 2017 American Society for Microbiology.</rights><rights>Copyright © 2017 American Society for Microbiology. 2017 American Society for Microbiology</rights><lds50>peer_reviewed</lds50><oa>free_for_read</oa><woscitedreferencessubscribed>false</woscitedreferencessubscribed><citedby>FETCH-LOGICAL-c417t-4da67756f39d2ae3b27f890167a853b2d20b06ec37a1640f0d8dc8c6f86867913</citedby><cites>FETCH-LOGICAL-c417t-4da67756f39d2ae3b27f890167a853b2d20b06ec37a1640f0d8dc8c6f86867913</cites></display><links><openurl>$$Topenurl_article</openurl><openurlfulltext>$$Topenurlfull_article</openurlfulltext><thumbnail>$$Tsyndetics_thumb_exl</thumbnail><linktopdf>$$Uhttps://www.ncbi.nlm.nih.gov/pmc/articles/PMC5440713/pdf/$$EPDF$$P50$$Gpubmedcentral$$H</linktopdf><linktohtml>$$Uhttps://www.ncbi.nlm.nih.gov/pmc/articles/PMC5440713/$$EHTML$$P50$$Gpubmedcentral$$H</linktohtml><link.rule.ids>230,314,723,776,780,881,3174,27903,27904,53769,53771</link.rule.ids><backlink>$$Uhttps://www.ncbi.nlm.nih.gov/pubmed/28363957$$D View this record in MEDLINE/PubMed$$Hfree_for_read</backlink></links><search><contributor>Atomi, Haruyuki</contributor><creatorcontrib>Hayashi, Junji</creatorcontrib><creatorcontrib>Seto, Tomonari</creatorcontrib><creatorcontrib>Akita, Hironaga</creatorcontrib><creatorcontrib>Watanabe, Masahiro</creatorcontrib><creatorcontrib>Hoshino, Tamotsu</creatorcontrib><creatorcontrib>Yoneda, Kazunari</creatorcontrib><creatorcontrib>Ohshima, Toshihisa</creatorcontrib><creatorcontrib>Sakuraba, Haruhiko</creatorcontrib><title>Structure-Based Engineering of an Artificially Generated NADP + -Dependent d-Amino Acid Dehydrogenase</title><title>Applied and environmental microbiology</title><addtitle>Appl Environ Microbiol</addtitle><description>A stable NADP
-dependent d-amino acid dehydrogenase (DAADH) was recently created from
-diaminopimelate dehydrogenase through site-directed mutagenesis. To produce a novel DAADH mutant with different substrate specificity, the crystal structure of apo-DAADH was determined at a resolution of 1.78 Å, and the amino acid residues responsible for the substrate specificity were evaluated using additional site-directed mutagenesis. By introducing a single D94A mutation, the enzyme's substrate specificity was dramatically altered; the mutant utilized d-phenylalanine as the most preferable substrate for oxidative deamination and had a specific activity of 5.33 μmol/min/mg at 50°C, which was 54-fold higher than that of the parent DAADH. In addition, the specific activities of the mutant toward d-leucine, d-norleucine, d-methionine, d-isoleucine, and d-tryptophan were much higher (6 to 25 times) than those of the parent enzyme. For reductive amination, the D94A mutant exhibited extremely high specific activity with phenylpyruvate (16.1 μmol/min/mg at 50°C). The structures of the D94A-Y224F double mutant in complex with NADP
and in complex with both NADPH and 2-keto-6-aminocapronic acid (lysine oxo-analogue) were then determined at resolutions of 1.59 Å and 1.74 Å, respectively. The phenylpyruvate-binding model suggests that the D94A mutation prevents the substrate phenyl group from sterically clashing with the side chain of Asp94. A structural comparison suggests that both the enlarged substrate-binding pocket and enhanced hydrophobicity of the pocket are mainly responsible for the high reactivity of the D94A mutant toward the hydrophobic d-amino acids with bulky side chains.
In recent years, the potential uses for d-amino acids as source materials for the industrial production of medicines, seasonings, and agrochemicals have been growing. To date, several methods have been used for the production of d-amino acids, but all include tedious steps. The use of NAD(P)
-dependent d-amino acid dehydrogenase (DAADH) makes single-step production of d-amino acids from oxo-acid analogs and ammonia possible. We recently succeeded in creating a stable DAADH and demonstrated that it is applicable for one-step synthesis of d-amino acids, such as d-leucine and d-isoleucine. As the next step, the creation of an enzyme exhibiting different substrate specificity and higher catalytic efficiency is a key to the further development of d-amino acid production. In this study, we succeeded in creating a novel mutant exhibiting extremely high catalytic activity for phenylpyruvate amination. Structural insight into the mutant will be useful for further improvement of DAADHs.</description><subject>Amino Acid Motifs</subject><subject>Amino Acid Oxidoreductases - chemistry</subject><subject>Amino Acid Oxidoreductases - genetics</subject><subject>Amino Acid Oxidoreductases - metabolism</subject><subject>Amino Acid Sequence</subject><subject>Bacterial Proteins - chemistry</subject><subject>Bacterial Proteins - genetics</subject><subject>Bacterial Proteins - metabolism</subject><subject>Binding Sites</subject><subject>Enzymology and Protein Engineering</subject><subject>Kinetics</subject><subject>Models, Molecular</subject><subject>Mutagenesis, Site-Directed</subject><subject>NADP - metabolism</subject><subject>Planococcaceae - chemistry</subject><subject>Planococcaceae - enzymology</subject><subject>Planococcaceae - genetics</subject><subject>Protein Engineering</subject><subject>Substrate Specificity</subject><issn>0099-2240</issn><issn>1098-5336</issn><fulltext>true</fulltext><rsrctype>article</rsrctype><creationdate>2017</creationdate><recordtype>article</recordtype><recordid>eNpVkV1LHDEUhoO06Gq963XJZaHGJpOZfNwIU3e1BbWCeh2yyZk1MpvZJjOF_ffGT9qrw-E8vOeFB6HPjB4zVqnv7eLymNJaM8LkDpoxqhVpOBcf0IxSrUlV1XQP7ef8QAtGhdpFe5XigutGzhDcjGly45SA_LAZPF7EVYgAKcQVHjpsI27TGLrggu37LT6HCMmOBbxq59f4GyZz2ED0EEfsSbsOccCtCx7P4X7r07CCWGI_oY-d7TMcvs4DdHe2uD39SS5-n_86bS-Iq5kcSe2tkLIRHde-ssCXleyUpkxIq5qy-YouqQDHpWWiph31yjvlRKeEElIzfoBOXnI303IN3pVWyfZmk8Lapq0ZbDD_X2K4N6vhr2nqmkrGS8DX14A0_Jkgj2YdsoO-txGGKRumGRNV09S6oEcvqEtDzgm69zeMmiczppgxz2YMkwX_8m-1d_hNBX8E0ZeI8Q</recordid><startdate>20170601</startdate><enddate>20170601</enddate><creator>Hayashi, Junji</creator><creator>Seto, Tomonari</creator><creator>Akita, Hironaga</creator><creator>Watanabe, Masahiro</creator><creator>Hoshino, Tamotsu</creator><creator>Yoneda, Kazunari</creator><creator>Ohshima, Toshihisa</creator><creator>Sakuraba, Haruhiko</creator><general>American Society for Microbiology</general><scope>CGR</scope><scope>CUY</scope><scope>CVF</scope><scope>ECM</scope><scope>EIF</scope><scope>NPM</scope><scope>AAYXX</scope><scope>CITATION</scope><scope>7T7</scope><scope>8FD</scope><scope>C1K</scope><scope>FR3</scope><scope>P64</scope><scope>5PM</scope></search><sort><creationdate>20170601</creationdate><title>Structure-Based Engineering of an Artificially Generated NADP + -Dependent d-Amino Acid Dehydrogenase</title><author>Hayashi, Junji ; Seto, Tomonari ; Akita, Hironaga ; Watanabe, Masahiro ; Hoshino, Tamotsu ; Yoneda, Kazunari ; Ohshima, Toshihisa ; Sakuraba, Haruhiko</author></sort><facets><frbrtype>5</frbrtype><frbrgroupid>cdi_FETCH-LOGICAL-c417t-4da67756f39d2ae3b27f890167a853b2d20b06ec37a1640f0d8dc8c6f86867913</frbrgroupid><rsrctype>articles</rsrctype><prefilter>articles</prefilter><language>eng</language><creationdate>2017</creationdate><topic>Amino Acid Motifs</topic><topic>Amino Acid Oxidoreductases - chemistry</topic><topic>Amino Acid Oxidoreductases - genetics</topic><topic>Amino Acid Oxidoreductases - metabolism</topic><topic>Amino Acid Sequence</topic><topic>Bacterial Proteins - chemistry</topic><topic>Bacterial Proteins - genetics</topic><topic>Bacterial Proteins - metabolism</topic><topic>Binding Sites</topic><topic>Enzymology and Protein Engineering</topic><topic>Kinetics</topic><topic>Models, Molecular</topic><topic>Mutagenesis, Site-Directed</topic><topic>NADP - metabolism</topic><topic>Planococcaceae - chemistry</topic><topic>Planococcaceae - enzymology</topic><topic>Planococcaceae - genetics</topic><topic>Protein Engineering</topic><topic>Substrate Specificity</topic><toplevel>peer_reviewed</toplevel><toplevel>online_resources</toplevel><creatorcontrib>Hayashi, Junji</creatorcontrib><creatorcontrib>Seto, Tomonari</creatorcontrib><creatorcontrib>Akita, Hironaga</creatorcontrib><creatorcontrib>Watanabe, Masahiro</creatorcontrib><creatorcontrib>Hoshino, Tamotsu</creatorcontrib><creatorcontrib>Yoneda, Kazunari</creatorcontrib><creatorcontrib>Ohshima, Toshihisa</creatorcontrib><creatorcontrib>Sakuraba, Haruhiko</creatorcontrib><collection>Medline</collection><collection>MEDLINE</collection><collection>MEDLINE (Ovid)</collection><collection>MEDLINE</collection><collection>MEDLINE</collection><collection>PubMed</collection><collection>CrossRef</collection><collection>Industrial and Applied Microbiology Abstracts (Microbiology A)</collection><collection>Technology Research Database</collection><collection>Environmental Sciences and Pollution Management</collection><collection>Engineering Research Database</collection><collection>Biotechnology and BioEngineering Abstracts</collection><collection>PubMed Central (Full Participant titles)</collection><jtitle>Applied and environmental microbiology</jtitle></facets><delivery><delcategory>Remote Search Resource</delcategory><fulltext>fulltext</fulltext></delivery><addata><au>Hayashi, Junji</au><au>Seto, Tomonari</au><au>Akita, Hironaga</au><au>Watanabe, Masahiro</au><au>Hoshino, Tamotsu</au><au>Yoneda, Kazunari</au><au>Ohshima, Toshihisa</au><au>Sakuraba, Haruhiko</au><au>Atomi, Haruyuki</au><format>journal</format><genre>article</genre><ristype>JOUR</ristype><atitle>Structure-Based Engineering of an Artificially Generated NADP + -Dependent d-Amino Acid Dehydrogenase</atitle><jtitle>Applied and environmental microbiology</jtitle><addtitle>Appl Environ Microbiol</addtitle><date>2017-06-01</date><risdate>2017</risdate><volume>83</volume><issue>11</issue><issn>0099-2240</issn><eissn>1098-5336</eissn><abstract>A stable NADP
-dependent d-amino acid dehydrogenase (DAADH) was recently created from
-diaminopimelate dehydrogenase through site-directed mutagenesis. To produce a novel DAADH mutant with different substrate specificity, the crystal structure of apo-DAADH was determined at a resolution of 1.78 Å, and the amino acid residues responsible for the substrate specificity were evaluated using additional site-directed mutagenesis. By introducing a single D94A mutation, the enzyme's substrate specificity was dramatically altered; the mutant utilized d-phenylalanine as the most preferable substrate for oxidative deamination and had a specific activity of 5.33 μmol/min/mg at 50°C, which was 54-fold higher than that of the parent DAADH. In addition, the specific activities of the mutant toward d-leucine, d-norleucine, d-methionine, d-isoleucine, and d-tryptophan were much higher (6 to 25 times) than those of the parent enzyme. For reductive amination, the D94A mutant exhibited extremely high specific activity with phenylpyruvate (16.1 μmol/min/mg at 50°C). The structures of the D94A-Y224F double mutant in complex with NADP
and in complex with both NADPH and 2-keto-6-aminocapronic acid (lysine oxo-analogue) were then determined at resolutions of 1.59 Å and 1.74 Å, respectively. The phenylpyruvate-binding model suggests that the D94A mutation prevents the substrate phenyl group from sterically clashing with the side chain of Asp94. A structural comparison suggests that both the enlarged substrate-binding pocket and enhanced hydrophobicity of the pocket are mainly responsible for the high reactivity of the D94A mutant toward the hydrophobic d-amino acids with bulky side chains.
In recent years, the potential uses for d-amino acids as source materials for the industrial production of medicines, seasonings, and agrochemicals have been growing. To date, several methods have been used for the production of d-amino acids, but all include tedious steps. The use of NAD(P)
-dependent d-amino acid dehydrogenase (DAADH) makes single-step production of d-amino acids from oxo-acid analogs and ammonia possible. We recently succeeded in creating a stable DAADH and demonstrated that it is applicable for one-step synthesis of d-amino acids, such as d-leucine and d-isoleucine. As the next step, the creation of an enzyme exhibiting different substrate specificity and higher catalytic efficiency is a key to the further development of d-amino acid production. In this study, we succeeded in creating a novel mutant exhibiting extremely high catalytic activity for phenylpyruvate amination. Structural insight into the mutant will be useful for further improvement of DAADHs.</abstract><cop>United States</cop><pub>American Society for Microbiology</pub><pmid>28363957</pmid><doi>10.1128/AEM.00491-17</doi><oa>free_for_read</oa></addata></record> |
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| ispartof | Applied and environmental microbiology, 2017-06, Vol.83 (11) |
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| source | American Society for Microbiology (ASM) Journals; PubMed Central |
| subjects | Amino Acid Motifs Amino Acid Oxidoreductases - chemistry Amino Acid Oxidoreductases - genetics Amino Acid Oxidoreductases - metabolism Amino Acid Sequence Bacterial Proteins - chemistry Bacterial Proteins - genetics Bacterial Proteins - metabolism Binding Sites Enzymology and Protein Engineering Kinetics Models, Molecular Mutagenesis, Site-Directed NADP - metabolism Planococcaceae - chemistry Planococcaceae - enzymology Planococcaceae - genetics Protein Engineering Substrate Specificity |
| title | Structure-Based Engineering of an Artificially Generated NADP + -Dependent d-Amino Acid Dehydrogenase |
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