Targeting prion-like protein doppel selectively suppresses tumor angiogenesis
Taslim A. Al-Hilal, … , In-San Kim, Youngro Byun
Taslim A. Al-Hilal, … , In-San Kim, Youngro Byun
Published March 7, 2016
Citation Information: J Clin Invest. 2016;126(4):1251-1266. https://doi.org/10.1172/JCI83427.
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Research Article Oncology

Targeting prion-like protein doppel selectively suppresses tumor angiogenesis

Abstract

Controlled and site-specific regulation of growth factor signaling remains a major challenge for current antiangiogenic therapies, as these antiangiogenic agents target normal vasculature as well tumor vasculature. In this article, we identified the prion-like protein doppel as a potential therapeutic target for tumor angiogenesis. We investigated the interactions between doppel and VEGFR2 and evaluated whether blocking the doppel/VEGFR2 axis suppresses the process of angiogenesis. We discovered that tumor endothelial cells (TECs), but not normal ECs, express doppel; tumors from patients and mouse xenografts expressed doppel in their vasculatures. Induced doppel overexpression in ECs enhanced vascularization, whereas doppel constitutively colocalized and complexed with VEGFR2 in TECs. Doppel inhibition depleted VEGFR2 from the cell membrane, subsequently inducing the internalization and degradation of VEGFR2 and thereby attenuating VEGFR2 signaling. We also synthesized an orally active glycosaminoglycan (LHbisD4) that specifically binds with doppel. We determined that LHbisD4 concentrates over the tumor site and that genetic loss of doppel in TECs decreases LHbisD4 binding and targeting both in vitro and in vivo. Moreover, LHbisD4 eliminated VEGFR2 from the cell membrane, prevented VEGF binding in TECs, and suppressed tumor growth. Together, our results demonstrate that blocking doppel can control VEGF signaling in TECs and selectively inhibit tumor angiogenesis.

Authors

Taslim A. Al-Hilal, Seung Woo Chung, Jeong Uk Choi, Farzana Alam, Jooho Park, Seong Who Kim, Sang Yoon Kim, Fakhrul Ahsan, In-San Kim, Youngro Byun

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Figure 4

Doppel interacts with VEGFR2 on TECs.

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Doppel interacts with VEGFR2 on TECs. Representative images of the PLA o...
Representative images of the PLA of doppel (A), VEGFR2 (B), and doppel-VEGFR2 interactions (C) identified on TECs. PLA signals are shown with red dots, cytoskeletal staining (FITC-phalloidin) is shown in green, and nuclear staining (DAPI) is shown in blue. Scale bars: 5 μm (AC). (D) Quantification of doppel, VEGFR2, and doppel-VEGFR2 heterodimer PLA signals in TECs. Co-IP followed by immunoblotting (IB) of VEGFR2 and doppel in Hu.dpl cells and TECs (E), immunoblot of VEGFR1 and doppel (F), and immunoblot of VEGFR3 and doppel (G) in Hu.dpl cells. Input: whole-cell lysates. Single asterisk indicates a light or heavy chain. Each experiment was repeated 3–5 times.