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TTF-1/Nkx2.1 functional connection with mutated EGFR relies on LRIG1 and ?-catenin pathways in lung cancer cells

Articolo
Data di Pubblicazione:
2018
Abstract:
In non-small lung cancer, the expression of the transcription factor TTF-1/Nkx2.1 correlates with the presence of EGFR mutations, therefore TTF-1/Nkx2.1 expression is used to optimize an EGFR testing strategy and to guide clinical treatment. We investigate the molecular mechanisms underlying the functional connection between EGFR and TTF-1/Nkx2.1 gene expression in lung adenocarcinoma. Using the H1975 cell line as a non-small cell lung cancer model system and short hairpin RNA, we have selected clones with TTF-1/Nkx2.1 silenced expression. We have found that Leucine-rich immunoglobulin repeats-1 (LRIG1) gene is a direct target of TTF-1/Nkx2.1 and the transcription factor binding to the LRIG1 genomic sequence inhibits its gene expression. In TTF-1/Nkx2.1 depleted clones, we have found high levels of LRIG1 and decreased presence of EGFR protein. Furthermore, in TTF-1/Nkx2.1 depleted clones we detected a reduced ?-catenin level and we provide experimental evidence indicating that TTF-1/Nkx2.1 gene expression is regulated by ?-catenin. Published studies indicate that LRIG1 triggers EGFR degradation and that mutated EGFR induces ?-catenin activity. Hence, with the present study we show that mutated EGFR, enhancing ?-catenin, stimulates TTF-1/Nkx2.1 gene expression and, at the same time, TTF-1/Nkx2.1, down-regulating LRIG1, sustains EGFR pathway. Therefore, LRIG1 and ?-catenin mediate the functional connection between TTF-1/Nkx2.1 and mutated EGFR.
Tipologia CRIS:
01.01 Articolo in rivista
Keywords:
EGFR; LRIG1; Non-small cell lung cancer; TTF-1/Nkx2.1; ?-catenin
Elenco autori:
Zamboni, Michela; Civitareale, Donato
Autori di Ateneo:
ZAMBONI MICHELA
Link alla scheda completa:
https://iris.cnr.it/handle/20.500.14243/351004
Pubblicato in:
BIOCHEMICAL AND BIOPHYSICAL RESEARCH COMMUNICATIONS (PRINT)
Journal
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http://www.scopus.com/record/display.url?eid=2-s2.0-85054461484&origin=inward
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