Characterization, subsite mapping and N-terminal sequence of miliin, a serine-protease isolated from the latex of Euphorbia milii

被引：7

作者：

Moro, L. P. ^{[1
]}

Cabral, H. ^{[2
]}

Okamoto, D. N. ^{[3
]}

Hirata, I. ^{[3
]}

Juliano, M. A. ^{[3
]}

Juliano, L. ^{[3
]}

Bonilla-Rodriguez, G. O. ^{[1
]}

机构：

[1] State Univ Sao Paulo, IBILCE UNESP, Sao Jose Do Rio Preto, SP, Brazil

[2] Univ Sao Paulo, USP, BR-14049 Ribeirao Preto, SP, Brazil

[3] Univ Fed Sao Paulo, UNIFESP, Sao Paulo, Brazil

来源：

PROCESS BIOCHEMISTRY | 2013年 / 48卷 / 04期

基金：

巴西圣保罗研究基金会;

关键词：

Euphorbia milii; Miliin; Subsite mapping; Serine protease; Plant protease; FRET substrates; FUNCTIONAL-CHARACTERIZATION; BACTERIOLYTIC ENZYME; PURIFICATION; PROTEINASE; SPECIFICITY; EXPRESSION; SARCOCARP; FAMILIES; FRUITS;

D O I：

10.1016/j.procbio.2013.02.017

中图分类号：

Q5 [生物化学]; Q7 [分子生物学];

学科分类号：

071010 ; 081704 ;

摘要：

Miliin is a serine protease purified from the latex of Euphorbia milii. This work reports the effect of pH and temperature on the catalytic activity of miliin, using fluorescence resonance energy transfer (FRET) substrates. Miliin displayed the highest activity at pH 9 and 35 degrees C. Subsite mapping shows that subsites S-2 to S-2' prefer uncharged residues. The S-2 subsite prefers hydrophobic aliphatic amino acids (Val, Pro and Ile) and defines the cleavage site. This work is the first one that reports subsite mapping of Euphorbiacea proteases. The N-terminal sequence showed higher similarity (40%) with the serine protease LIM9 isolated from Lilium. The presence of Tyr, Pro and Lys at positions 2, 5 and 10 respectively, were observed for most of the serine proteases used for comparison. The N-terminal sequence has striking differences with those reported previously for milin and eumiliin, other serine proteases isolated from the latex of E. milii. (C) 2013 Elsevier Ltd. All rights reserved.

引用

页码：633 / 637

页数：5

共 49 条

[1] S3 to S3′ subsite specificity of recombinant human cathepsin K and development of selective internally quenched fluorescent substrates
Alves, MFM
Puzer, L
Cotrin, SS
Juliano, MA
Juliano, L
Brömme, D
Carmona, AK
[J]. BIOCHEMICAL JOURNAL, 2003, 373 : 981 - 986
[2] Isolation and characterization of a serine protease from the sprouts of Pleioblastus hindsii Nakai
Arima, K
Uchikoba, T
Yonezawa, H
Shimada, M
Kaneda, M
[J]. PHYTOCHEMISTRY, 2000, 54 (06) : 559 - 565
[3] Purification and characterization of a serine protease from Cucumis trigonus Roxburghi
Asif-Ullah, Mufti
Kim, Key-Sun
Yu, Yeon Gyu
[J]. PHYTOCHEMISTRY, 2006, 67 (09) : 870 - 875
[4] L-TRANS-EPOXYSUCCINYL-LEUCYLAMIDO(4-GUANIDINO)BUTANE (E-64) AND ITS ANALOGS AS INHIBITORS OF CYSTEINE PROTEINASES INCLUDING CATHEPSINS B, H AND L
BARRETT, AJ
KEMBHAVI, AA
BROWN, MA
KIRSCHKE, H
KNIGHT, CG
TAMAI, M
HANADA, K
[J]. BIOCHEMICAL JOURNAL, 1982, 201 (01) : 189 - 198
[5] PERSPECTIVES IN BIOCHEMISTRY AND BIOPHYSICS - FAMILIES AND CLANS OF SERINE PEPTIDASES
BARRETT, AJ
RAWLINGS, ND
[J]. ARCHIVES OF BIOCHEMISTRY AND BIOPHYSICS, 1995, 318 (02) : 247 - 250
[6] MAPPING ACTIVE SITE OF PAPAIN WITH AID OF PEPTIDE SUBSTRATES AND INHIBITORS
BERGER, A
SCHECHTER, I
[J]. PHILOSOPHICAL TRANSACTIONS OF THE ROYAL SOCIETY B-BIOLOGICAL SCIENCES, 1970, 257 (813) : 249 - +
[7] Hieronymain I, a new cysteine peptidase isolated from unripe fruits of Bromelia hieronymi Mez (Bromeliaceae)
Bruno, MA
Pardo, MF
Caffini, NO
López, LMI
[J]. JOURNAL OF PROTEIN CHEMISTRY, 2003, 22 (02): : 127 - 134
[8] Preliminary functional characterization, cloning and primary sequence of Fastuosain, a cysteine peptidase isolated from fruits of Bromelia fastuosa
Cabral, H
Leopoldino, AM
Tajara, EH
Greene, LJ
Faça, VM
Mateus, RP
Ceron, CR
Judice, WAD
Juliano, L
Bonilla-Rodriguez, GO
[J]. PROTEIN AND PEPTIDE LETTERS, 2006, 13 (01) : 83 - 89
[9] Carareto CMA, 2000, DROS INF SERV, V83, P178
[10] ISOLATION AND PARTIAL CHARACTERIZATION OF A PROTEASE FROM CUCURBITA-FICIFOLIA
CUROTTO, E
GONZALEZ, G
OREILLY, S
TAPIA, G
[J]. FEBS LETTERS, 1989, 243 (02): : 363 - 365

← 1 2 3 4 5 →