Oops, you're using an old version of your browser so some of the features on this page may not be displaying properly.

MINIMAL Requirements: Google Chrome 24+Mozilla Firefox 20+Internet Explorer 11Opera 15–18Apple Safari 7SeaMonkey 2.15-2.23

Become a member
  1. OncologyPRO
  2. Meeting Resources
  3. Molecular Analysis for Precision Oncology Congress 2022

Poster display session

76P - Modulation of mutant p53 activity using indazole derivatives

Date

15 Oct 2022

Session

Poster display session

Presenters

Damir Davletshin

Citation

Annals of Oncology (2022) 33 (suppl_8): S1383-S1430. 10.1016/annonc/annonc1095

Authors

D. Davletshin1, E. Khusainova1, R. Khadiullina1, R. Mirgayazova1, M. Baud2, E. Bulatov1

Author affiliations

  • 1 Kazan Federal University, Kazan/RU
  • 2 University of Southampton, Southampton/GB

Resources

Login to get immediate access to this content.

If you do not have an ESMO account, please create one for free.

Login

Abstract 76P

Background

Oncogenic mutation p53 Y220C is the ninth most common mutation of p53 protein. The Y220C mutation creates an expanded surface pocket in the DNA-binding domain, rapidly unfolds and denatures under physiological conditions, which effectively cancels p53 signaling and leads to the development of a tumor. In this work the novel indazole derived compounds were tested. It was found that these molecules bind to the mutated p53 protein and stabilize its structure in vitro.

Methods

In this work the human breast carcinoma (MCF7 p53 wt, MCF7 p53 Y220C, MCF7 p53 -/-) and the human hepatocarcinoma (HUH7 p53 Y220C) cell lines were used. Cell viability was evaluated using colorimetric MTS test. The cells were treated with compounds at the concentration range of 0-200 μM. The obtained data were processed in GraphPad Prism. The expression of p53 target genes upon treatment with the compounds was also quantified using real-time quantitative PCR (RT-qPCR).

Results

Viability of cells incubated with the compounds were determined for cell lines with different p53 status. IC50 values for cells with wild-type p53 status (MCF7 p53 wt) and cells with TP53 knockout (MCF7 p53 -/-) could not be detected in the selected concentration range while in cells with mutated p53 (HUH7 p53 Y220C and MCF7 p53 Y220C) IC50 values were determined in the range of 32-55 μM. Expression of PUMA (BBC3) was found to be upregulated in HUH7 p53 Y220C and MCF7 p53 Y220C cells upon treatment with the compounds.

Conclusions

The results demonstrated that the compounds exert targeted effect on cells carrying p53 Y220C mutation. We established that the compounds selectively reduced the viability of p53 Y220C cell lines and upregulated transcription of p53 target genes associated with apoptosis in p53 Y220C-dependent manner. The work was funded by grant from the Russian Science Foundation 22-24-20034 and supported by the Kazan Federal University Strategic Academic Leadership Program (PRIORITY-2030).

Legal entity responsible for the study

Kazan Federal University.

Funding

The work was funded by grant from the Russian Science Foundation 22-24-20034 and supported by the Kazan Federal University Strategic Academic Leadership Program (PRIORITY-2030).

Disclosure

All authors have declared no conflicts of interest.

This site uses cookies. Some of these cookies are essential, while others help us improve your experience by providing insights into how the site is being used.

For more detailed information on the cookies we use, please check our Privacy Policy.

Customise settings

  • Necessary cookies enable core functionality. The website cannot function properly without these cookies, and you can only disable them by changing your browser preferences.