# Regulating Microtubule Severing Physically and Chemically

> **NIH NIH R15** · SYRACUSE UNIVERSITY · 2021 · $450,000

## Abstract

Project Summary/Abstract
The goal of this new proposal application is to uncover the physical and chemical regulatory schemes
to control the microtubule severing enzyme, katanin. Katanin is a AAA+ enzyme that hexamerizes in
order to remove tubulin diimers from the microtubule filament resulting in filament severing. When at
high levels, and unregulated in cells, katanin can destroy the entire microtubule network, thus turning
it off is an essential control knob. Overactivity of katanin can lead to complete loss of microtubule
polymer, but underactivity is linked with developmental defects in the brain and ciliopathies. The
central hypothesis of the proposed work is that the mechanisms to control katanin actually regulate
katanin hexamer oligomerization. Our prior work indicated that oligomerization is the a rate-limiting
step for katanin. We seek to use quantitative fluorescence microscopy to directly test the hypothesis
that oligomerization controls severing through physical and chemical means. Specifically, we will
explore the regulation of katanin concentration in live cells using a novel light-sensitive dimerization
domain to drive katanin concentration locally by exploring the following aims: (1) Quantification of
both the katanin concentration and the microtubule filament density as a function of time will enable
biochemistry in the cell for the first time for katanin. (2) Using in vitro reconstitution of microtubule
severing and a novel single molecule counting technique, we will examine the effect of the
phosphorylation state of serine 131 on binding, oligomerization, and severing by katanin. (3) The
tubulin carboxy-terminal tail has been shown to act as a code to control many microtubule-associated
proteins and enzymes. Severing enzymes are no different and are known to require the carboxy-
terminal tail to sever microtubules. Our preliminary data shows that katanin’s regulation is distinct
from other severing enzymes. We will use a severing inhibition assay and single molecule counting to
quantify the ability to katanin to bind and act on microtubules of various carboxy-terminal tail
sequences.
Accomplishing the proposed aims will create a novel microtubule disruption tool that could be used in
a variety of cellular and organismal assays to control the location and density of the microtubule
network. Further, the proposed studies will reveal new information on how microtubule severing can
be regulated in cells through controlling the katanin oligomerization state. This crucial step for katanin
activity may be an entry-point for creating small molecule inhibitors for microtubule severing enzymes
and other AAA+ enzymes that are important for a host of essential cellular functions including protein
homeostasis, DNA recombination, replication, and repair.

## Key facts

- **NIH application ID:** 10202821
- **Project number:** 1R15GM141722-01
- **Recipient organization:** SYRACUSE UNIVERSITY
- **Principal Investigator:** JENNIFER L ROSS
- **Activity code:** R15 (R01, R21, SBIR, etc.)
- **Funding institute:** NIH
- **Fiscal year:** 2021
- **Award amount:** $450,000
- **Award type:** 1
- **Project period:** 2021-05-01 → 2025-04-30

## Primary source

NIH RePORTER: https://reporter.nih.gov/project-details/10202821

## Citation

> US National Institutes of Health, RePORTER application 10202821, Regulating Microtubule Severing Physically and Chemically (1R15GM141722-01). Retrieved via AI Analytics 2026-05-26 from https://api.ai-analytics.org/grant/nih/10202821. Licensed CC0.

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