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Protein kinase LKB1 promotes RAB7-mediated neuropilin-1 degradation to inhibit angiogenesis
Imoh S. Okon, … , Guangpu Li, Ming-Hui Zou
Imoh S. Okon, … , Guangpu Li, Ming-Hui Zou
Published September 2, 2014
Citation Information: J Clin Invest. 2014;124(10):4590-4602. https://doi.org/10.1172/JCI75371.
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Research Article Vascular biology

Protein kinase LKB1 promotes RAB7-mediated neuropilin-1 degradation to inhibit angiogenesis

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Abstract

After internalization, transmembrane receptors (TMRs) are typically recycled back to the cell surface or targeted for degradation. Efficient TMR trafficking is critical for regulation of several processes, including signal transduction pathways, development, and disease. Here, we determined that trafficking of the angiogenic receptor neuropilin-1 (NRP-1) is abrogated by the liver kinase B1 (LKB1), a serine-threonine kinase of the calcium calmodulin family. We found that aberrant NRP-1 expression in tumor cells from patients with lung adenocarcinoma is associated with decreased levels of LKB1. In cultured lung cells, LKB1 accentuated formation of a complex between NRP-1 and RAB7 in late endosomes. LKB1 specifically bound GTP-bound RAB7, but not a dominant-negative GDP-bound form of RAB7, promoting rapid transfer and lysosome degradation of NRP-1. siRNA-mediated depletion of RAB7 disrupted the transfer of NRP-1 to the lysosome, resulting in recovery of the receptor as well as increased tumor growth and angiogenesis. Together, our findings indicate that LKB1 functions as a RAB7 effector and suppresses angiogenesis by promoting the cellular trafficking of NRP-1 from RAB7 vesicles to the lysosome for degradation. Furthermore, these data suggest that LKB1 and NRP-1 have potential as therapeutic targets for limiting tumorigenesis.

Authors

Imoh S. Okon, Kathleen A. Coughlan, Cheng Zhang, Cate Moriasi, Ye Ding, Ping Song, Wencheng Zhang, Guangpu Li, Ming-Hui Zou

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Figure 2

LKB1 attenuates NRP-1 expression in a VEGF-independent manner.

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LKB1 attenuates NRP-1 expression in a VEGF-independent manner.
(A and B)...
(A and B) Response of NRP-1 to hypoxia treatment (1% O2; 3 hours) or VEGF stimulation (25 ng/ml for 5 [+] or 30 [++] minutes) in LacZ- or LKB1-transfected A549 cells was assessed by immunoblot. Mean ± SD is shown (n = 3). (C) Under normal or hypoxia treatment (3 hours), NRP1 and LKB1 mRNA expression was assessed by RT-PCR in LacZ- or LKB1-transfected A549 cells. Mean ± SD is shown (n = 3). (D) Under the same experimental conditions, secreted VEGF levels were measured by ELISA; mean ± SD is shown (n = 4). (E and F) VEGF expression was silenced for 48 hours (siRNA) in LacZ- or LKB1-transfected A549 cells, and NRP-1 levels were assessed by Western blot. Mean ± SD is shown (n = 2). (G and H) Expression of VEGF and NRP-1 in various lung cancer cell lines was measured by immunoblot; mean ± SD is shown (n = 2). *P < 0.05, ***P < 0.001, ****P < 0.0001.

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