IDENTIFICATION AND EXPRESSION OF 2 FORMS OF THE HUMAN TRANSFORMING GROWTH FACTOR-BETA-BINDING PROTEIN ENDOGLIN WITH DISTINCT CYTOPLASMIC REGIONS

被引：193

作者：

BELLON, T

CORBI, A

LASTRES, P

CALES, C

CEBRIAN, M

VERA, S

CHEIFETZ, S

MASSAGUE, J

LETARTE, M

BERNABEU, C

机构：

[1] CSIC,CTR INVEST BIOL,VELAZQUEZ 144,E-28006 MADRID,SPAIN

[2] HOSP LA PRINCESA,UNIDAD BIOL MOLEC,MADRID,SPAIN

[3] HOSP SICK CHILDREN,DIV IMMUNOL & CANC RES,TORONTO M5G 1X8,ONTARIO,CANADA

[4] MEM SLOAN KETTERING CANC CTR,HOWARD HUGHES MED INST,CELL BIOL & GENET PROGRAM,NEW YORK,NY 10021

来源：

EUROPEAN JOURNAL OF IMMUNOLOGY | 1993年 / 23卷 / 09期

关键词：

ENDOGLIN; MACROPHAGES; TRANSFORMING GROWTH FACTOR-BETA;

D O I：

10.1002/eji.1830230943

中图分类号：

R392 [医学免疫学]; Q939.91 [免疫学];

学科分类号：

100102 ;

摘要：

Endoglin is an homodimeric membrane antigen with capacity to bind transforming growth factor-beta (TGF-beta) and whose expression is up-regulated on myeloid cells upon differentiation to macrophages. We have isolated full-length cDNA clones from a lambdagt10 library, prepared from phorbol 12-myristate 13-acetate-differentiated HL60 cells by screening with an endoglin-specific cDNA probe from endothelial cells. Sequencing of the largest clone (3073 bp), revealed that the leader sequence contains 25 residues and that the 586 amino acids of the extracellular and transmembrane domains were identical to those described for endothelial endoglin. However, the cytoplasmic tail encoded by this cDNA clone contains only 14 amino acids as opposed to the 47 residues previously reported, suggesting the existence of two alternative endoglin variants. The expression of these isoforms was demonstrated by polymerase chain reaction analyses on endothelial cells, myelomonocytic cell lines HL-60 and U-937, and placenta. Independent cDNA constructs corresponding to both forms were transfected into mouse fibroblasts leading to the expression of two distinct endoglin molecules. Both forms were shown to bind TGF-beta1 and, when overexpressed in transfected mouse fibroblasts. to form disulfide-linked homodimers, indicating that the cysteine residues present in the extracellular domain are responsible for the dimerization.

引用

页码：2340 / 2345

页数：6

共 27 条

[1] NOVEL ACTIVIN RECEPTORS - DISTINCT GENES AND ALTERNATIVE MESSENGER-RNA SPLICING GENERATE A REPERTOIRE OF SERINE THREONINE KINASE RECEPTORS
ATTISANO, L
WRANA, JL
CHEIFETZ, S
MASSAGUE, J
[J]. CELL, 1992, 68 (01) : 97 - 108
[2] BUHRING HJ, 1991, LEUKEMIA, V5, P841
[3] CELADA A, 1992, J IMMUNOL, V148, P1102
[4] CHEIFETZ S, 1991, J BIOL CHEM, V266, P20767
[5] CHEIFETZ S, 1992, J BIOL CHEM, V267, P19027
[6] CHEIFETZ S, 1989, J BIOL CHEM, V264, P12025
[7] ISOLATION OF BIOLOGICALLY-ACTIVE RIBONUCLEIC-ACID FROM SOURCES ENRICHED IN RIBONUCLEASE
CHIRGWIN, JM
PRZYBYLA, AE
MACDONALD, RJ
RUTTER, WJ
[J]. BIOCHEMISTRY, 1979, 18 (24) : 5294 - 5299
[8] CDNA CLONING AND COMPLETE PRIMARY STRUCTURE OF THE ALPHA-SUBUNIT OF A LEUKOCYTE ADHESION GLYCOPROTEIN, P150,95
CORBI, AL
MILLER, LJ
OCONNOR, K
LARSON, RS
SPRINGER, TA
[J]. EMBO JOURNAL, 1987, 6 (13) : 4023 - 4028
[9] Gilliland G., 1990, PCR PROTOCOLS GUIDE, P60
[10] GOUGOS A, 1988, J IMMUNOL, V141, P1925

← 1 2 3 →