SEQUENCE VERIFICATION OF HUMAN CREATINE-KINASE (43 KDA) ISOZYMES BY HIGH-RESOLUTION TANDEM MASS-SPECTROMETRY

被引：39

作者：

WOOD, TD ^{[1
]}

CHEN, LH ^{[1
]}

WHITE, CB ^{[1
]}

BABBITT, PC ^{[1
]}

KENYON, GL ^{[1
]}

MCLAFFERTY, FW ^{[1
]}

机构：

[1] UNIV CALIF SAN FRANCISCO,DEPT PHARMACEUT CHEM,SAN FRANCISCO,CA 94143

来源：

PROCEEDINGS OF THE NATIONAL ACADEMY OF SCIENCES OF THE UNITED STATES OF AMERICA | 1995年 / 92卷 / 25期

关键词：

ELECTROSPRAY IONIZATION; FOURIER-TRANSFORM MASS SPECTROMETRY; PROTEIN SEQUENCING;

D O I：

10.1073/pnas.92.25.11451

中图分类号：

O [数理科学和化学]; P [天文学、地球科学]; Q [生物科学]; N [自然科学总论];

学科分类号：

07 ; 0710 ; 09 ;

摘要：

Amino acid sequencing by recombinant DNA technology, although dramatically useful, is subject to base reading errors, is indirect, and is insensitive to posttranslational processing. Mass spectrometry techniques can provide molecular weight data from even relatively large proteins for such cDNA sequences and can serve as a check of an enzyme's purity and sequence integrity. Multiply-charged ions from electrospray ionization can be dissociated to yield structural information by tandem mass spectrometry, providing a second method for gaining additional confidence in primary sequence confirmation. Here, accurate (+/-1 Da) molecular weight and molecular ion dissociation information for human muscle and brain creatine kinases has been obtained by electrospray ionization coupled with Fourier-transform mass spectrometry to help distinguish which of several published amino acid sequences for both enzymes are correct. The results herein are consistent with one published sequence for each isozyme, and the heterogeneity indicated by isoelectric focusing due to 1-Da deamidation changes. This approach appears generally useful for detailed sequence verification of recombinant proteins.

引用

页码：11451 / 11455

页数：5

共 36 条

[1] EXPRESSION OF A RAT-BRAIN CREATINE KINASE-BETA-GALACTOSIDASE FUSION PROTEIN IN ESCHERICHIA-COLI AND DERIVATION OF THE COMPLETE AMINO-ACID-SEQUENCE OF RAT-BRAIN CREATINE-KINASE [J].

BENFIELD, PA ;

HENDERSON, L ;

PEARSON, ML .

GENE, 1985, 39 (2-3) :263-267

[2] FOURIER-TRANSFORM ELECTROSPRAY INSTRUMENTATION FOR TANDEM HIGH-RESOLUTION MASS-SPECTROMETRY OF LARGE MOLECULES [J].

BEU, SC ;

SENKO, MW ;

QUINN, JP ;

WAMPLER, FM ;

MCLAFFERTY, FW .

JOURNAL OF THE AMERICAN SOCIETY FOR MASS SPECTROMETRY, 1993, 4 (07) :557-565

[3] THE MOUSE MUSCLE CREATINE-KINASE CDNA AND DEDUCED AMINO-ACID SEQUENCES - COMPARISON TO EVOLUTIONARILY RELATED ENZYMES [J].

BUSKIN, JN ;

JAYNES, JB ;

CHAMBERLAIN, JS ;

HAUSCHKA, SD .

JOURNAL OF MOLECULAR EVOLUTION, 1985, 22 (04) :334-341

[4]

CHEN LH, 1991, J BIOL CHEM, V266, P12053

[5] ELECTROSPRAY IONIZATION-PRINCIPLES AND PRACTICE [J].

FENN, JB ;

MANN, M ;

MENG, CK ;

WONG, SF ;

WHITEHOUSE, CM .

MASS SPECTROMETRY REVIEWS, 1990, 9 (01) :37-70

[6] SUSTAINED OFF-RESONANCE IRRADIATION FOR COLLISION-ACTIVATED DISSOCIATION INVOLVING FOURIER-TRANSFORM MASS-SPECTROMETRY - COLLISION-ACTIVATED DISSOCIATION TECHNIQUE THAT EMULATES INFRARED MULTIPHOTON DISSOCIATION [J].

GAUTHIER, JW ;

TRAUTMAN, TR ;

JACOBSON, DB .

ANALYTICA CHIMICA ACTA, 1991, 246 (01) :211-225

[7] COMPLETE NUCLEOTIDE-SEQUENCE OF TORPEDO-MARMORATA MESSENGER-RNA CODING FOR THE 43,000-DALTON NU-2-PROTEIN - MUSCLE-SPECIFIC CREATINE-KINASE [J].

GIRAUDAT, J ;

DEVILLERSTHIERY, A ;

PERRIARD, JC ;

CHANGEUX, JP .

PROCEEDINGS OF THE NATIONAL ACADEMY OF SCIENCES OF THE UNITED STATES OF AMERICA-BIOLOGICAL SCIENCES, 1984, 81 (23) :7313-7317

[8] HIGH-RESOLUTION ELECTROSPRAY MASS-SPECTRA OF LARGE MOLECULES [J].

HENRY, KD ;

QUINN, JP ;

MCLAFFERTY, FW .

JOURNAL OF THE AMERICAN CHEMICAL SOCIETY, 1991, 113 (14) :5447-5449

[9]

HILLENKAMP F, 1991, ANAL CHEM, V63, pA1193

[10] THE PRIMARY STRUCTURE OF CHICKEN B-CREATINE KINASE AND EVIDENCE FOR HETEROGENEITY OF ITS MESSENGER-RNA [J].

HOSSLE, JP ;

ROSENBERG, UB ;

SCHAFER, B ;

EPPENBERGER, HM ;

PERRIARD, JC .

NUCLEIC ACIDS RESEARCH, 1986, 14 (03) :1449-1463

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