Probing the specificity of cysteine proteinases at subsites remote from the active site: analysis of P-4, P-3, P-2 ' and P-3 ' variations in extended substrates

Portaro, Fernanda Calheta Vieira [UNIFESP]; Santos, Ana Beatriz F; Cezari, Maria Helena S; Juliano, Maria Aparecida [UNIFESP]; Juliano, Luiz [UNIFESP]; Carmona, Euridice

Probing the specificity of cysteine proteinases at subsites remote from the active site: analysis of P-4, P-3, P-2 ' and P-3 ' variations in extended substrates

Detalhes bibliográficos
Autor(a) principal:	Portaro, Fernanda Calheta Vieira [UNIFESP]
Data de Publicação:	2000
Outros Autores:	Santos, Ana Beatriz F, Cezari, Maria Helena S, Juliano, Maria Aparecida [UNIFESP], Juliano, Luiz [UNIFESP], Carmona, Euridice
Tipo de documento:	Artigo
Idioma:	eng
Título da fonte:	Repositório Institucional da UNIFESP
Texto Completo:	http://dx.doi.org/10.1042/0264-6021:3470123 http://repositorio.unifesp.br/handle/11600/26274
Resumo:	We have determined the kinetic parameters for the hydrolysis by papain, cathepsin B and cathepsin L of internally quenched fluorescent peptides derived from the lead peptides Abz-AAFRSAQ-EDDnp [in which Abz and EDDnp stand for o-aminobenzoic acid and N-(2,4-dinitrophenyl)ethylenediamine respectively], to map the specificity of S-4 and S-3 subsites, and Abz-AFRSAAQ-EDDnp, to identify the specificity of S-2' and S-3'. Abz and EDDnp were the fluorescent quencher pair. These two series of peptides were cleaved at the Arg-Ser bond and systematic modifications at P-4, P-3, P-2' and P-3' were made. the S-4 to S-2' subsites had a significant influence on the hydrolytic efficiencies of the three enzymes. Only papain activity was observed to be dependent on S-3', indicating that its binding site is larger than those of cathepsins B and L. Hydrophobic amino acids were accepted at S-4, S-3, S-3' and S-3' of the three enzymes. the best substrates for cathepsins L and B had Trp and Asn at P-2' respectively; variations at this position were less accepted by these enzymes. the best substrates for papain were peptides containing Trp, Tyr or Asn at P-3'. Basic residues at P-3 and p(4) were well accepted by cathepsin L and papain. We also explored the susceptibility of substrates Abz-AFRSXAQ-EDDnp, modified at P-2' (X), to human cathepsin B mutants from which one or two occluding loop contacts had been removed. the modifications at His(111) (H111A) and His(110) (H110A) of cathepsin B led to an increase in k(cat) values of one or two orders of magnitude. the hydrolytic efficiencies of these cathepsin B mutants became closer to those of papain or cathepsin L.

Metadados do item

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network_acronym_str	UFSP
network_name_str	Repositório Institucional da UNIFESP
repository_id_str	3465
spelling	Probing the specificity of cysteine proteinases at subsites remote from the active site: analysis of P-4, P-3, P-2 ' and P-3 ' variations in extended substratescathepsins B and Lfluorogenic peptidelimited proteolysispapainprotease substrateWe have determined the kinetic parameters for the hydrolysis by papain, cathepsin B and cathepsin L of internally quenched fluorescent peptides derived from the lead peptides Abz-AAFRSAQ-EDDnp [in which Abz and EDDnp stand for o-aminobenzoic acid and N-(2,4-dinitrophenyl)ethylenediamine respectively], to map the specificity of S-4 and S-3 subsites, and Abz-AFRSAAQ-EDDnp, to identify the specificity of S-2' and S-3'. Abz and EDDnp were the fluorescent quencher pair. These two series of peptides were cleaved at the Arg-Ser bond and systematic modifications at P-4, P-3, P-2' and P-3' were made. the S-4 to S-2' subsites had a significant influence on the hydrolytic efficiencies of the three enzymes. Only papain activity was observed to be dependent on S-3', indicating that its binding site is larger than those of cathepsins B and L. Hydrophobic amino acids were accepted at S-4, S-3, S-3' and S-3' of the three enzymes. the best substrates for cathepsins L and B had Trp and Asn at P-2' respectively; variations at this position were less accepted by these enzymes. the best substrates for papain were peptides containing Trp, Tyr or Asn at P-3'. Basic residues at P-3 and p(4) were well accepted by cathepsin L and papain. We also explored the susceptibility of substrates Abz-AFRSXAQ-EDDnp, modified at P-2' (X), to human cathepsin B mutants from which one or two occluding loop contacts had been removed. the modifications at His(111) (H111A) and His(110) (H110A) of cathepsin B led to an increase in k(cat) values of one or two orders of magnitude. the hydrolytic efficiencies of these cathepsin B mutants became closer to those of papain or cathepsin L.Inst Butantan, Dept Pharmacol, BR-05503900 São Paulo, BrazilEscola Paulista Med, Dept Biofis, BR-04044020 São Paulo, BrazilEscola Paulista Med, Dept Biofis, BR-04044020 São Paulo, BrazilWeb of SciencePortland PressInst ButantanUniversidade Federal de São Paulo (UNIFESP)Portaro, Fernanda Calheta Vieira [UNIFESP]Santos, Ana Beatriz FCezari, Maria Helena SJuliano, Maria Aparecida [UNIFESP]Juliano, Luiz [UNIFESP]Carmona, Euridice2016-01-24T12:31:02Z2016-01-24T12:31:02Z2000-04-01info:eu-repo/semantics/articleinfo:eu-repo/semantics/publishedVersion123-129http://dx.doi.org/10.1042/0264-6021:3470123Biochemical Journal. London: Portland Press, v. 347, p. 123-129, 2000.10.1042/0264-6021:34701230264-6021http://repositorio.unifesp.br/handle/11600/26274WOS:000086792600016engBiochemical Journalinfo:eu-repo/semantics/openAccessreponame:Repositório Institucional da UNIFESPinstname:Universidade Federal de São Paulo (UNIFESP)instacron:UNIFESP2016-01-24T10:31:02Zoai:repositorio.unifesp.br/:11600/26274Repositório InstitucionalPUBhttp://www.repositorio.unifesp.br/oai/requestbiblioteca.csp@unifesp.bropendoar:34652016-01-24T10:31:02Repositório Institucional da UNIFESP - Universidade Federal de São Paulo (UNIFESP)false
dc.title.none.fl_str_mv	Probing the specificity of cysteine proteinases at subsites remote from the active site: analysis of P-4, P-3, P-2 ' and P-3 ' variations in extended substrates
title	Probing the specificity of cysteine proteinases at subsites remote from the active site: analysis of P-4, P-3, P-2 ' and P-3 ' variations in extended substrates
spellingShingle	Probing the specificity of cysteine proteinases at subsites remote from the active site: analysis of P-4, P-3, P-2 ' and P-3 ' variations in extended substrates Portaro, Fernanda Calheta Vieira [UNIFESP] cathepsins B and L fluorogenic peptide limited proteolysis papain protease substrate
title_short	Probing the specificity of cysteine proteinases at subsites remote from the active site: analysis of P-4, P-3, P-2 ' and P-3 ' variations in extended substrates
title_full	Probing the specificity of cysteine proteinases at subsites remote from the active site: analysis of P-4, P-3, P-2 ' and P-3 ' variations in extended substrates
title_fullStr	Probing the specificity of cysteine proteinases at subsites remote from the active site: analysis of P-4, P-3, P-2 ' and P-3 ' variations in extended substrates
title_full_unstemmed	Probing the specificity of cysteine proteinases at subsites remote from the active site: analysis of P-4, P-3, P-2 ' and P-3 ' variations in extended substrates
title_sort	Probing the specificity of cysteine proteinases at subsites remote from the active site: analysis of P-4, P-3, P-2 ' and P-3 ' variations in extended substrates
author	Portaro, Fernanda Calheta Vieira [UNIFESP]
author_facet	Portaro, Fernanda Calheta Vieira [UNIFESP] Santos, Ana Beatriz F Cezari, Maria Helena S Juliano, Maria Aparecida [UNIFESP] Juliano, Luiz [UNIFESP] Carmona, Euridice
author_role	author
author2	Santos, Ana Beatriz F Cezari, Maria Helena S Juliano, Maria Aparecida [UNIFESP] Juliano, Luiz [UNIFESP] Carmona, Euridice
author2_role	author author author author author
dc.contributor.none.fl_str_mv	Inst Butantan Universidade Federal de São Paulo (UNIFESP)
dc.contributor.author.fl_str_mv	Portaro, Fernanda Calheta Vieira [UNIFESP] Santos, Ana Beatriz F Cezari, Maria Helena S Juliano, Maria Aparecida [UNIFESP] Juliano, Luiz [UNIFESP] Carmona, Euridice
dc.subject.por.fl_str_mv	cathepsins B and L fluorogenic peptide limited proteolysis papain protease substrate
topic	cathepsins B and L fluorogenic peptide limited proteolysis papain protease substrate
description	We have determined the kinetic parameters for the hydrolysis by papain, cathepsin B and cathepsin L of internally quenched fluorescent peptides derived from the lead peptides Abz-AAFRSAQ-EDDnp [in which Abz and EDDnp stand for o-aminobenzoic acid and N-(2,4-dinitrophenyl)ethylenediamine respectively], to map the specificity of S-4 and S-3 subsites, and Abz-AFRSAAQ-EDDnp, to identify the specificity of S-2' and S-3'. Abz and EDDnp were the fluorescent quencher pair. These two series of peptides were cleaved at the Arg-Ser bond and systematic modifications at P-4, P-3, P-2' and P-3' were made. the S-4 to S-2' subsites had a significant influence on the hydrolytic efficiencies of the three enzymes. Only papain activity was observed to be dependent on S-3', indicating that its binding site is larger than those of cathepsins B and L. Hydrophobic amino acids were accepted at S-4, S-3, S-3' and S-3' of the three enzymes. the best substrates for cathepsins L and B had Trp and Asn at P-2' respectively; variations at this position were less accepted by these enzymes. the best substrates for papain were peptides containing Trp, Tyr or Asn at P-3'. Basic residues at P-3 and p(4) were well accepted by cathepsin L and papain. We also explored the susceptibility of substrates Abz-AFRSXAQ-EDDnp, modified at P-2' (X), to human cathepsin B mutants from which one or two occluding loop contacts had been removed. the modifications at His(111) (H111A) and His(110) (H110A) of cathepsin B led to an increase in k(cat) values of one or two orders of magnitude. the hydrolytic efficiencies of these cathepsin B mutants became closer to those of papain or cathepsin L.
publishDate	2000
dc.date.none.fl_str_mv	2000-04-01 2016-01-24T12:31:02Z 2016-01-24T12:31:02Z
dc.type.driver.fl_str_mv	info:eu-repo/semantics/article
dc.type.status.fl_str_mv	info:eu-repo/semantics/publishedVersion
format	article
status_str	publishedVersion
dc.identifier.uri.fl_str_mv	http://dx.doi.org/10.1042/0264-6021:3470123 Biochemical Journal. London: Portland Press, v. 347, p. 123-129, 2000. 10.1042/0264-6021:3470123 0264-6021 http://repositorio.unifesp.br/handle/11600/26274 WOS:000086792600016
url	http://dx.doi.org/10.1042/0264-6021:3470123 http://repositorio.unifesp.br/handle/11600/26274
identifier_str_mv	Biochemical Journal. London: Portland Press, v. 347, p. 123-129, 2000. 10.1042/0264-6021:3470123 0264-6021 WOS:000086792600016
dc.language.iso.fl_str_mv	eng
language	eng
dc.relation.none.fl_str_mv	Biochemical Journal
dc.rights.driver.fl_str_mv	info:eu-repo/semantics/openAccess
eu_rights_str_mv	openAccess
dc.format.none.fl_str_mv	123-129
dc.publisher.none.fl_str_mv	Portland Press
publisher.none.fl_str_mv	Portland Press
dc.source.none.fl_str_mv	reponame:Repositório Institucional da UNIFESP instname:Universidade Federal de São Paulo (UNIFESP) instacron:UNIFESP
instname_str	Universidade Federal de São Paulo (UNIFESP)
instacron_str	UNIFESP
institution	UNIFESP
reponame_str	Repositório Institucional da UNIFESP
collection	Repositório Institucional da UNIFESP
repository.name.fl_str_mv	Repositório Institucional da UNIFESP - Universidade Federal de São Paulo (UNIFESP)
repository.mail.fl_str_mv	biblioteca.csp@unifesp.br
_version_	1814268400455647232

Probing the specificity of cysteine proteinases at subsites remote from the active site: analysis of P-4, P-3, P-2 ' and P-3 ' variations in extended substrates

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