Warning, /office/kbibtex-testset/isi/estrogen.isi is written in an unsupported language. File is not indexed.

 FN ISI Export Format
 VR 1.0
 PT J
 AU Eertmans, F
    Dhooge, W
    De Wever, O
    Bracke, M
    Comhaire, F
    Kaufman, JM
 AF Eertmans, Frank
    Dhooge, Willem
    De Wever, Olivier
    Bracke, Marc
    Comhaire, Frank
    Kaufman, Jean-Marc
 TI Estrogen receptor alpha (ER alpha) and insulin-like growth factor I
    receptor (IGF-IR) cross-talk in the gonadotropic alpha T3-1 cell line
 SO JOURNAL OF CELLULAR PHYSIOLOGY
 LA English
 DT Article
 ID ACTIVATED PROTEIN-KINASE; BREAST-CANCER; PHOSPHORYLATION; HORMONE;
    ESTRADIOL; PATHWAY; VITRO; MEMBRANE; NEURONS; BRAIN
 AB In reproductive tissues such as the breast and the uterus, cell
    proliferation and differentiation is strongly regulated by complex
    interactions between estrogen receptor a (ER alpha) and growth factor
    receptors. In the present study, we investigated the potential
    occurrence of such cross-talk in the murine, gonadotropic alpha T3-I
    cell line, which expresses ER alpha and the IGF-I receptor (IGF-IR).
    Under estrogen-free conditions, basal cell proliferation and
    ER-mediated gene transcription was strongly inhibited by the selective
    estrogen receptor modulator (SERM) 4-hydroxy-tamoxifen (4-OH-Tam) and
    by the pure anti-estrogen ICI 182,780 (ICI). These effects can be
    reversed by either 17-beta-estradiol (E-2) or insulin-like growth
    factor I (IGF-1), both exerting modest mitogenic effects in the alpha
    T3-1 cell line. Furthermore, IGF-I enhanced both basal and E-2-induced
    ER-driven gene transcription. This may be explained, at least in part,
    by enhanced phosphorylation of ER alpha atserine 118, a prerequisite
    for the transactivation capacity of the receptor. Finally, the
    IGF-l-induced response on cell growth and ER-mediated transactivation
    can be inhibited with either ICI or 4-CH-Tam. In conclusion, our data
    indicate IGF-IR and ER interactions in the aT3-1 cell line, an in vitro
    model for the pituitary gonadotrophs, hereby suggesting a role of IGF-I
    in the regulation of gonaclotropin synthesis and secretion.
 C1 State Univ Ghent Hosp, Dept Endocrinol, B-9000 Ghent, Belgium.
    State Univ Ghent Hosp, Expt Cancerol Lab, B-9000 Ghent, Belgium.
 RP Eertmans, F, State Univ Ghent Hosp, Dept Endocrinol, 6K 121E,De
    Pintelaan 185, B-9000 Ghent, Belgium.
 EM Frank.Eertmans@ugent.be
 NR 50
 TC 1
 PU WILEY-LISS
 PI HOBOKEN
 PA DIV JOHN WILEY & SONS INC, 111 RIVER ST, HOBOKEN, NJ 07030 USA
 SN 0021-9541
 J9 J CELL PHYSIOL
 JI J. Cell. Physiol.
 PD SEP
 PY 2007
 VL 212
 IS 3
 BP 583
 EP 590
 PG 8
 SC Cell Biology; Physiology
 GA 200NQ
 UT ISI:000248770500005
 ER
 
 EF