Supplemental Figure 1 from PRAS40 Phosphorylation Correlates with Insulin-Like Growth Factor-1 Receptor-Induced Resistance to Epidermal Growth Factor Receptor Inhibition in Head and Neck Cancer Cells
posted on 2023-04-03, 17:11authored byMichael I. Dougherty, Christine E. Lehman, Adam Spencer, Rolando E. Mendez, Abel P. David, Linnea E. Taniguchi, Julie Wulfkuhle, Emanuel F. Petricoin, Daniel Gioeli, Mark J. Jameson
Supplemental Figure 1: The signaling impact of IGF1R activation in sensitive vs. resistant cell lines. Lysates from 6 HNSCC cell lines were assessed by reverse phase protein array (RPPA) to determine protein changes following treatment with desIGF1 (NT+IGF), each single EGFR-TKI (Erl = erlotinib, Gef = gefitinib, or Lap = lapatinib), or the combination of EGFR-TKI and desIGF1 (Erl+IGF, Gef+IGF, or Lap+IGF). Representative heat maps depict changes among the 157 epitopes in each of the 6 cell lines assessed by RPPA. Heat map representing changes upon treatment with (A) gefitinib, (B) erlotinib and (C) lapatinib. Asterisks represent significant changes with p<0.05 as compared to untreated.
Funding
NIH
NIDCR
UVA Cancer Center
UVA Department of Otolaryngology- Head and Neck Surgery Pilot Project
Ruth L. Kirschstein T32 Institutional Research Award
History
ARTICLE ABSTRACT
EGFR inhibitors have shown poor efficacy in head and neck squamous cell carcinoma (HNSCC) with demonstrated involvement of the insulin-like growth factor-1 receptor (IGF1R) in resistance to EGFR inhibition. IGF1R activates the PI3K–Akt pathway, which phosphorylates proline-rich Akt substrate of 40 kDa (PRAS40) to cease mTOR inhibition resulting in increased mTOR signaling. Proliferation assays separated six HNSCC cell lines into two groups: sensitive to EGFR inhibition or resistant; all sensitive cell lines demonstrated reduced sensitivity to EGFR inhibition upon IGF1R activation. Reverse phase protein microarray analysis and immunoblot identified a correlation between increased PRAS40 phosphorylation and IGFR-mediated resistance to EGFR inhibition. In sensitive cell lines, PRAS40 phosphorylation decreased 44%–80% with EGFR inhibition and was restored to 98%–196% of control by IGF1R activation, while phosphorylation was unaffected in resistant cell lines. Possible involvement of mTOR in this resistance mechanism was demonstrated through a similar pattern of p70S6K phosphorylation. However, addition of temsirolimus, an mTORC1 inhibitor, was insufficient to overcome IGF1R-mediated resistance and suggested an alternative mechanism. Forkhead box O3a (FOXO3a), which has been reported to complex with PRAS40 in the cytoplasm, demonstrated a 6-fold increase in nuclear to cytoplasmic ratio upon EGFR inhibition that was eliminated with concurrent IGF1R activation. Transcription of FOXO3a-regulated TRAIL and PTEN-induced putative kinase-1 (PINK1) was increased with EGFR inhibition in sensitive cell lines; this effect was diminished with IGF1R stimulation.
These data suggest PRAS40 may play an important role in IGF1R-based therapeutic resistance to EGFR inhibition, and this likely occurs via inhibition of FOXO3a-mediated proapoptotic gene transcription.