# A clone's genomic stability as biomarker of its DNA-damage resilience

> **NIH NIH R00** · H. LEE MOFFITT CANCER CTR & RES INST · 2020 · $248,930

## Abstract

A main problem in the treatment of advanced cancers, including gastric cancers and glioblastoma, is the incertitude at which
we predict how individual patients will respond to DNA-damaging agents, especially on the long run. Knowing the mechanism
behind a patient's response, or the lack thereof, will help us depart from the oversimplified “more-is-better” and “one-size-
fits-all” principles according to which DNA-damaging agents are administered. This will improve clinical outcome by allowing
us to pinpoint those who would respond better and longer to lower doses of DNA-damaging agents, than to higher doses.
Under the assumption that the success of DNA-damaging therapy increases with the proliferation rate of a relatively
homogeneous tumor population, there was little reason to assume anything other than monotonic dose-response relations. But
with the recent paradigm shift that most cancers are in fact DNA mosaic products of ongoing evolution, comes the urgency to
reconsider these fundamental principles behind DNA-damaging therapy administration. As the developers of one of the first
DNA deconvolution methods and with access to technologies to profile the transcriptomes of up to 10,000 cells
simultaneously, we are equipped to embark on first personalized dose-finding strategies for DNA-damaging therapies. We will
test the potential of the very long-term legacy that DNA-damage entails on a cell – genomic instability – as new biomarker of DNA-
damage response. Our preliminary studies showed that, for most cancer types, DNA-damaging agents change a clone's genomic
instability and that clones succumb to a limit in the amount of genomic instability they can tolerate. In particular, our results
showed that patients with intermediate genomic instability have a very poor outcome and that this relation is only evident
among treatment-naïve patients, but not among patients treated with DNA-damaging agents. Further they show that we can
measure genomic instability per clone and that clones with extreme genomic instability typically don't grow large. Our
hypothesis that genomic instability, rather than proliferation rate, determines how sensitive a tumor is to DNA damaging
agents on the long-term, is founded on two unexpected findings: (i) Patients with extremely high genomic instability per tumor
clone have an exceptionally good outcome. Aim 1 will integrate exome- and single cell RNA-seq data to characterize clones
and to measure how much genomic instability they can tolerate. (ii) Low genomic instability is associated with reduced benefit
from DNA-damaging agents. Aim 2 will use comet assays and treatment history to quantify DNA damage per clone, relating it
to the clones' ability to tolerate DNA damage and to changes in the genomic instability of therapy-surviving clones. This
would be the first study to test the potential of genomic instability as biomarker of DNA-damage sensitivity. We will also use
the clone specific transcriptomes and genomes from th...

## Key facts

- **NIH application ID:** 10015210
- **Project number:** 5R00CA215256-04
- **Recipient organization:** H. LEE MOFFITT CANCER CTR & RES INST
- **Principal Investigator:** Noemi Andor
- **Activity code:** R00 (R01, R21, SBIR, etc.)
- **Funding institute:** NIH
- **Fiscal year:** 2020
- **Award amount:** $248,930
- **Award type:** 5
- **Project period:** 2017-03-01 → 2022-07-31

## Primary source

NIH RePORTER: https://reporter.nih.gov/project-details/10015210

## Citation

> US National Institutes of Health, RePORTER application 10015210, A clone's genomic stability as biomarker of its DNA-damage resilience (5R00CA215256-04). Retrieved via AI Analytics 2026-05-23 from https://api.ai-analytics.org/grant/nih/10015210. Licensed CC0.

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