Determination of copy number of c-Myc protein per cell by quantitative Western blotting

被引:43
作者
Rudolph, C
Adam, G
Simm, A
机构
[1] Univ Konstanz, Fak Biol, Arbeitsgrp Zellbiol Tumorbiol, D-78457 Constance, Germany
[2] Biozentrum, D-97074 Wurzburg, Germany
关键词
D O I
10.1006/abio.1999.3095
中图分类号
Q5 [生物化学];
学科分类号
071010 ; 081704 ;
摘要
The protooncogene c-Myc plays a key role in growth control, differentiation, and apoptosis. An abnormally high expression of c-myc has been found to be associated with many neoplasms. c-Myc gene expression is usually measured at the mRNA level Few studies have been published on quantitative Myc protein determination. A major drawback of ELISA (enzyme-linked immunosorbent assay) methods is the uncertainty of the specificity of the antibody reaction. In contrast, antibody specificity can be easily controlled by Western/immunoblotting. Here we describe a method to quantify c-Myc protein in primary human IMR90 lung fibroblasts based on Western blotting Using a high-resolution polyacrylamide gel, we were able to differentiate the cellular c-Myc protein (64 kDa) from a c-Myc internal standard (65 kDa). We determined both the total c-Myc protein content per cell and its distribution in the cytoplasmic and nuclear fractions. About 4000 c-Myc protein molecules were detected in the cytoplasmic fraction and 29,000 copies in the nuclear fraction for proliferating human limp fibroblasts IMR90. The ratio of nuclear (active) to cytoplasmic (inactive) c-Myc protein changed from 17:1 for proliferating cells to 2.5:1 for confluent cells. (C) 1999 Academic Press.
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页码:66 / 71
页数:6
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