# Mechanism of MRNA Localization and Localized Translation in Neurons

> **NIH NIH R01** · ALBERT EINSTEIN COLLEGE OF MEDICINE · 2020 · $14,887

## Abstract

ABSTRACT
The neuron is the basic cellular unit of the brain. For neurons to work properly, they must
be plastic and constantly capable of changing in response to stimuli, forming and
stabilizing new connections. This process requires proteins to be added to the new
synaptic contact, and this in turn results from the targeting of mRNA to these sites of
activity. This is the mechanistic basis of learning and memory since the synapse is
stabilized by the production of proteins in response to stimulation that are important for its
structural integrity. How this mRNA is regulated in neurons to make the right protein at the
right place and time has been the subject of our investigations over the years of this
funding. This proposal exploits the tools we generated during the last funding period to
address how mRNA is regulated in dendrites. One of these tools is a mouse where we
have tagged the β-actin gene with a fluorescent marker to follow individual mRNAs in live
neurons. We have found that the mRNA is encased in an inert form as it travels around in
the dendrite. When it comes into the proximity of a stimulated dendritic spine, it unfurls its
RNA payload and makes a burst of protein, but then returns to a dormant state after 16
minutes. The mRNA sits at the place where it was last stimulated for hours, awaiting the
next signal, wherein it will initiate another round of proteins. In this way, the synaptic
contact is built up, consistent with a learning and memory paradigm that relies on repetitive
stimulation. If there are no further activating signals, the mRNA continues its search,
moving in short processive movements broken by periods of diffusion. The current
proposal follows up on the discovery of the particular protein that binds to the mRNA
zipcode responsible for directing it to its site (zipcode binding protein, ZBP1), anchors the
mRNA at the site of stimulation. The model we have constructed suggests that the mRNA
translates upon a further stimulation and we intend to focus on this point of regulation by
describing the kinetics of these events and the proteins that play a role in these events.
Up to this point we have investigated β-actin mRNA because actin is the major structural
protein in cells, and in the synapse as well. However the regulatory mechanism leading to
a complex structure such as a synapse must orchestrate the expression of many proteins.
For this reason, we have constructed another mouse with an mRNA important for learning,
Arc, that has been tagged with a different fluorescent marker. In this proposal, we will
characterize the mRNAs for β-actin and Arc in mice together where both mRNAs are
individually detectable by different colored fluorochromes. We propose eventually a third
hybrid-color mRNA for CaMKIIα, an essential protein in synapses. Our goal is to uncover
the mechanisms that govern the regulation of different mRNAs in response to stimulatory
activations of the neuron: the timing of their synthesis, localization ...

## Key facts

- **NIH application ID:** 10110297
- **Project number:** 3R01NS083085-27S1
- **Recipient organization:** ALBERT EINSTEIN COLLEGE OF MEDICINE
- **Principal Investigator:** Carolina Ines Eliscovich
- **Activity code:** R01 (R01, R21, SBIR, etc.)
- **Funding institute:** NIH
- **Fiscal year:** 2020
- **Award amount:** $14,887
- **Award type:** 3
- **Project period:** 1992-03-03 → 2022-08-31

## Primary source

NIH RePORTER: https://reporter.nih.gov/project-details/10110297

## Citation

> US National Institutes of Health, RePORTER application 10110297, Mechanism of MRNA Localization and Localized Translation in Neurons (3R01NS083085-27S1). Retrieved via AI Analytics 2026-05-24 from https://api.ai-analytics.org/grant/nih/10110297. Licensed CC0.

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