The crystal structure of an EST2 mutant unveils structural insights on the H group of the carboxylesterase/lipase family. (Articolo in rivista)

Type

• Prodotto della ricerca (Classe)
• Articolo in rivista (Classe)

Label

• The crystal structure of an EST2 mutant unveils structural insights on the H group of the carboxylesterase/lipase family. (Articolo in rivista) (literal)

Anno

• 2004-01-01T00:00:00+01:00 (literal)

Http://www.cnr.it/ontology/cnr/pubblicazioni.owl#doi

• 10.1016/j.jmb.2004.08.014 (literal)

Alternative label

• De Simone G; Menchise V; Alterio V; Mandrich L; Rossi M; Manco G; Pedone C. (2004)
  The crystal structure of an EST2 mutant unveils structural insights on the H group of the carboxylesterase/lipase family.
  in Journal of Molecular Biology
  (literal)

Http://www.cnr.it/ontology/cnr/pubblicazioni.owl#autori

• De Simone G; Menchise V; Alterio V; Mandrich L; Rossi M; Manco G; Pedone C. (literal)

Pagina inizio

• 137 (literal)

Pagina fine

• 146 (literal)

Http://www.cnr.it/ontology/cnr/pubblicazioni.owl#numeroVolume

• 343 (literal)

Rivista

• Journal of Molecular Biology (Rivista)

Note

• Scopu (literal)
• ISI Web of Science (WOS) (literal)

Http://www.cnr.it/ontology/cnr/pubblicazioni.owl#affiliazioni

• Dipartimento di Chimica Biologica-Sezione Biostrutture and Istituto di Biostrutture e Bioimmagini-CNR; University of Naples Federico II\", via Mezzocannone 16, 80134 Naples, Italy; Bioindustry Park del Canavese (Bi.P.Ca.), via Ribes 5, Colleretto Giocosa (TO) I-10010, Italy; Istituto di Biochimica delle Proteine-CNR, via P. Castellino 111, 80131 Naples, Italy. (literal)

Titolo

• The crystal structure of an EST2 mutant unveils structural insights on the H group of the carboxylesterase/lipase family. (literal)

Abstract

• Esterase 2 (EST2) from the thermophilic eubacterium Alicyclobacillus acidocaldarius is a thermostable serine hydrolase belonging to the H group of the esterase/lipase family. This enzyme hydrolyzes monoacylesters of different acyl-chain length and various compounds with industrial interest. EST2 displays an optimal temperature at 70 degrees C and maximal activity with pNP-esters having acyl-chain bearing from six to eight carbon atoms. EST2 mutants with different substrate specificity were also designed, generated by site-directed mutagenesis, and biochemically characterized. To better define at structural level the enzyme reaction mechanism, a crystallographic analysis of one of these mutants, namely M211S/R215L, was undertaken. Here we report its three-dimensional structure at 2.10A resolution. Structural analysis of the enzyme revealed an unexpected dimer formation as a consequence of a domain-swapping event involving its N-terminal region. This phenomenon was absent in the case of the enzyme bound to an irreversible inhibitor having optimal substrate structural features. A detailed comparison of the enzyme structures before and following binding to this molecule showed a movement of the N-terminal helices resulting from a trans-cis isomerization of the F37-P38 peptide bond. These findings suggest that this carboxylesterase presents two distinct structural arrangements reminiscent of the open and closed forms already reported for lipases. Potential biological implications associated with the observed quaternary reorganization are here discussed in light of the biochemical properties of other lipolytic members of the H group. (literal)
• Esterase 2 (EST2) from the thermophilic eubacterium Alicyclobacillus acidocaldarius is a thermostable serine hydrolase belonging to the H group of the esterase/lipase family. This enzyme hydrolyzes monoacylesters of different acyl-chain length and various compounds with industrial interest. EST2 displays an optimal temperature at 70 °C and maximal activity with pNP-esters having acyl-chain bearing from six to eight carbon atoms. EST2 mutants with different substrate specificity were also designed, generated by site-directed mutagenesis, and biochemically characterized. To better define at structural level the enzyme reaction mechanism, a crystallographic analysis of one of these mutants, namely M211S/R215L, was undertaken. Here we report its three-dimensional structure at 2.10 Å resolution. Structural analysis of the enzyme revealed an unexpected dimer formation as a consequence of a domain-swapping event involving its N-terminal region. This phenomenon was absent in the case of the enzyme bound to an irreversible inhibitor having optimal substrate structural features. A detailed comparison of the enzyme structures before and following binding to this molecule showed a movement of the N-terminal helices resulting from a trans–cis isomerization of the F37–P38 peptide bond. These findings suggest that this carboxylesterase presents two distinct structural arrangements reminiscent of the open and closed forms already reported for lipases. Potential biological implications associated with the observed quaternary reorganization are here discussed in light of the biochemical properties of other lipolytic members of the H group. (literal)

Prodotto di

• Institute of protein biochemistry (IBP) (Istituto)

Autore CNR

• GIUSEPPINA DE SIMONE (Unità di personale interno)
• GIUSEPPE MANCO (Unità di personale interno)
• VINCENZO ALTERIO (Persona)
• VALERIA MENCHISE (Persona)
• Mosè Rossi (Unità di personale esterno)
• LUIGI MANDRICH (Unità di personale esterno)

Incoming links:

Autore CNR di

• GIUSEPPE MANCO (Unità di personale interno)
• GIUSEPPINA DE SIMONE (Unità di personale interno)
• Mosè Rossi (Unità di personale esterno)
• VALERIA MENCHISE (Persona)
• LUIGI MANDRICH (Unità di personale esterno)
• VINCENZO ALTERIO (Persona)

Prodotto

• Institute of protein biochemistry (IBP) (Istituto)

Http://www.cnr.it/ontology/cnr/pubblicazioni.owl#rivistaDi

• Journal of Molecular Biology (Rivista)