# Functional interplay between MAP and PTM patterns in the human neuron

> **NIH NIH FI2** · U.S. NATIONAL INST/NEURO/DS/STROKE · 2024 · —

## Abstract

Project Summary/Abstract
 Neurons form two distinct processes during polarization, axons and dendrites, each with a unique and
tightly packed microtubule array of post-translationally modified microtubules coated in microtubule associated
proteins (MAPs), which control the activity of kinesin and dynein motors responsible for long-range intracellular
transport. MAPs are upregulated during polarization and are spatiotemporally regulated. MAPs play an integral
role in establishing the process-specific microtubule arrays by controlling microtubule organization, microtubule
dynamics, and the binding of molecular motors. In vitro studies demonstrated that MAPs at saturating
concentrations form inhibitory patches or “islands” along microtubules, deterring kinesin and dynein binding,
However, neurons still achieve long-range transport, suggesting regulation of the deposition of MAPs along
microtubules. Two mechanisms through which MAP regulation can be achieved are: (1) competitive binding with
other MAPs or (2) modifications to the underlying microtubule substrate. Post-translational modifications (PTMs)
of microtubules regulate the interactions of molecular motors, severing enzymes and tip-tracking proteins with
the microtubules, forming a “tubulin code”. Recent findings revealed a distinct organization of PTMs across the
microtubule bundles in dendrites. I hypothesize that MAPs also form highly organized, stereotyped nanopatterns
that specialize microtubules, or microtubule segments, facilitating efficient, dedicated high-volume transport of
cargo and that these stereotyped MAP nanopatterns control microtubule organization, dynamics, and tubulin
PTMs in neuronal processes. In Aim 1, I will investigate the interplay between MAPs and PTMs by utilizing iPSC-
derived neurons to generate high-resolution maps of MAPs and PTMs during neuronal maturation using
Expansion Microscopy (ExM). In Aim 2, I will knockdown MAPs, both individually and in combination, using
CRISPRi to monitor changes to neuronal morphology, microtubule organization, intracellular trafficking, and the
nanopatterns of MAPs and PTMs. This will shed light on the specific roles each MAP plays in establishing the
intricate microtubule arrays necessary to maintain neuronal health. In Aim 3, I will dissect the interplay between
MAPs and PTMs through in vitro reconstitution assays, offering mechanistic insights into the principles governing
MAP nanopattern formation on microtubules. Overall, this work will explore fundamental questions regarding the
formation of the neuronal cytoskeleton and intracellular transport, with broader implications for the field of cell
biology. This proposal will give me the opportunity to gain a wide breadth of knowledge ranging from in vitro
reconstitution of the tubulin code to genetic engineering of iPSC-derived neurons and super-resolution
microscopy in the labs of my primary sponsor Dr. Roll-Mecak and co-sponsor Dr. Hari Shroff as well as through
consultation w...

## Key facts

- **NIH application ID:** 10941508
- **Project number:** 1FI2GM154713-01
- **Recipient organization:** U.S. NATIONAL INST/NEURO/DS/STROKE
- **Principal Investigator:** Joseph Cleary
- **Activity code:** FI2 (R01, R21, SBIR, etc.)
- **Funding institute:** NIH
- **Fiscal year:** 2024
- **Award amount:** —
- **Award type:** 1
- **Project period:** 2024-09-01 → 2027-08-31

## Primary source

NIH RePORTER: https://reporter.nih.gov/project-details/10941508

## Citation

> US National Institutes of Health, RePORTER application 10941508, Functional interplay between MAP and PTM patterns in the human neuron (1FI2GM154713-01). Retrieved via AI Analytics 2026-05-21 from https://api.ai-analytics.org/grant/nih/10941508. Licensed CC0.

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