# Endogenous barcoding to reveal neural stem cell lineage

> **NIH NIH R21** · STATE UNIVERSITY NEW YORK STONY BROOK · 2020 · $199,375

## Abstract

ABSTRACT
There are several models, partially overlapping and partially conflicting, of how stem cells of the adult brain
maintain their pool, divide, and give rise to neuronal and glial cells. Resolving those modes is important
because they imply different long-term consequences for the cognitive function, effects of stress and
disease, and response to therapies. Depending on the model, these consequences range from the
continuous support of the stem cell pool and their ability to generate neuronal and glial progeny to the
exhaustion of the stem cell pool and cessation of the ability to produce progeny. Partially, the debate about
the basic scheme of the stem cell life cycle is explained by inherent limitations of the approaches employed
to study this issue, which are now limited to nucleotide labeling of division events, clonal analysis, or live
observation. Here we propose endogenous barcoding as an orthogonal approach and describe
experiments to assess its feasibility for studying stem cells and generation of neurons and glia. This
approach is based on Polylox, a new Cre recombinase-driven DNA recombination substrate introduced
into the mouse germline. Cre induces random recombination of nine unique DNA elements, creating over
a million distinct codes and uniquely marking cells that have supported recombination of the Polylox allele
and all of their progeny. We propose to induce the recombination events in neural stem cells of the adult
hippocampus of compound lines carrying the Polylox allele and determine the overall composition of their
progeny. Furthermore, we propose to combine the Polylox endogenous barcoding approach with single
cell transcriptomics to determine the profiles of individual barcoded cells and their position on the trajectory
from stem cells to differentiated neurons or glia. Thus, in our first specific aim we will generate multiallelic
transgenic mouse lines carrying a combination of the Polylox transgene with transgenes for stem cell-
specific Cre recombinase and for lineage markers and will then assess and isolate hippocampal cells
carrying particulars barcode and deduce their relation. In our second specific aim, we will generate
additional multiallelic lines carrying Polylox barcode cassette, apply recombination-induced endogenous
barcoding, and then use single-cell transcription analysis combined with barcode analysis as a novel
approach for determining division, differentiation, and lineage of individual neural stem cells. Both
approaches will also help to resolve some of the unanswered or contradictory questions about the models
of stem cell maintenance and division and generation of glial and neuronal progeny. Our exploratory
project will introduce a new modality in the studies of neural stem cells, neurons, and glia and will serve
as a platform for further studies of dynamic regulation of the stem cell life cycle in the developing and adult
nervous system.

## Key facts

- **NIH application ID:** 9979726
- **Project number:** 5R21AG063004-02
- **Recipient organization:** STATE UNIVERSITY NEW YORK STONY BROOK
- **Principal Investigator:** GRIGORI N ENIKOLOPOV
- **Activity code:** R21 (R01, R21, SBIR, etc.)
- **Funding institute:** NIH
- **Fiscal year:** 2020
- **Award amount:** $199,375
- **Award type:** 5
- **Project period:** 2019-08-01 → 2022-04-30

## Primary source

NIH RePORTER: https://reporter.nih.gov/project-details/9979726

## Citation

> US National Institutes of Health, RePORTER application 9979726, Endogenous barcoding to reveal neural stem cell lineage (5R21AG063004-02). Retrieved via AI Analytics 2026-05-25 from https://api.ai-analytics.org/grant/nih/9979726. Licensed CC0.

---

*[NIH grants dataset](/datasets/nih-grants) · CC0 1.0*