Abstract 64P
Background
The prevalence of bladder cancer (BC) has been increasing worldwide. Particularly, patients carrying the Basal/Squamous BC (BSBC) have poor prognosis. Mammalian models such as cultured human BSBC cells and their xenografts have provided critical insights into its mechanisms, but effective therapeutics for BSBC is still lacking. Recently, the fruit fly Drosophila has made significant contributions to cancer research. Here, we employed Drosophila to generate the first fly model reproducing the BSBC genotypes and to discover novel therapeutic candidates for BSBC treatment.
Methods
BSBC often harbors mutations in genes ‘A’, ‘B’ and/or ‘C’. To model various alteration patterns in Drosophila, we employed the binary GAL4/UAS system, which targets expression of exogenous transgenes to a desired fly tissue. We prepared GAL4 driver strains expressing a transcription factor GAL4 specifically in the eye cells and wing cells (GMR-GAL4 and nub-GAL4, respectively, for validating transgene functions), or the Malpighian tubule which corresponds to human bladder (for modeling BSBC genotypes). We also generated UAS transgenic strains which carry mutated cDNA and/or shRNA sequences as transgenes downstream of the GAL4 target UAS sequence.
Results
Previous studies have reported that induction of wild-type A in fly eyes causes ‘rough eye’ phenotype by promoting apoptosis, which we confirmed using the eye-specific GMR-GAL4 driver. We found that additional expression of missense-mutated A or knockdown of A by shRNA rescued the phenotype as expected. Furthermore, we confirmed that overexpression of B using the same driver increased the fly eye size as previously reported. Using the wing-specific nub-GAL4 driver, we validated that knockdown of C by shRNA reduced the fly wing area, verifying its reported function to control tissue growth.
Conclusions
The eye and wing phenotypes induced by transgenes were consistent with their reported functions and our expectation, proving our strategy effective in validating functions of the transgenes and in modeling the BSBC genotypes in flies. We will next perform whole-body assays such as comprehensive genetic and drug screenings using these flies to demonstrate the mechanisms of BSBC pathogenesis and to develop novel BSBC treatments.
Clinical trial identification
Editorial acknowledgement
Legal entity responsible for the study
The authors.
Funding
Has not received any funding.
Disclosure
All authors have declared no conflicts of interest.
Resources from the same session
35P - SAT-122: A potential first-in-class, potent, small-molecule disruptor of RAD51-BRCA2, attenuates RAD51 foci formation and tumor progression in preclinical models
Presenter: Sukanya Patra
Session: Poster session 09
36P - Molecular assessment of clinical antitumour therapeutics utilising established pancreatic ductal adenocarcinoma patient-derived models
Presenter: Young-Ah Suh
Session: Poster session 09
37P - Nischarin can be a target for stromal normalisation in pancreatic ductal adenocarcinoma
Presenter: Jelena Grahovac
Session: Poster session 09
38P - Effects of antiemetics on zolbetuximab-induced gastric injury and emesis frequency in ferrets
Presenter: Jane Weng
Session: Poster session 09
39P - Casein kinase 2 modulates epithelial–mesenchymal transition through helicobacter pylori CagA-dependent pathway in gastric cancer cells
Presenter: SODAM LEE
Session: Poster session 09
40P - Bioinformatic evaluation of the transcriptomic and immunologic profile of prostate tumors with high expression of kallikrein-2
Presenter: Irene Moreno
Session: Poster session 09
42P - Developing a photodynamic therapy strategy targeted to endometrial cancer stem cells
Presenter: Beatriz Serambeque
Session: Poster session 09
43P - Looking for therapeutic targets on the proteome profile of endometrial cancer stem cells
Presenter: Mafalda Laranjo
Session: Poster session 09
44P - PAUF as a target for treatment of high PAUF-expressing ovarian cancer
Presenter: Junghyun Cho
Session: Poster session 09