Substrate specificity of mammalian prenyl protein-specific endoprotease activity

被引：22

作者：

Jang, GF

Gelb, MH ^{[1
]}

机构：

[1] Univ Washington, Dept Chem, Seattle, WA 98195 USA

[2] Univ Washington, Dept Biochem, Seattle, WA 98195 USA

来源：

BIOCHEMISTRY | 1998年 / 37卷 / 13期

关键词：

D O I：

10.1021/bi972289b

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：

We have previously identified proteolytic activity in rat liver microsomes that cleaves an intact tripeptide, VIS, from S-farnesylated-CVIS tetrapeptide. This enzymatic activity, termed prenyl protein-specific endoprotease (PPEP) activity, has been solubilized in CHAPS and purified 5-fold. To probe the peptide recognition features of PPEP activity, 64 tripeptides [N-acetyl-C(S-farnesyl)a(1)a(2)] were prepared and tested as competitive inhibitors of PPEP activity-catalyzed hydrolysis of N-acetyl-C(S-farnesyl)VI-[H-3]S. It was found that PPEP activity prefers large hydrophobic residues in the a(1) and a(2) positions. A subset of N-acetyl-C(S-farnesyl)a(1)a(2) peptides were prepared in radiolabeled form, and it was found that PPEP activity preferences for these substrates correlated well in most cases with the inhibition data. The exception is that R in the a(1) position does not prevent binding of peptide to PPEP activity, but such peptides are poor substrates. The anionic residue D in the a(2) position is not tolerated by PPEP activity. Five farnesylated radiolabeled tetrapeptides, Ac-C(F)FM[H-3]L, Ac-C(F)LI[H-3]L, Ac-C(F)LL[H-3]L, Ac-C(F)LM[(3)h]L, and Ac-C(F)VI[H-3]L were prepared, and PPEP activity kinetic studies revealed that they are good substrates and show comparable K-M values (2.2-13.5 mu M). Ac-C(F)RL[H-3]S is a poor substrate. The reported peptide binding preferences of PPEP activity should be useful in designing compounds that block the C-terminal proteolysis of prenylated proteins. Nonprenylated peptides do not bind to PPEP activity, and replacement of the farnesyl group with an n-pentadecyl group modestly reduces binding. Peptide-membrane partitioning studies were used together with theoretical arguments to fully understand the substrate specificity of PPEP activity toward these compounds.

引用

页码：4473 / 4481

页数：9

共 50 条

[31] PRENYLATED PROTEIN METHYLTRANSFERASES DO NOT DISTINGUISH BETWEEN FARNESYLATED AND GERANYLGERANYLATED SUBSTRATES
PEREZSALA, D
GILBERT, BA
TAN, EW
RANDO, RR
[J]. BIOCHEMICAL JOURNAL, 1992, 284 : 835 - 840
[32] PILLINGER MH, 1994, J BIOL CHEM, V269, P1486
[33] REISS Y, 1992, J BIOL CHEM, V267, P6403
[34] SEQUENCE REQUIREMENT FOR PEPTIDE RECOGNITION BY RAT-BRAIN P21RAS PROTEIN FARNESYLTRANSFERASE
REISS, Y
STRADLEY, SJ
GIERASCH, LM
BROWN, MS
GOLDSTEIN, JL
[J]. PROCEEDINGS OF THE NATIONAL ACADEMY OF SCIENCES OF THE UNITED STATES OF AMERICA, 1991, 88 (03) : 732 - 736
[35] INHIBITION OF PURIFIED P21RAS FARNESYL - PROTEIN TRANSFERASE BY CYS-AAX TETRAPEPTIDES
REISS, Y
GOLDSTEIN, JL
SEABRA, MC
CASEY, PJ
BROWN, MS
[J]. CELL, 1990, 62 (01) : 81 - 88
[36] NUCLEOTIDE-SEQUENCE OF THE YEAST STE14 GENE, WHICH ENCODES FARNESYLCYSTEINE CARBOXYL METHYLTRANSFERASE, AND DEMONSTRATION OF ITS ESSENTIAL ROLE IN A-FACTOR EXPORT
SAPPERSTEIN, S
BERKOWER, C
MICHAELIS, S
[J]. MOLECULAR AND CELLULAR BIOLOGY, 1994, 14 (02) : 1438 - 1449
[37] ENZYMATIC COUPLING OF CHOLESTEROL INTERMEDIATES TO A MATING PHEROMONE PRECURSOR AND TO THE RAS PROTEIN
SCHAFER, WR
TRUEBLOOD, CE
YANG, CC
MAYER, MP
ROSENBERG, S
POULTER, CD
KIM, SH
RINE, J
[J]. SCIENCE, 1990, 249 (4973) : 1133 - 1139
[38] PROTEIN FARNESYLTRANSFERASE AND GERANYLGERANYLTRANSFERASE SHARE A COMMON ALPHA-SUBUNIT
SEABRA, MC
REISS, Y
CASEY, PJ
BROWN, MS
GOLDSTEIN, JL
[J]. CELL, 1991, 65 (03) : 429 - 434
[39] SHI YQ, 1992, J BIOL CHEM, V267, P9547
[40] STEPHENSON RC, 1992, J BIOL CHEM, V267, P13314

← 1 2 3 4 5 →