INVITRO EXPRESSION AND SECRETION OF FUNCTIONAL MAMMALIAN INTRINSIC-FACTOR USING RECOMBINANT BACULOVIRUS

被引：14

作者：

GORDON, M ^{[1
]}

CHOKSHI, H ^{[1
]}

ALPERS, DH ^{[1
]}

机构：

[1] WASHINGTON UNIV,SCH MED,DEPT MED,DIV GASTROENTEROL,660 S EUCLID,BOX 8124,ST LOUIS,MO 63110

来源：

BIOCHIMICA ET BIOPHYSICA ACTA | 1992年 / 1132卷 / 03期

关键词：

COBALAMIN BINDING PROTEIN; IF-CBL; EUKARYOTIC EXPRESSION;

D O I：

10.1016/0167-4781(92)90161-R

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：

Intrinsic factor was produced at levels of 1-2 mg per 1 (0.25 mug per 10(6) cells) by growth of recombinant baculovirus-infected Sf9 cells in spinner culture. The recombinant IF showed a binding affinity for cobalamin (2.6 . 10(-10) M) and for the intrinsic factor-cobalamin receptor (3.5 . 10(-10) M) nearly identical with native IF. Purification of the recombinant intrinsic factor could be accomplished by affinity chromatography, but final purification by gel chromatography (FPLC) was necessary to separate intrinsic factor from a 62 kDa protein secreted from uninfected Sf9 cells. This protein binds selectively to the cobalamin-Sepharose column, but demonstrates no cobalamin binding activity after elution. Microgram quantities of radiolabelled protein could be produced for metabolic and autoradiographic studies. The stability of intrinsic factor to pancreatic proteinases was nearly identical with human gastric intrinsic factor, both native and recombinant as produced in mammalian cells. Glycosylation of the intrinsic factor was demonstrated by lectin binding to the recombinant protein separated on SDS-PAGE, and by a shift in apparent molecular mass from 47 kDa to 43 kDa following treatment of Sf9 cells with tunicamycin. Most of the recombinant IF was produced by Sf9 cells in the first 48 h post infection.

引用

页码：276 / 283

页数：8

共 26 条

[1]

Allen R H, 1975, Prog Hematol, V9, P57

[2]

CHOKSHI H, 1991, Gastroenterology, V100, pA517

[3] ASPARAGINE-LINKED OLIGOSACCHARIDE PROCESSING IN LEPIDOPTERAN INSECT CELLS - TEMPORAL DEPENDENCE OF THE NATURE OF THE OLIGOSACCHARIDES ASSEMBLED ON ASPARAGINE-289 OF RECOMBINANT HUMAN PLASMINOGEN PRODUCED IN BACULOVIRUS VECTOR INFECTED SPODOPTERA-FRUGIPERDA (IPLB-SF-21AE) CELLS [J].

DAVIDSON, DJ ;

CASTELLINO, FJ .

BIOCHEMISTRY, 1991, 30 (25) :6167-6174

[4] ISOLATION AND STRUCTURAL CHARACTERIZATION OF A CDNA CLONE ENCODING RAT GASTRIC INTRINSIC-FACTOR [J].

DIECKGRAEFE, BK ;

SEETHARAM, B ;

BANASZAK, L ;

LEYKAM, JF ;

ALPERS, DH .

PROCEEDINGS OF THE NATIONAL ACADEMY OF SCIENCES OF THE UNITED STATES OF AMERICA, 1988, 85 (01) :46-50

[5] GLYCOSYLATION IS NOT REQUIRED FOR LIGAND OR RECEPTOR-BINDING BY EXPRESSED RAT INTRINSIC-FACTOR [J].

GORDON, MM ;

HU, C ;

CHOKSHI, H ;

HEWITT, JE ;

ALPERS, DH .

AMERICAN JOURNAL OF PHYSIOLOGY, 1991, 260 (05) :G736-G742

[6] RAPID CHARCOAL ASSAY FOR INTRINSIC FACTOR (IF) GASTRIC JUICE UNSATURATED B12 BINDING CAPACITY ANTIBODY TO IF AND SERUM UNSATURATED B12 BINDING CAPACITY [J].

GOTTLIEB, C ;

LAU, KS ;

WASSERMA.LR ;

HERBERT, V .

BLOOD-THE JOURNAL OF HEMATOLOGY, 1965, 25 (06) :875-&

[7] ESTABLISHMENT OF 4 STRAINS OF CELLS FROM INSECT TISSUES GROWN IN VITRO [J].

GRACE, TDC .

NATURE, 1962, 195 (4843) :788-&

[8] PURIFICATION OF HUMAN INTRINSIC-FACTOR USING HIGH-PERFORMANCE ION-EXCHANGE CHROMATOGRAPHY AS THE FINAL STEP [J].

GUEANT, JL ;

KOUVONEN, I ;

MICHALSKI, JC ;

MASSON, C ;

GRASBECK, R ;

NICOLAS, JP .

FEBS LETTERS, 1985, 184 (01) :14-19

[9] AUTORADIOGRAPHIC LOCALIZATION OF IODINATED HUMAN INTRINSIC-FACTOR IN THE GUINEA-PIG ILEUM USING ELECTRON-MICROSCOPY [J].

GUEANT, JL ;

GERARD, A ;

MONIN, B ;

CHAMPIGNEULLE, B ;

GERARD, H ;

NICOLAS, JP .

GUT, 1988, 29 (10) :1370-1378

[10] PURIFICATION OF INTRINSIC-FACTOR RECEPTOR FROM PIG ILEUM USING AS AFFINITY MEDIUM HUMAN INTRINSIC-FACTOR COVALENTLY BOUND TO SEPHAROSE [J].

GUEANT, JL ;

JOKINEN, O ;

SCHOHN, H ;

MONIN, B ;

NICOLAS, JP ;

GRASBECK, R .

BIOCHIMICA ET BIOPHYSICA ACTA, 1989, 992 (03) :281-288

← 1 2 3 →