Induced clustering of SHP2-depleted tumor cells in vascular islands restores sensitivity to MEK/ERK inhibition
Yuyi Wang, … , Michael Kruhlak, Giovanna Tosato
Yuyi Wang, … , Michael Kruhlak, Giovanna Tosato
Published March 25, 2025
Citation Information: J Clin Invest. 2025;135(10):e181609. https://doi.org/10.1172/JCI181609.
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Research Article Angiogenesis Oncology

Induced clustering of SHP2-depleted tumor cells in vascular islands restores sensitivity to MEK/ERK inhibition

Abstract

Allosteric inhibitors of the tyrosine phosphatase Src homology 2 domain–containing protein tyrosine phosphatase 2 (SHP2) hold therapeutic promise in cancers with overactive RAS/ERK signaling, but adaptive resistance to SHP2 inhibitors may limit benefits. Here, we utilized tumor cells that proliferate similarly with or without endogenous SHP2 to explore means to overcome this growth independence from SHP2. We found that SHP2 depletion profoundly altered the output of vascular regulators, cytokines, chemokines, and other factors from SHP2 growth-resistant cancer cells. Tumors derived from inoculation of SHP2-depleted, but SHP2 growth–independent, mouse melanoma and colon carcinoma cell lines displayed a typically subverted architecture, in which proliferative tumor cells surrounding a remodeled vessel formed “vascular islands”, each limited by surrounding hypoxic and dead tumor tissue, where inflammatory blood cells were limited. Although vascular islands generally reflect protected sanctuaries for tumor cells, we found that vascular island–resident, highly proliferative, SHP2-depleted tumor cells acquired an increased sensitivity to blockage of MEK/ERK signaling, resulting in reduced tumor growth. Our results show that the response to targeted therapies in resistant tumor cells was controlled by tumor cell–induced vascular changes and tumor architectural reorganization, providing a compelling approach to elicit tumor responses by exploiting tumor- and endothelium-dependent biochemical changes.

Authors

Yuyi Wang, Hidetaka Ohnuki, Andy D. Tran, Dunrui Wang, Taekyu Ha, Jing-Xin Feng, Minji Sim, Raymond Barnhill, Claire Lugassy, Michael R. Sargen, Emanuel Salazar-Cavazos, Michael Kruhlak, Giovanna Tosato

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Figure 3

SHP2 silencing regulates B16F10 cell clustering, ERK activation, cell proliferation, and cell death in 3D culture models.

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SHP2 silencing regulates B16F10 cell clustering, ERK activation, cell pr...
(A) Control p-LKO and SHP2-silenced B16F10 cells cultured (14 days) in ultra-low attachment plates were visualized by bright-field imaging (top and mid panels show representative images). Confocal cluster images are shown in the bottom panels (p-ERK, green; DAPI/nuclei, blue). Scale bars: 500 μm (middle panel) and 50 μm (bottom panel). (B) Quantification of cell cluster size; gray circles reflect individual clusters; colored dots reflect the mean cluster size/culture (n = 9); results are presented as mean (horizontal lines). **P < 0.01 by 2-way Student’s t test. (C) Immunoblot results of p-ERKT202/Y204 in lysates of B16F10 cells cultured for 7 days on ultra-low attachment plates. (D) Schematic diagram illustrating the experimental in vitro culturing system; left: a suspension of tumor cells, Matrigel, and DMEM was introduced into a tight-sealed chamber to evenly occupy the space; right: the chamber was transferred into a Petri dish containing DMEM with 10% FBS, which entered the chamber only through the 2 holes. (E) Fluorescence images of chamber holes and surrounding Matrigel 3, 30, and 60 minutes after addition of the Alexa Fluor 594–Fab fragment, showing the time-dependent fluorescence diffusion from the hole. Scale bar: 200 μm. (F) Representative bright-field images of control and SHP2-silenced B16F10 cells surrounding the chamber holes after 1- and 48-hour incubations (n = 3 experiments). The red arrows point to cell clustering around the hole. Scale bar: 500 μm. (G) Representative bright-field and fluorescence images of the indicated areas after staining with PI (48-hour incubation; n = 3 experiments). Scale bar: 500 μm (left panels) and 100 μm (middle and right panels). (H) Number of PI+/dead p-LKO and SHP2-silenced B16F10 cells as a function of distance from the corresponding hole (n = 3 experiments). ***P < 0.001, by 2-tailed Student’s t test. Results are presented as means± SEM. (I) Representative images of chambers containing B16F10 cells stained with Hoechst (nuclei/blue), Ki67 (green), and p-ERK (red) (48-hour incubation; n = 3 experiments). Scale bar: 500 μm. (J) Magnified images of the areas outlined in I (area 1: p-LKO B16F10 cells; areas 2 and 3: SHP2-silenced B16F10 cells) showing the cell clusters. Scale bar: 100 μm.