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Chemokine receptor CXCR7 activates Aurora Kinase A and promotes neuroendocrine prostate cancer growth
Galina Gritsina, … , Maha Hussain, Jindan Yu
Galina Gritsina, … , Maha Hussain, Jindan Yu
Published June 22, 2023
Citation Information: J Clin Invest. 2023;133(15):e166248. https://doi.org/10.1172/JCI166248.
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Research Article Oncology Article has an altmetric score of 3

Chemokine receptor CXCR7 activates Aurora Kinase A and promotes neuroendocrine prostate cancer growth

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Abstract

CXCR7 is an atypical chemokine receptor that recruits β-arrestin (ARRB2) and internalizes into clathrin-coated intracellular vesicles where the complex acts as a scaffold for cytoplasmic kinase assembly and signal transduction. Here, we report that CXCR7 was elevated in the majority of prostate cancer (PCa) cases with neuroendocrine features (NEPC). CXCR7 markedly induced mitotic spindle and cell cycle gene expression. Mechanistically, we identified Aurora Kinase A (AURKA), a key regulator of mitosis, as a novel target that was bound and activated by the CXCR7-ARRB2 complex. CXCR7 interacted with proteins associated with microtubules and golgi, and, as such, the CXCR7-ARRB2-containing vesicles trafficked along the microtubules to the pericentrosomal golgi apparatus, where the complex interacted with AURKA. Accordingly, CXCR7 promoted PCa cell proliferation and tumor growth, which was mitigated by AURKA inhibition. In summary, our study reveals a critical role of CXCR7-ARRB2 in interacting and activating AURKA, which can be targeted by AURKA inhibitors to benefit a subset of patients with NEPC.

Authors

Galina Gritsina, Ka-wing Fong, Xiaodong Lu, Zhuoyuan Lin, Wanqing Xie, Shivani Agarwal, Dong Lin, Gary E. Schiltz, Himisha Beltran, Eva Corey, Colm Morrissey, Yuzhuo Wang, Jonathan C. Zhao, Maha Hussain, Jindan Yu

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Figure 1

CXCR7 is upregulated in neuroendocrine PCa.

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CXCR7 is upregulated in neuroendocrine PCa.
(A) The box plots show that ...
(A) The box plots show that CXCR7 is significantly upregulated in NEPC tumors. CXCR7 (ACKR3) expression (mRNA) was queried from the data sets indicated. (B) Scatter plots show a significant correlation between CXCR7 and ENO2 in the PCa patient data sets. The dark grey area indicates the 95% CI, X- and Y-axes show normalized expression. Statistical analysis is based on linear regression. (C) Representative IHC staining of CXCR7, AR, and SYP in selected CRPC or NEPC LuCaP PDX tumors. Scale bar: 60 μm. (D) Tissue microarray constructed with clinical tumor samples was subjected to IHC staining with anti-CXCR7 (RnD, 11G8), anti-AR (AR-N Biogenex, MU256-UC), and anti-SYP (Santa Cruz, SC-17750) antibodies. Representative images of 3 independent CRPC or NEPC tumors are shown. Scale bars: 60 μm (inset); 200 μm (larger image). (E) Correlation between CXCR7 and SYP IHC staining scores in TMAs. Every dot represents the average intensity score of 3 cores for each tumor. A total of 31 tumors were analyzed. P < 0.001 by linear regression. (F) Quantification of CXCR7 IHC intensity scores in primary PCa, CRPC, and NEPC samples. The Y-axis shows the percentage of tumors with none (0; gray), weak (1; light pink), moderate (2; dark pink), and intense (3; red) IHC scores for each category.

Copyright © 2025 American Society for Clinical Investigation
ISSN: 0021-9738 (print), 1558-8238 (online)

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