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Notch1 is an effector of Akt and hypoxia in melanoma development
Barbara Bedogni, … , Amato J. Giaccia, Marianne Broome Powell
Barbara Bedogni, … , Amato J. Giaccia, Marianne Broome Powell
Published October 16, 2008
Citation Information: J Clin Invest. 2008;118(11):3660-3670. https://doi.org/10.1172/JCI36157.
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Research Article Oncology

Notch1 is an effector of Akt and hypoxia in melanoma development

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Abstract

Melanomas are highly aggressive neoplasms resistant to most conventional therapies. These tumors result from the interaction of altered intracellular tumor suppressors and oncogenes with the microenvironment in which these changes occur. We previously demonstrated that physiologic skin hypoxia contributes to melanomagenesis in conjunction with Akt activation. Here we show that Notch1 signaling is elevated in human melanoma samples and cell lines and is required for Akt and hypoxia to transform melanocytes in vitro. Notch1 facilitated melanoma development in a xenograft model by maintaining cell proliferation and by protecting cells from stress-induced cell death. Hyperactivated PI3K/Akt signaling led to upregulation of Notch1 through NF-κB activity, while the low oxygen content normally found in skin increased mRNA and protein levels of Notch1 via stabilization of HIF-1α. Taken together, these findings demonstrate that Notch1 is a key effector of both Akt and hypoxia in melanoma development and identify the Notch signaling pathway as a potential therapeutic target in melanoma treatment.

Authors

Barbara Bedogni, James A. Warneke, Brian J. Nickoloff, Amato J. Giaccia, Marianne Broome Powell

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Figure 4

Notch1-NIC colocalizes with hypoxia, and its expression is regulated by HIF-1α.

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Notch1-NIC colocalizes with hypoxia, and its expression is regulated by ...
(A–C) Akt-dependent tumors were stained for Notch1-NIC (A) and with the hypoxia marker EF5 (B), showing colocalization (C). Scale bars: 50 μm. (D) qRT-PCR analysis of Akt-expressing melanocytes treated with normoxia (Nx; 21% O2) or hypoxia (Hx; 2% O2) and expressing either shGFP or shHIF-1α. (E) Western blot analysis for HIF-1α and Notch1-NIC in nuclear lysates. Tata-binding protein was used as loading control. (F and G) HES1 and HEY1 expression, as measured by qRT-PCR. As an internal control, 18S was used for normalization. Data in D, F, and G are mean ± SD. *P < 0.05 versus hypoxic control, Student’s t test.

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