4.5 Article

PKP1 and MYC create a feedforward loop linking transcription and translation in squamous cell lung cancer

CELLULAR ONCOLOGY (2022)

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Journal

CELLULAR ONCOLOGY
Volume 45, Issue 2, Pages 323-332

Publisher

SPRINGER
DOI: 10.1007/s13402-022-00660-1

Keywords

Non-small cell lung cancer; Squamous cell lung cancer; Plakophilin; MYC; Biomarker; Feedforward loop

Categories

Oncology Cell Biology Pathology

Funding

  1. Ministry of Economy of Spain [SAF2015-67919-R]
  2. Junta de Andalucia [Pl-0245-2017, PIGE-0440-2019, PI-0135-2020, PIGE-0213-2020,, P20-00688]
  3. Plan propio de la Universidad de Granada, an International Association for the Study of Lung Cancer (IASLC) Young Investigator Award 2017 [PPJIA2019-06, B-CTS-126-UGR18]
  4. Spanish Association for Cancer Research [LAB-AECC-2018]
  5. Fundacion Benefica Anticancer Santa Candida y San Francisco Javier predoctoral fellowship
  6. Ministry of Health and Social Welfare of Junta de Andalucia [RH-0051-2020]
  7. European Commission [837897]
  8. La Caixa Foundation [LCF/BQ/DE15/10360019]
  9. Spanish Ministry of Education, Culture and Sports FPU fellowship [FPU17/00067, FPU17/01258, FPU19/05124]
  10. Marie Curie Actions (MSCA) [837897] Funding Source: Marie Curie Actions (MSCA)

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The study reveals a significant functional relationship between PKP1 and MYC in squamous cell lung cancer, where PKP1 enhances oncogenic activity by promoting MYC translation, while MYC can also regulate PKP1 transcription. This suggests that PKP1 may serve as a potential therapeutic target for squamous cell lung cancer.
Purpose Plakophilin 1 (PKP1) is well-known as an important component of the desmosome, a cell structure specialized in spot-like cell-to-cell adhesion. Although desmosomes have generally been associated with tumor suppressor functions, we recently found that PKP1 is recurrently overexpressed in squamous cell lung cancer (SqCLC) to exert an oncogenic role by enhancing the translation of MYC (c-Myc), a major oncogene. In this study, we aim to further characterize the functional relationship between PKP1 and MYC. Methods To determine the functional relationship between PKP1 and MYC, we performed correlation analyses between PKP1 and MYC mRNA expression levels, gain/loss of function models, chromatin immunoprecipitation (ChIP) and promoter mutagenesis followed by luciferase assays. Results We found a significant correlation between the mRNA levels of MYC and PKP1 in SqCLC primary tumor samples. In addition, we found that MYC is a direct transcription factor of PKP1 and binds to specific sequences within its promoter. In agreement with this, we found that MYC knockdown reduced PKP1 protein expression in different SqCLC models, which may explain the PKP1-MYC correlation that we found. Conversely, we found that PKP1 knockdown reduced MYC protein expression, while PKP1 overexpression enhanced MYC expression in these models. Conclusions Based on these results, we propose a feedforward functional relationship in which PKP1 enhances MYC translation in conjunction with the translation initiation complex by binding to the 5'-UTR of MYC mRNA, whereas MYC promotes PKP1 transcription by binding to its promoter. These results suggest that PKP1 may serve as a therapeutic target for SqCLC.

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