ELISA FOR QUANTITATION OF THE EXTRACELLULAR DOMAIN OF P185HER2 IN BIOLOGICAL-FLUIDS

被引：36

作者：

SIAS, PE

KOTTS, CE

VETTERLEIN, D

SHEPARD, M

WONG, WLT

机构：

[1] GENENTECH INC,DEPT IMMUNOL RES & ASSAY TECHNOL,460 POINT SAN BRUNO BLVD,S SAN FRANCISCO,CA 94080

[2] GENENTECH INC,DEPT MED & ANALYT CHEM,S SAN FRANCISCO,CA 94080

[3] GENENTECH INC,DEPT PROC RECOVERY,S SAN FRANCISCO,CA 94080

[4] GENENTECH INC,DEPT DEV BIOL,S SAN FRANCISCO,CA 94080

来源：

JOURNAL OF IMMUNOLOGICAL METHODS | 1990年 / 132卷 / 01期

关键词：

Bioassay; c-erbB-2; ELISA; HER2/neu;

D O I：

10.1016/0022-1759(90)90400-P

中图分类号：

Q5 [生物化学];

学科分类号：

071010 ; 081704 ;

摘要：

The HER2/neu proto-oncogene encodes a receptor that belong to the tyrosine-specific protein kinase family. Amplification of the HER2 gene in patients with breast and ovarian cancer has been shown to predict poorer survival rates. In order to understand the role of HER2 in malignant and normal cells, it is necessary to devise assays that can quantitate expression levels of the HER2 gene product (p185HER2) in production samples, biopsy specimens and biological fluids. We have developed a simple, quantitative ELISA that uses two monoclonal antibodies directed against the extracellular domain of the HER2 gene product, p185HER2 (HER2 ECD). The assay has a detection range of 0.25-120 ng/ml, is precise and sensitive. The ability of this assay to detect biologically active rHER2 ECD is demonstrated by its correlation to a growth inhibitory bioassay (r = 0.92). The sandwich ELISA can also accurately quantitate rHER2 ECD in mouse and monkey serum. This assay should be useful for quantitating low levels of circulating rHER2 ECD in animals in which rHER2 ECD is being used as antigen for immunotherapy and in patients which 'shed' receptor. © 1990.

引用

页码：73 / 80

页数：8

共 18 条

[1] TYROSINE KINASE RECEPTOR WITH EXTENSIVE HOMOLOGY TO EGF RECEPTOR SHARES CHROMOSOMAL LOCATION WITH NEU ONCOGENE
COUSSENS, L
YANGFENG, TL
LIAO, YC
CHEN, E
GRAY, A
MCGRATH, J
SEEBURG, PH
LIBERMANN, TA
SCHLESSINGER, J
FRANCKE, U
LEVINSON, A
ULLRICH, A
[J]. SCIENCE, 1985, 230 (4730) : 1132 - 1139
[2] ISOLATION OF PURE IGG1, IGG2A AND IGG2B IMMUNOGLOBULINS FROM MOUSE SERUM USING PROTEIN A-SEPHAROSE
EY, PL
PROWSE, SJ
JENKIN, CR
[J]. IMMUNOCHEMISTRY, 1978, 15 (07): : 429 - 436
[3] FENDLY BM, 1990, CANCER RES, V50, P1550
[4] LOCALIZATION OF A NOVEL V-ERBB-RELATED GENE, C-ERBB-2, ON HUMAN CHROMOSOME-17 AND ITS AMPLIFICATION IN A GASTRIC-CANCER CELL-LINE
FUKUSHIGE, S
MATSUBARA, K
YOSHIDA, M
SASAKI, M
SUZUKI, T
SEMBA, K
TOYOSHIMA, K
YAMAMOTO, T
[J]. MOLECULAR AND CELLULAR BIOLOGY, 1986, 6 (03) : 955 - 958
[5] USE OF STAPHYLOCOCCAL PROTEIN-A AS AN IMMUNOLOGICAL REAGENT
GODING, JW
[J]. JOURNAL OF IMMUNOLOGICAL METHODS, 1978, 20 (APR) : 241 - 253
[6] P185HER2 MONOCLONAL-ANTIBODY HAS ANTIPROLIFERATIVE EFFECTS INVITRO AND SENSITIZES HUMAN-BREAST TUMOR-CELLS TO TUMOR NECROSIS FACTOR
HUDZIAK, RM
LEWIS, GD
WINGET, M
FENDLY, BM
SHEPARD, HM
ULLRICH, A
[J]. MOLECULAR AND CELLULAR BIOLOGY, 1989, 9 (03) : 1165 - 1172
[7] KEARNEY JF, 1979, J IMMUNOL, V123, P1548
[8] AMPLIFICATION OF A NOVEL V-ERBB-RELATED GENE IN A HUMAN MAMMARY-CARCINOMA
KING, CR
KRAUS, MH
AARONSON, SA
[J]. SCIENCE, 1985, 229 (4717) : 974 - 976
[9] SINGLE-STEP INDUCTION OF MAMMARY ADENOCARCINOMA IN TRANSGENIC MICE BEARING THE ACTIVATED C-NEU ONCOGENE
MULLER, WJ
SINN, E
PATTENGALE, PK
WALLACE, R
LEDER, P
[J]. CELL, 1988, 54 (01) : 105 - 115
[10] PEROXIDASE-LABELED ANTIBODY - NEW METHOD OF CONJUGATION
NAKANE, PK
KAWAOI, A
[J]. JOURNAL OF HISTOCHEMISTRY & CYTOCHEMISTRY, 1974, 22 (12) : 1084 - 1091

← 1 2 →