# Mitochondrial DNA of Normal and Mutant Trypanosomes

> **NIH NIH R01** · SEATTLE CHILDREN'S HOSPITAL · 2022 · $887,091

## Abstract

Abstract
This project will determine how three closely related editosomes, precisely edit mRNAs and do so differentially
between life cycle stages in Trypanosoma brucei. We hypothesize that insertion and deletion editosome
compositional and structural differences enable differential binding and catalysis of specific gRNA/mRNA
substrates during editing and the differential editing between developmental stages. We will: 1. Determine the
high resolution structures of insertion and deletion editosomes, subcomplexes thereof, and RNA association by
cryoEM. Samples for cryoEM will be purified from cells with one type of functional or catalytically arrested
editosome. This will determine detailed editosomes architecture, protein stoichiometry, RNA location and
differences between these editosomes. 2. Determine the roles non-catalytic editosome proteins/domains. We
will determine if endonuclease partner proteins function as heterodimers and if noncatalytic proteins function in
substrate RNA binding and positioning. The catalytic function of recombinant heterodimers will be assayed by
crosslinking, mutagenesis and sequencing and functional RNA-protein interactions will be identified in vivo. 3.
Determine how editosomes progress from one editing site (ES) to the next and test whether editing is either
processive or progresses non-sequentially 3' to 5' and if endonuclease subcomplexes exchange between
editosomes or not as they encounter different ESs. Cognate gRNA/mRNA pairs engaged in editing in cells with
single or multiple types of functional editosomes will be identified and sequenced to resolve whether editing is
processive or not. Proximal editosome specific proteins that will be tagged in vivo in cells that contain all three,
combinations of two, one, or no functional editosomes that have specific tags and assayed to determine if
editosome components exchange or not during editing. These results along RNAseq analysis of their edited
RNAs will elucidate how the three different editosomes collaborate to edit multiple ESs specified by a single
gRNA, including gRNAs that specify insertion and deletion. 4. Identify key aspects of developmental regulation
of RNA editing. We will determine the order in which differentially edited mRNAs arise during development, if
these are accompanied by differences in the abundances and editosome associations, of specific 3' initiating
gRNAs and cognate gRNA/mRNA pairs, and if these are impacted by mutations that differentially affect editing.
Selected structures of BF and PF editosomes will be compared by CXMS, SILAC and cryoEM based on Aim 1.
These studies will determine whether specific cognate gRNA/mRNA pairs are differentially bound and utilized
as a result of stage specific editosome differences. The project will provide key insights into how three poly-
protein complexes function in an integrated fashion to precisely edit mt mRNAs and differentially regulate this
process between life cycle stages which adapts energy...

## Key facts

- **NIH application ID:** 10397526
- **Project number:** 5R01AI014102-46
- **Recipient organization:** SEATTLE CHILDREN'S HOSPITAL
- **Principal Investigator:** KENNETH D STUART
- **Activity code:** R01 (R01, R21, SBIR, etc.)
- **Funding institute:** NIH
- **Fiscal year:** 2022
- **Award amount:** $887,091
- **Award type:** 5
- **Project period:** 1978-09-01 → 2024-04-30

## Primary source

NIH RePORTER: https://reporter.nih.gov/project-details/10397526

## Citation

> US National Institutes of Health, RePORTER application 10397526, Mitochondrial DNA of Normal and Mutant Trypanosomes (5R01AI014102-46). Retrieved via AI Analytics 2026-05-24 from https://api.ai-analytics.org/grant/nih/10397526. Licensed CC0.

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