# Mechanisms of Nuclear Migration

> **NIH NIH R35** · UNIVERSITY OF CALIFORNIA AT DAVIS · 2020 · $152,408

## Abstract

Project Summary
Nuclear migration and anchorage are central to many cellular events. We uncovered a conserved network of
nuclear envelope proteins and force generators that mediate nuclear positioning. LINC (linker of nucleoskele-
ton and cytoskeleton) complexes, which we discovered, maintain nuclear envelope architecture, mark the
surface of nuclei distinctly from the contiguous ER, and were instrumental in the early evolution of eukaryotes.
We address four gaps in our knowledge of the mechanisms regulating nuclear positioning. (1) How is the
developmental switch between nuclear migration and anchorage mediated? We hypothesize that different
LINC complexes are required for a nucleus to switch from migrating to being anchored. We propose that an
intermolecular disulfide bond, which could be regulated by protein disulfide isomerases and/or the AAA+
ATPase torsin, is central to the switch. We further hypothesize that LINC directly interacts with the outer
nuclear membrane to optimize the transfer of forces across the nuclear envelope. (2) How are nuclei anchored
in large syncytial cells? It is important for nuclei to be evenly spaced so that multi-nucleated syncytia are able
to act as a single unit. We recently found that ANC-1 anchors syncytial nuclei and mitochondria through
unknown, LINC-independent mechanisms, and hypothesize that ANC-1 organizes the cytoplasm through
microtubules. (3) How do nuclei favor one microtubule motor over another at different stages of development?
The KASH protein UNC-83 mediates nuclear movements toward plus or minus ends of microtubules at differ-
ent stages of development. We hypothesize that the choice is regulated by alternative isoforms of UNC-83 that
differentially activate kinesin-1 motor activity. (4) How do nuclei deform to migrate through narrow spaces? Our
data support a model where LINC complexes function parallel to branched actin networks to deform nuclei as
they squeeze through narrow constrictions. Our experimental system is innovative because we can view live
nuclei throughout development, including a tissue where 139 nuclei are in a single hypodermal syncytium and
a second tissue where nuclei migrate through narrow constrictions as a normal part of development. Further-
more, we have developed reagents essential to our future plans, including an array of point mutants in LINC
complexes that separate function, cell-specific markers, a tissue-specific auxin-induced degron system, and
over ten mutant lines from a forward genetic screen for defects in nuclear migration through constrictions. To
complement our C. elegans genetic approaches, we also collaborate to confirm our findings in mammalian
tissue culture cells and an in vitro microtubule motor assay with TIRF microscopy. Our studies are expected to
determine how LINC complexes are regulated at molecular and biophysical levels, how the outer nuclear
membrane is involved in force transmission, how giant KASH proteins organize the global cytoskeleto...

## Key facts

- **NIH application ID:** 9850786
- **Project number:** 1R35GM134859-01
- **Recipient organization:** UNIVERSITY OF CALIFORNIA AT DAVIS
- **Principal Investigator:** DANIEL A STARR
- **Activity code:** R35 (R01, R21, SBIR, etc.)
- **Funding institute:** NIH
- **Fiscal year:** 2020
- **Award amount:** $152,408
- **Award type:** 1
- **Project period:** 2020-01-01 → 2024-12-31

## Primary source

NIH RePORTER: https://reporter.nih.gov/project-details/9850786

## Citation

> US National Institutes of Health, RePORTER application 9850786, Mechanisms of Nuclear Migration (1R35GM134859-01). Retrieved via AI Analytics 2026-05-23 from https://api.ai-analytics.org/grant/nih/9850786. Licensed CC0.

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