4.6 Article

Transcriptome profiling unveils GAP43 regulates ABC transporters and EIF2 signaling in colorectal cancer cells

BMC CANCER (2021)

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Journal

BMC CANCER
Volume 21, Issue 1, Pages -

Publisher

BMC
DOI: 10.1186/s12885-020-07728-x

Keywords

GAP43; Colorectal cancer; RNA-seq; DNA methylation; Transcriptome profiling

Categories

Oncology

Funding

  1. National Natural Science Foundation of China [31870891, 81502781, 81903046]
  2. China Scholarship Council [CSC 201806125051]
  3. China's Manned space pre-research project [17420205]
  4. China Postdoctoral Science Foundation [2020M673596XB]
  5. Hangzhou Social Development Self-declaration Project [20180533B63]
  6. Zhejiang Health Science and Technology Project [2018KY595]

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The study showed that the expression of GAP43 in colorectal cancer is influenced by DNA methylation, and overexpression of GAP43 significantly affects the expression of genes in multiple signaling pathways. The findings reveal the important role of GAP43 in the development of human colorectal cancer.
Background The growth- and plasticity-associated protein-43 (GAP43) is biasedly expressed in indigestive system and nervous system. Recent study has shown that GAP43 is responsible for the development of neuronal growth and axonal regeneration in normal nervous tissue, while serves as a specific biomarker of relapsed or refractory neuroblastoma. However, its expression pattern and function in digestive system cancer remains to be clarified. Methods In this study, we examined the GAP43 status with qRT-PCR and bisulfite genomic sequencing in colorectal cancer (CRC). We investigated the effect of overexpressed GAP43 in CRC cells with RNA-seq. The RNA-seq data was analyzed with DAVID and IPA. Results GAP43 was downregulated in CRC compared to the adjacent tissues. DNA methylase inhibitor 5-Aza-CdR treatment could significantly induce GAP43, indicated that the silencing of GAP43 gene in CRC is closely related to DNA methylation. Bisulfite genomic sequencing confirmed the promoter methylation of GAP43 in CRC. To explore the transcriptional alterations by overexpressed GAP43 in CRC, we performed RNA-seq and found that upregulated genes were significantly enriched in the signaling pathways of ABC transporters and ECM-receptor interaction, while downregulated genes were significantly enriched in Ribosome signaling pathway. Further Ingenuity Pathway Analysis (IPA) showed that EIF2 signaling pathway was significantly repressed by overexpression of GAP43. Conclusion Our findings provide a novel mechanistic insight of GAP43 in CRC. Transcriptome profiling of overexpressed GAP43 in CRC uncovered the functional roles of GAP43 in the development of human CRC.

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