RECOVERY OF A CHARGED-FUSION PROTEIN FROM CELL-EXTRACTS BY POLYELECTROLYTE PRECIPITATION

被引：28

作者：

PARKER, DE

GLATZ, CE

FORD, CF

GENDEL, SM

SUOMINEN, I

ROUGVIE, MA

机构：

[1] IOWA STATE UNIV SCI & TECHNOL,DEPT CHEM ENGN,AMES,IA 50011

[2] IOWA STATE UNIV SCI & TECHNOL,DEPT GENET,AMES,IA 50011

[3] IOWA STATE UNIV SCI & TECHNOL,DEPT BIOCHEM & BIOPHYS,AMES,IA 50011

来源：

BIOTECHNOLOGY AND BIOENGINEERING | 1990年 / 36卷 / 05期

关键词：

D O I：

10.1002/bit.260360506

中图分类号：

Q81 [生物工程学（生物技术）]; Q93 [微生物学];

学科分类号：

071005 ; 0836 ; 090102 ; 100705 ;

摘要：

β‐Galactosidase served as a model system to explore the feasibility of enhancing the selectivity of a low‐cost, easily scaled separation method—precipitation. Enhanced selectivity was sought by fusing the enzyme with polypeptide tails including 5 and 11 aspartaies. The unfused protein could not be selectively removed from the Escherichia coli cell extract by precipitation with polyethylenimine (PEI), but the longest fusion could be selectively removed. The presence of nucleic acids limited the purification attainable. Pretreatment with nuclease followed by diafiltration resulted in an extract from which the same fusion could be precipitated with greater than fivefold enrichment, while the untailed enzyme remained unenriched by the same precipitation step. Selectivitiy is attributed to the binding strength of the polyanionic tails to the polycationic PEI. Copyright © 1990 John Wiley & Sons, Inc.

引用

页码：467 / 475

页数：9

共 25 条

[1] SECRETION OF HETEROLOGOUS GENE-PRODUCTS TO THE CULTURE-MEDIUM OF ESCHERICHIA-COLI [J].

ABRAHMSEN, L ;

MOKS, T ;

NILSSON, B ;

UHLEN, M .

NUCLEIC ACIDS RESEARCH, 1986, 14 (18) :7487-7500

[2] PRECIPITATION OF NUCLEIC-ACIDS WITH POLYETHYLENEIMINE AND CHROMATOGRAPHY OF NUCLEIC-ACIDS AND PROTEINS ON IMMOBILIZED POLYETHYLENEIMINE [J].

ATKINSON, A ;

JACK, GW .

BIOCHIMICA ET BIOPHYSICA ACTA, 1973, 308 (01) :41-52

[3]

BJURSTROM E, 1985, CHEM ENG-NEW YORK, V92, P126

[4]

BRADFORD MM, 1976, ANAL BIOCHEM, V72, P248, DOI 10.1016/0003-2697(76)90527-3

[5]

CORDES RM, 1987, THESIS IOWA STATE U

[6] RAPID PURIFICATION OF A CLONED GENE-PRODUCT BY GENETIC FUSION AND SITE-SPECIFIC PROTEOLYSIS [J].

GERMINO, J ;

BASTIA, D .

PROCEEDINGS OF THE NATIONAL ACADEMY OF SCIENCES OF THE UNITED STATES OF AMERICA-BIOLOGICAL SCIENCES, 1984, 81 (15) :4692-4696

[7] PROTEOLYTIC DEGRADATION OF FUSED PROTEIN A-BETA-GALACTOSIDASE IN ESCHERICHIA-COLI [J].

HELLEBUST, H ;

VEIDE, A ;

ENFORS, SO .

JOURNAL OF BIOTECHNOLOGY, 1988, 7 (03) :185-198

[8]

Herbert D., 1971, METHODS MICROBIOL, V5 B, P209, DOI [10.1016/S0580-9517(08)70641-X, DOI 10.1016/S0580-9517(08)70641-X]

[9] GENETIC APPROACH TO FACILITATE PURIFICATION OF RECOMBINANT PROTEINS WITH A NOVEL METAL CHELATE ADSORBENT [J].

HOCHULI, E ;

BANNWARTH, W ;

DOBELI, H ;

GENTZ, R ;

STUBER, D .

BIO-TECHNOLOGY, 1988, 6 (11) :1321-1325

[10] A SHORT POLYPEPTIDE MARKER SEQUENCE USEFUL FOR RECOMBINANT PROTEIN IDENTIFICATION AND PURIFICATION [J].

HOPP, TP ;

PRICKETT, KS ;

PRICE, VL ;

LIBBY, RT ;

MARCH, CJ ;

CERRETTI, DP ;

URDAL, DL ;

CONLON, PJ .

BIO-TECHNOLOGY, 1988, 6 (10) :1204-1210

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