FLOW CYTOMETRIC METHOD FOR THE MEASUREMENT OF EPIDERMAL GROWTH-FACTOR RECEPTOR AND COMPARISON WITH THE RADIO-LIGAND BINDING ASSAY

被引：31

作者：

BROTHERICK, I

LENNARD, TWJ

WILKINSON, SE

COOK, S

ANGUS, B

SHENTON, BK

机构：

[1] UNIV NEWCASTLE UPON TYNE,SCH MED,DEPT SURG,NEWCASTLE TYNE NE2 4HH,ENGLAND

[2] UNIV NEWCASTLE UPON TYNE,SCH MED,DEPT PATHOL,NEWCASTLE TYNE NE2 4HH,ENGLAND

来源：

CYTOMETRY | 1994年 / 16卷 / 03期

关键词：

FLOW CYTOMETRY; EGF-R; SAPONIN; RADIO-LIGAND BINDING;

D O I：

10.1002/cyto.990160311

中图分类号：

Q5 [生物化学];

学科分类号：

071010 ; 081704 ;

摘要：

A method for the purification, conjugation, and use of EGF-R antibody 60 quantify EGF receptors on tumour cells by flow cytometry is described. The quantification of both internal and external EGF receptors was determined by treatment with saponin, rendering the cells permeable 60 the EGF-R antibody. Using QCS bead standards, the number of EGF-R binding sites per cell was assessed. Results were compared with conventional EGF-R quantification using a radio-ligand binding assay. A high degree of correlation was found between the two methods. The flow cytometric method for EGF-R quantification described is sim-ple, rapid, and reproducible. The assay may be of particular value in measuring EGF-R on urgent clinical samples or those that are too small (such as breast aspirates) for measurement by the radio-ligand binding assay. Advantages of this assay over the radio-ligand binding assay include reduction in use of radio-labelled iodine compounds, a decrease in analysis time, and reduced cost and quantity of material needed for assay. In addition, flow cytometry offers the possibility of selecting cell phenotypes by gating as well as live/dead cells by using multi-parameter flow cytometry. (C) 1994 Wiley-Liss,Inc.

引用

页码：262 / 269

页数：8

共 15 条

[1] EPIDERMAL GROWTH-FACTOR RECEPTORS
ADAMSON, ED
REES, AR
[J]. MOLECULAR AND CELLULAR BIOCHEMISTRY, 1981, 34 (03) : 129 - 152
[2] ENUMERATION OF ANTIGEN SITES ON CELLS BY FLOW-CYTOMETRY
DAWSON, CD
SCHEPPLER, JA
NICHOLSON, JKA
HOLMAN, RC
[J]. PATHOBIOLOGY, 1991, 59 (02) : 57 - 61
[3] FABBRO D, 1986, CANCER RES, V46, P2720
[4] FITZPATRICK SL, 1984, CANCER RES, V44, P3443
[5] GIVAN AL, 1991, CYTOMETRY, V4, P360
[6] USE OF DETERGENTS AND IMMUNOPEROXIDASE REAGENTS FOR ULTRASTRUCTURAL DEMONSTRATION OF INTERNAL IMMUNOGLOBULIN IN LYMPH CELLS
HALL, JG
BIRBECK, MSC
ROBERTSON, D
PEPPARD, J
ORLANS, E
[J]. JOURNAL OF IMMUNOLOGICAL METHODS, 1978, 19 (04) : 351 - 359
[7] IMAI Y, 1982, CANCER RES, V42, P4394
[8] LOPEZ JG, 1992, INVEST OPHTH VIS SCI, V33, P2053
[9] QUANTITATIVE ASSAYS OF EPIDERMAL GROWTH-FACTOR RECEPTOR IN HUMAN-BREAST CANCER - CUTOFFS POINTS OF CLINICAL RELEVANCE
NICHOLSON, S
SAINSBURY, JRC
NEEDHAM, GK
CHAMBERS, P
FARNDON, JR
HARRIS, AL
[J]. INTERNATIONAL JOURNAL OF CANCER, 1988, 42 (01) : 36 - 41
[10] OSBORNE CK, 1984, J CLIN ENDOCR METAB, V55, P86

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