Clinical Cancer Research AACR Conference on Cancer Prevention
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Clinical Cancer Research Vol. 10, 3479-3489, May 15, 2004
© 2004 American Association for Cancer Research


Molecular Oncology, Markers, Clinical Correlates

Rapid and Sensitive p53 Alteration Analysis in Biopsies from Lung Cancer Patients Using a Functional Assay and A Universal Oligonucleotide Array

A Prospective Study

Coralie Fouquet1, Martine Antoine1,2, Pascaline Tisserand1, Reyna Favis4, Marie Wislez1,3, Fréderic Commo2, Nathalie Rabbe1,3, Marie France Carette1,3, Bernard Milleron1,3, Francis Barany4, Jacques Cadranel1,3, Gérard Zalcman1 and Thierry Soussi1

1 Laboratoire de génotoxicologie des tumeurs, Paris, France; 2 Service d’Anatomie Pathologique, and 3 Service de Pneumologie et de Radiologie, Hôpital Tenon, Paris, France; and 4 Department of Microbiology, Cornell University, New York, New York

Purpose: Molecular profiling of alterations associated with lung cancer holds the promise to define clinical parameters such as response to treatment or survival. Because <5% of small cell lung cancers and <30% of non-small cell lung cancers are surgically resectable, molecular analysis will perforce rely on routinely available clinical samples such as biopsies. Identifying tumor mutations in such samples will require a sensitive and robust technology to overcome signal from excess amounts of normal DNA.

Experimental Design: p53 mutation status was assessed from the DNA and RNA of biopsies collected prospectively from 83 patients with lung cancer. Biopsies were obtained either by conventional bronchoscopy or computed tomography-guided percutaneous biopsy. Matched surgical specimens were available for 22 patients. Three assays were used: direct sequencing; a functional assay in yeast; and a newly developed PCR/ligase detection reaction/Universal DNA array assay.

Results: Using the functional assay, p53 mutation was found in 62% of biopsies and 64% of surgical specimens with a concordance of 80%. The sensitivity of the functional assay was determined to be 5%. Direct sequencing confirmed mutations in 92% of surgical specimens but in only 78% of biopsies. The DNA array confirmed 100% of mutations in both biopsies and surgical specimens. Using this newly developed DNA array, we demonstrate the feasibility of directly identifying p53 mutations in clinical samples containing <5% of tumor cells.

Conclusions: The versatility and sensitivity of this new array assay should allow additional development of mutation profiling arrays that could be applied to biological samples with a low tumor cell content such as bronchial aspirates, bronchoalveolar lavage fluid, or serum.




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H. Pincas, M. R. Pingle, J. Huang, K. Lao, P. B. Paty, A. M. Friedman, and F. Barany
High sensitivity EndoV mutation scanning through real-time ligase proofreading
Nucleic Acids Res., October 28, 2004; 32(19): e148 - e148.
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HOME HELP FEEDBACK SUBSCRIPTIONS ARCHIVE SEARCH TABLE OF CONTENTS
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Copyright © 2004 by the American Association for Cancer Research.