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JNCI Journal of the National Cancer Institute 1999 91(10):874-881;
© 1999 by Oxford University Press
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Journal of the National Cancer Institute, Vol. 91, No. 10, 874-881, May 19, 1999
© 1999 Oxford University Press


REPORTS

Prognostic Significance of Transcription Factor E2F-1 in Bladder Cancer: Genotypic and Phenotypic Characterization

Farhang Rabbani, Victoria M. Richon, Irene Orlow, Ming-Lan Lu, Marija Drobnjak, Maria Dudas, Elizabeth Charytonowicz, Guido Dalbagni, Carlos Cordon-Cardo

Affiliations of authors: F. Rabbani, G. Dalbagni (Urology Service, Department of Surgery), V. M. Richon (Cell Biology Program), I. Orlow, M.-L. Lu, M. Drobnjak, M. Dudas, E. Charytonowicz, C. Cordon-Cardo (Department of Pathology), Memorial Sloan-Kettering Cancer Center, New York, NY.

Correspondence to: Carlos Cordon-Cardo, M.D., Ph.D., Division of Molecular Pathology, Memorial Sloan-Kettering Cancer Center, Rm. S-801, 1275 York Ave., New York, NY 10021 (e-mail: cordon-c{at}mskcc.org).

BACKGROUND: We sought to identify and characterize potential alterations in E2F-1, a transcription factor that binds to the retinoblastoma protein (pRB), in bladder neoplasms and to elucidate a possible role for E2F-1 as an oncogene or a tumor suppressor gene. METHODS: Tumor samples from 133 evaluable patients with bladder cancer were analyzed for E2F-1 gene mutations by use of polymerase chain reaction-single-strand conformational polymorphism (PCR-SSCP) analysis and DNA sequencing. In addition, tumors were studied for E2F-1 and pRB protein expression by use of immunohistochemistry. Results from the above analyses were correlated with clinicopathologic parameters and outcome. All P values are two-sided. RESULTS: A polymorphism, consisting of a nucleotide change at amino acid codon 393 in exon 7 (GGC->AGC [Gly->Ser]), was identified in seven of 133 case patients, being present in both tumor and corresponding normal tissues. No band-shifts were identified in the nuclear-localization or DNA-binding domains on PCR-SSCP analysis. On immunohistochemical analysis, E2F-1 nuclear reactivity was observed in less than 5% of the cells from 53 tumors and in 5%-75% of the cells from the remaining 80 tumors. The pattern of E2F-1 protein expression was not altered in relation to the identified polymorphism. pRB nuclear reactivity greater than 20% (of tumor cells stained) was present in 66% of the samples. E2F-1 nuclear reactivity correlated inversely with the percentage of cells showing pRB reactivity (Kendall {tau}b = -0.18; P = .019). On multivariate analysis, patients with lower E2F-1 reactivity had statistically significantly increased risks of progression to metastases (P = .001) and death (P = .02). CONCLUSIONS: E2F-1 alterations occur at the phenotypic level, rather than at the genotypic level, in bladder cancer. The adverse outcome for patients whose tumors exhibit low E2F-1 nuclear expression suggests a possible tumor suppressor role for E2F-1 in bladder cancer.



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