MOLECULAR-CLONING AND BACTERIAL EXPRESSION OF CDNA FOR RAT CALPAIN-II 80 KDA SUBUNIT

被引：52

作者：

DELUCA, CI ^{[1
]}

DAVIES, PL ^{[1
]}

SAMIS, JA ^{[1
]}

ELCE, JS ^{[1
]}

机构：

[1] QUEENS UNIV, DEPT BIOCHEM, KINGSTON K7L 3N6, ONTARIO, CANADA

来源：

BIOCHIMICA ET BIOPHYSICA ACTA | 1993年 / 1216卷 / 01期

基金：

英国医学研究理事会;

关键词：

CALPAIN; CLONING; GENE EXPRESSION; PROTEINASE; (RAT);

D O I：

10.1016/0167-4781(93)90040-K

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：

The complete cDNA of 3.2 kb for rat calpain II large subunit has been constructed from library- and polymerase chain reaction-derived fragments, and sequenced. The cDNA encodes a protein of 700 amino acids having 93% sequence identity with human calpain II, and 61% identity with human calpain I. The gene possesses 21 exons, of which exons 3-21 have been mapped over 33 kb of the rat genome. A new phagemid expression vector was created from pT7-7 by insertion of the f1 origin and mutation of an NdeI to an NcoI site. Rat calpain II cDNA ligated into this vector expressed in Escherichia coli an 80 kDa protein identical in size to highly purified rat calpain II; this protein was specifically recognized on immunoblots by an affinity-purified anti-rat calpain II antibody. This is the second mammalian calpain II large subunit to be fully sequenced, and the first to be artificially expressed.

引用

页码：81 / 93

页数：13

共 29 条

[1] COMPLETE AMINO-ACID-SEQUENCE OF THE LARGE SUBUNIT OF THE LOW-CA-2+-REQUIRING FORM OF HUMAN CA-2+-ACTIVATED NEUTRAL PROTEASE (MU-CANP) DEDUCED FROM ITS CDNA SEQUENCE [J].

AOKI, K ;

IMAJOH, S ;

OHNO, S ;

EMORI, Y ;

KOIKE, M ;

KOSAKI, G ;

SUZUKI, K .

FEBS LETTERS, 1986, 205 (02) :313-317

[2]

BOORSTEIN WR, 1989, METHOD ENZYMOL, V180, P347

[3]

CHOMCZYNSKI P, 1987, ANAL BIOCHEM, V162, P156, DOI 10.1016/0003-2697(87)90021-2

[4] CALCIUM-ACTIVATED NEUTRAL PROTEASE (CALPAIN) SYSTEM - STRUCTURE, FUNCTION, AND REGULATION [J].

CROALL, DE ;

DEMARTINO, GN .

PHYSIOLOGICAL REVIEWS, 1991, 71 (03) :813-847

[5] CA-2+-ACTIVATED PROTEINASE IN THE RAT - QUANTIFICATION BY IMMUNOASSAY IN THE UTERUS DURING PREGNANCY AND INVOLUTION, AND IN OTHER TISSUES [J].

ELCE, JS ;

BAENZIGER, JE ;

YOUNG, DCR .

BIOCHEMICAL JOURNAL, 1984, 220 (02) :507-512

[6] GENE STRUCTURE OF CALCIUM-DEPENDENT PROTEASE RETAINS THE ANCESTRAL ORGANIZATION OF THE CALCIUM-BINDING PROTEIN GENE [J].

EMORI, Y ;

OHNO, S ;

TOBITA, M ;

SUZUKI, K .

FEBS LETTERS, 1986, 194 (02) :249-252

[7]

EMORI Y, 1986, J BIOL CHEM, V261, P9465

[8] RAPID PRODUCTION OF FULL-LENGTH CDNAS FROM RARE TRANSCRIPTS - AMPLIFICATION USING A SINGLE GENE-SPECIFIC OLIGONUCLEOTIDE PRIMER [J].

FROHMAN, MA ;

DUSH, MK ;

MARTIN, GR .

PROCEEDINGS OF THE NATIONAL ACADEMY OF SCIENCES OF THE UNITED STATES OF AMERICA, 1988, 85 (23) :8998-9002

[9] IS CALPAIN ACTIVITY REGULATED BY MEMBRANES AND AUTOLYSIS OR BY CALCIUM AND CALPASTATIN [J].

GOLL, DE ;

THOMPSON, VF ;

TAYLOR, RG ;

ZALEWSKA, T .

BIOESSAYS, 1992, 14 (08) :549-556

[10] A SIMPLE AND VERY EFFICIENT METHOD FOR GENERATING CDNA LIBRARIES [J].

GUBLER, U ;

HOFFMAN, BJ .

GENE, 1983, 25 (2-3) :263-269

← 1 2 3 →