# Project 3: Metabolic imaging of TERT expression

> **NIH NIH P01** · UNIVERSITY OF CALIFORNIA, SAN FRANCISCO · 2023 · $12,281

## Abstract

ABSTRACT
Telomerase reverse transcriptase (TERT) enables telomere elongation that is essential for continuous cell
proliferation. TERT expression that is associated with activating mutations in the TERT promoter, is observed in
virtually all glioblastoma and oligodendroglioma cases. This makes TERT the most common genetic alteration
in brain tumors, and a novel therapeutic target. Noninvasive imaging of TERT expression could therefore help
in distinguishing between pseudo-progression and recurrent glioma, and provide a noninvasive biomarker for
assessment of treatment efficacy by TERT inhibitors. However, to date, no translational imaging approaches for
TERT expression have been reported. The goal of Project 3 is to address this critical need by developing
metabolic imaging biomarkers of TERT expression. Our approach is based on previous reports showing that
TERT expression is associated with control of cellular redox, and our preliminary data confirming this finding and
identifying additional metabolic alterations. Specifically, we have found that 1H magnetic resonance spectroscopy
(MRS)-detectable levels of glutathione and the 13C MRS-detectable metabolism of hyperpolarized
dehydroxyascorbate to vitamin C, are elevated in TERT-expressing cells. Additionally, hyperpolarized 13C MRS-
detectable fluxes of glucose and gluconolactone via the pentose phosphate pathway to 6-phosphogluconate are
elevated, as are the levels of aspartate and adenosine phosphates. We therefore hypothesize that advanced
MRS metabolic imaging could be used to distinguish glioma cells expressing TERT from normal brain
parenchyma and from tumor cells in which TERT expression is silenced by treatment. We will test this hypothesis
as follows. In Aim 1 we will identify 1H MRS and hyperpolarized 13C MRS metabolic imaging biomarkers that are
associated with TERT expression by investigating cell lines that differ only in their TERT status and determining
if levels of MRS-detectable metabolic biomarkers associated with redox, and other metabolic changes can
distinguish TERT-expressing from TERT non-expressing cells. In Aim 2 we will determine whether MRS-
detectable biomarkers of redox can be used to monitor TERT expression in vivo by using mouse models with
orthotopic TERT-expressing brain tumors, inhibiting TERT expression via genetic and/or pharmacological
approaches, and determining if this inhibition can be assessed using 1H and/or hyperpolarized 13C MRS
biomarkers of redox. If cell studies show that other metabolic pathways are modulated by TERT, these will also
be investigated in vivo. In Aim 3 we will investigate mechanisms linking TERT expression with metabolism by
assessing cellular processes known to be associated with TERT expression and determining if these processes
are mechanistically linked to changes in redox-associated metabolic pathways or other MRS-detectable
metabolic pathways altered by TERT. Our study is expected to lead to translatable MRS-detectable metaboli...

## Key facts

- **NIH application ID:** 10897352
- **Project number:** 3P01CA118816-15S1
- **Recipient organization:** UNIVERSITY OF CALIFORNIA, SAN FRANCISCO
- **Principal Investigator:** Sabrina Miriam Ronen
- **Activity code:** P01 (R01, R21, SBIR, etc.)
- **Funding institute:** NIH
- **Fiscal year:** 2023
- **Award amount:** $12,281
- **Award type:** 3
- **Project period:** 2007-07-01 → 2024-07-31

## Primary source

NIH RePORTER: https://reporter.nih.gov/project-details/10897352

## Citation

> US National Institutes of Health, RePORTER application 10897352, Project 3: Metabolic imaging of TERT expression (3P01CA118816-15S1). Retrieved via AI Analytics 2026-05-23 from https://api.ai-analytics.org/grant/nih/10897352. Licensed CC0.

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