APA
Silva, Javier & García, José M. & Peña, Cristina & García, Vanesa & Domínguez, Gemma & Suarez, Dolores & Camacho, Francisca I. & Espinosa, Ruth & Provencio, Mariano & España, Pilar & Bonilla, Félix (2006-12 ) .Implication of Polycomb Members Bmi-1, Mel-18, and Hpc-2 in the Regulation of p16INK4a, p14ARF, h-TERT, and c-Myc Expression in Primary Breast Carcinomas.
ISO 690
Silva, Javier & García, José M. & Peña, Cristina & García, Vanesa & Domínguez, Gemma & Suarez, Dolores & Camacho, Francisca I. & Espinosa, Ruth & Provencio, Mariano & España, Pilar & Bonilla, Félix. 2006-12 .Implication of Polycomb Members Bmi-1, Mel-18, and Hpc-2 in the Regulation of p16INK4a, p14ARF, h-TERT, and c-Myc Expression in Primary Breast Carcinomas.
https://hdl.handle.net/20.500.12080/39573
Abstract:
Purpose: Deregulation of mammalian Polycomb group (PcG) members may contribute to
human carcinogenesis. p16INK4a and p14ARF tumor suppressors, human telomerase reverse
transcriptase (h-TERT), and oncoprotein c-Myc have been implicated in the regulation of the
cell cycle and proliferation mediated by PcG proteins, mainly Bmi-1, in mice and in cell culture
experiments. Here, we examine whether these in vitro findings can be extrapolated to the in vivo
situation.
Experimental Design:We measure the expression of PcG members Bmi-1, Mel-18, and Hpc-2
and their potential targets by reverse transcription-PCR, immunostaining, andWestern blotting in
a series of 134 breast carcinomas and correlate the data with several clinical-pathologic variables
of the tumors.
Results: Expression of PcG genes was variably detected, but overexpression of Bmi-1 was the
most frequent PcG alteration observed. In addition, statistical direct correlation in expression level
of the three PcG members was detected. A correlation between c-Myc and Bmi-1 expression
levels was observed; however, there was no correlation between expression of Bmi-1 and
p16INK4a, p14ARF, or h-TERT. However, expression of the other PcG members Mel-18
and Hpc-2 correlated withthe cell cycle regulators. Moreover, PcG mRNA ^ altered expression
correlated significantly withcertain clinical-pathologic variables associated withpoor prognosis.
Conclusions: Our data suggest that the oncogenic role of Bmi-1 in human primary breast
carcinomas is not determined by its capacity to inhibit INK4a/ARF proteins or to induce telomer ase activity