Abstract
Amplification of genomic DNA encoding oncogenes such as HER-2 (syn. c-erbB2/c-neu) may be substantially involved in the initiation and progression of breast cancer. In order to refine and facilitate the quantitative analysis of HER-2 amplification in breast cancer, differential polymerase chain reaction (PCR) was performed on DNA derived from single cryosections of tumor tissue. This technique is based on the simultaneous amplification of a potentially amplified oncogene (HER-2) and a reference gene (IFN-gamma). Differential PCR yielded reproducible results that were in agreement with gene copy quantification using the dot blot technique. Thus we suggest differential PCR to be a reliable and rapid method for determining relative gene dosage in a minute amount of tumour tissue.
Original language | English |
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Pages (from-to) | 209-212 |
Number of pages | 4 |
Journal | Virchows Archiv B Cell Pathology Including Molecular Pathology |
Volume | 64 |
Issue number | 1 |
DOIs | |
State | Published - Dec 1993 |
Keywords
- Breast cancer
- Cryosection
- Differential polymerase chain reaction
- HER-2 oncogene amplification