R35GM141907
Project Grant
Overview
Grant Description
Defining and Controlling Protein-RNA Interactions in Editing and Interference Pathways
This Maximizing Investigators Research Award (MIRA) application is proposed to support research in the Beal Lab at UC Davis focused on defining and controlling protein-RNA interactions in RNA editing and RNA interference pathways.
The RNA editing ADAR enzymes convert adenosines (A) to inosines (I) in duplex RNA. Since I can behave similarly to guanosine (G) in RNA, this modification can have profound effects on the structure and function of the modified RNA, including changes in the meaning of specific codons (recoding). Mutations in the human ADAR1 gene cause the skin disorder dyschromatosis symmetrica hereditaria (DSH) and the autoimmune disease Aicardi-Goutieres syndrome (AGS). Additionally, ADAR1 upregulation and hyper editing have been observed in several different cancers. Despite the significance of this form of regulation of RNA structure and function, there remain key gaps in our understanding of A to I RNA editing. In addition, given ADARs' ability to change RNA sequence, there is growing interest in harnessing this property and directing it to correct disease-associated G-to-A mutations.
Key questions in this field that will be addressed in this project are:
1) What are the structures of key protein-RNA complexes in editing pathways? Structures of full-length human ADAR2 bound to different RNA substrates, along with structures of ADAR1 bound to RNA, are necessary for a full understanding of substrate recognition and selectivity in RNA editing.
2) Can we develop potent, selective, and low MW ADAR inhibitors? Such inhibitors could serve as lead compounds in the development of ADAR1-targeted cancer therapies.
3) Can we develop new strategies to evolve mutant editing enzymes and novel substrate RNAs? The results of these efforts will inform the design of highly efficient and selective reagents for directed RNA editing applications.
Our laboratory also has a longstanding interest in the development of chemical modifications of RNA that can control the interaction with RNA-binding proteins. Much of our recent work in this area has focused on controlling the interaction of RNA with components of siRNA-triggered or miRNA-triggered gene silencing pathways. The use of the RNAi pathway to study gene function has become a powerful tool in molecular biology and has been exploited in the development of new therapeutics. However, specific issues exist that limit its application. These issues include off-target effects that arise from the ability of an siRNA guide strand to function as a miRNA. In addition, antisense oligonucleotides targeting miRNAs (anti-miRs) have significant therapeutic potential and require chemical modification for stability and efficacy. Up to this point, the development of new chemical modifications of therapeutic RNAs has been largely an ad hoc process.
The key question addressed in this aspect of the proposed project is: Can we develop an effective systematic approach to new RNA modifications that modulate protein-RNA interactions in interference pathways? The immediate impact of these studies will be to provide new modifications to siRNAs and anti-miRs that improve potency and selectivity. However, our continued refinement of an approach that uses computational screening coupled with versatile RNA modification chemistry will be generally applicable to other projects that involve chemically modified RNA for therapeutics.
This Maximizing Investigators Research Award (MIRA) application is proposed to support research in the Beal Lab at UC Davis focused on defining and controlling protein-RNA interactions in RNA editing and RNA interference pathways.
The RNA editing ADAR enzymes convert adenosines (A) to inosines (I) in duplex RNA. Since I can behave similarly to guanosine (G) in RNA, this modification can have profound effects on the structure and function of the modified RNA, including changes in the meaning of specific codons (recoding). Mutations in the human ADAR1 gene cause the skin disorder dyschromatosis symmetrica hereditaria (DSH) and the autoimmune disease Aicardi-Goutieres syndrome (AGS). Additionally, ADAR1 upregulation and hyper editing have been observed in several different cancers. Despite the significance of this form of regulation of RNA structure and function, there remain key gaps in our understanding of A to I RNA editing. In addition, given ADARs' ability to change RNA sequence, there is growing interest in harnessing this property and directing it to correct disease-associated G-to-A mutations.
Key questions in this field that will be addressed in this project are:
1) What are the structures of key protein-RNA complexes in editing pathways? Structures of full-length human ADAR2 bound to different RNA substrates, along with structures of ADAR1 bound to RNA, are necessary for a full understanding of substrate recognition and selectivity in RNA editing.
2) Can we develop potent, selective, and low MW ADAR inhibitors? Such inhibitors could serve as lead compounds in the development of ADAR1-targeted cancer therapies.
3) Can we develop new strategies to evolve mutant editing enzymes and novel substrate RNAs? The results of these efforts will inform the design of highly efficient and selective reagents for directed RNA editing applications.
Our laboratory also has a longstanding interest in the development of chemical modifications of RNA that can control the interaction with RNA-binding proteins. Much of our recent work in this area has focused on controlling the interaction of RNA with components of siRNA-triggered or miRNA-triggered gene silencing pathways. The use of the RNAi pathway to study gene function has become a powerful tool in molecular biology and has been exploited in the development of new therapeutics. However, specific issues exist that limit its application. These issues include off-target effects that arise from the ability of an siRNA guide strand to function as a miRNA. In addition, antisense oligonucleotides targeting miRNAs (anti-miRs) have significant therapeutic potential and require chemical modification for stability and efficacy. Up to this point, the development of new chemical modifications of therapeutic RNAs has been largely an ad hoc process.
The key question addressed in this aspect of the proposed project is: Can we develop an effective systematic approach to new RNA modifications that modulate protein-RNA interactions in interference pathways? The immediate impact of these studies will be to provide new modifications to siRNAs and anti-miRs that improve potency and selectivity. However, our continued refinement of an approach that uses computational screening coupled with versatile RNA modification chemistry will be generally applicable to other projects that involve chemically modified RNA for therapeutics.
Awardee
Funding Goals
NOT APPLICABLE
Grant Program (CFDA)
Awarding / Funding Agency
Place of Performance
Davis,
California
95616
United States
Geographic Scope
Single Zip Code
Related Opportunity
Analysis Notes
Amendment Since initial award the End Date has been extended from 04/30/26 to 02/28/31 and the total obligations have increased 847% from $342,175 to $3,238,891.
Davis University Of California was awarded
Protein-RNA Interaction Control in Editing & Interference Pathways
Project Grant R35GM141907
worth $3,238,891
from the National Institute of General Medical Sciences in May 2021 with work to be completed primarily in Davis California United States.
The grant
has a duration of 9 years 9 months and
was awarded through assistance program 93.859 Biomedical Research and Research Training.
The Project Grant was awarded through grant opportunity Maximizing Investigators' Research Award (R35 - Clinical Trial Optional).
Status
(Ongoing)
Last Modified 6/22/26
Period of Performance
5/1/21
Start Date
2/28/31
End Date
Funding Split
$3.2M
Federal Obligation
$0.0
Non-Federal Obligation
$3.2M
Total Obligated
Activity Timeline
Transaction History
Modifications to R35GM141907
Additional Detail
Award ID FAIN
R35GM141907
SAI Number
R35GM141907-2619295097
Award ID URI
SAI UNAVAILABLE
Awardee Classifications
Public/State Controlled Institution Of Higher Education
Awarding Office
75NS00 NIH National Institute of General Medical Sciences
Funding Office
75NS00 NIH National Institute of General Medical Sciences
Awardee UEI
TX2DAGQPENZ5
Awardee CAGE
1CBG4
Performance District
CA-04
Senators
Dianne Feinstein
Alejandro Padilla
Alejandro Padilla
Budget Funding
| Federal Account | Budget Subfunction | Object Class | Total | Percentage |
|---|---|---|---|---|
| National Institute of General Medical Sciences, National Institutes of Health, Health and Human Services (075-0851) | Health research and training | Grants, subsidies, and contributions (41.0) | $1,102,487 | 100% |
Modified: 6/22/26