Abstract 32P
Background
Secondary trastuzumab resistance seriously affects HER2-positive breast cancer treatment. However, we still lack knowledge about changes in tumor cells and their interaction with tumor microenvironment (TME) components during resistance formation. This study aimed to uncover metabolism pathway changes during trastuzumab resistance formation and potential epigenetic variations that are relevant to these processes.
Methods
Induced secondary trastuzumab-resistant SKBR3_HR cell line together with the original trastuzumab-sensitive SKBR3 cell line were applied in this study. Total RNA was collected for transcriptome analysis. Anti-H3K4me3, K27me3 and K27ac antibodies were chosen for CUT&Tag sequencing library preparation. Total genome DNA was prepared for Micro-C sequencing library preparation. Activity score of metabolism pathway was calculated as relative gene expression value averaged over all genes in this pathway in certain cell types. Extracellular prostaglandin E2 (PGE2) was measured by ELISA.
Results
SKBR3_HR cells showed higher trastuzumab tolerance than SKBR3 cells. Upregulation of arachidonic acid metabolism, which was characterized by two overexpressed genes, PTGS1 and PTGES, was observed in SKBR3_HR cells, resulting in PGE2 accumulation in culture medium. Variations of 1519 H3K27me3 peaks and 256 H3K4me3 peaks at promoters were observed during resistance formation. Little H3K27me3 but considerable raised H3K4me3 levels at PTGS1 and PTGES gene promoters may stimulate their transcription.692 altered active enhancers were measured during resistance formation. Meanwhile, 2741 and 7007 DNA loops were lost and gained. New DNA loops formation between PTGS1 gene promoter and enhancers nearby, indicating a positive synergy regulatory on PTGS1 gene expression together with promoter modifications.
Conclusions
During trastuzumab resistance formation, promoter H3K4me3, active enhancers and DNA loops together regulate PTGS1 and PTGES expression, activate arachidonic acid metabolism, and eventually stimulate PGE2 accumulation.
Clinical trial identification
Editorial acknowledgement
Legal entity responsible for the study
The authors.
Funding
National Natural Science Foundation of China (81972484), National Natural Science Foundation of China (82203488).
Disclosure
All authors have declared no conflicts of interest.
Resources from the same session
89P - Cold atmospheric plasma-activated fluids as a potential new intravesical agent for the treatment of bladder cancer
Presenter: Maria Filomena Botelho
Session: Poster session 09
90P - Discovery of CMPD1 as a tumor-specific cytotoxic microtubule inhibitor
Presenter: Mamoru Takada
Session: Poster session 09
91P - Erythroid precursor-differentiated myeloid cells promote pulmonary metastasis in hepatocellular carcinoma
Presenter: Wei-hang Zhu
Session: Poster session 09
92P - Discovery of novel AXL and MER inhibitors as potential anticancer and immune modulator drugs
Presenter: Hsing-Pang Hsieh
Session: Poster session 09
93P - Transcriptome changes of immune cells across chemotherapy of triple-negative breast cancer
Presenter: Tatiana Gerashchenko
Session: Poster session 09
509P - Spatial analysis of tumor-associated macrophages within the tumor microenvironment of primary tumors and matched brain metastases
Presenter: Markus Kleinberger
Session: Poster session 09
510P - CD47 regulates cellular and metabolic plasticity in glioblastoma
Presenter: Ruhi Polara
Session: Poster session 09
511P - Immunodisruptive conditions and glioma diagnosis: 24-year retrospective study of an under-recognized scenario
Presenter: Santiago Cabezas-Camarero
Session: Poster session 09
512P - Heterozygous germline Fanconi anemia-related gene mutations increase susceptibility to central nervous system germ cell tumors
Presenter: Guangyu Wang
Session: Poster session 09
513P - Cyclin pathway in oligodendrogliomas IDH mut and 1p/19q codeleted
Presenter: Maria Angeles Vaz Salgado
Session: Poster session 09