SBIR-STTR Award

Modified RNA Tools and Diagnostics for Drug Abuse
Award last edited on: 11/18/19

Sponsored Program
STTR
Awarding Agency
NIH : NIDA
Total Award Amount
$224,975
Award Phase
1
Solicitation Topic Code
NIDA
Principal Investigator
Paul F Agris

Company Information

Athghin Biotechnology Inc

One Discovery Drive
Rensselaer, NY 12144
   (917) 628-8502
   N/A
   N/A

Research Institution

State University of New York

Phase I

Contract Number: 1R41DA038983-01
Start Date: 9/1/14    Completed: 8/31/16
Phase I year
2014
Phase I Amount
$224,975
RNA modifications are numerous, and range from simple methylation to complex changes such as addition of aminoacylcarbamoyl moieties. These modifications and, the levels at which are present, are emerging as important regulators of biological processes, and perturbations such as chemical or drug exposure can alter the patterns of specific modifications on RNA sub-types. Moreover, given their variety, specificity and their relationship to function and structure stability, RNA modifications are potentially valuable biomarkers of disease and treatment progression, especially given that modified nucleosides are relatively stable even after RNA degradation, and can be released from cells into bodily fluids. The long term objective of this study is to facilitae research into RNA modifications and their impact on health and disease. The immediate hurdle, and the goal of this application, is to develop extremely sensitive analytical methods for detection and quantification of common and novel RNA modifications that can be readily disseminated to the RNA research community. The test case biological system is based on human induced pluripotent stem cell derived nervous system cells that will be exposed to two different drugs of abuse, nicotine and cannabinoids. Aim 1. We will use RNA modified nucleoside standards to develop highly sensitive and robust method of analysis. The ultimate tool we will be developing is a product resultant from the combination of two technologies, UHPLC and MS that will be optimized for high resolution separation and highly sensitive detection of RNA modifications. The tools developed will be tested on differentiated anterior cerebral cortex neurons and glia cells and RNA modifications will be characterized and abundances quantified during the different stages of maturation. Aim 2. Tools developed during aim 1 will be further adapted to detect specific RNA modifications that may be playing a significant role on differentiated forebrain cells, as a result from treatment with drug of abuse. During this aim we will specifically study forebrain cells that will be exposed to different nicotie and cannabinoids concentrations and compared to vehicle controls. The results of the methods we are proposing will be in the form of highly sensitive and accurate tools for the analysis of a wide range of chemistries and abundances of RNA modifications present in regulatory RNAs. The ultimately goal is to develop highly sensitive RNA modifications-based biomarkers discovery tools that requires minimal level of technical expertise as a way to disseminate and accelerate the field of RNA modifications with regards to gain further insight into mechanisms of disease.

Public Health Relevance Statement:


Public Health Relevance:
RNA, the fundamental molecular building block, can be chemically modified in a variety of ways to achieve differences in stability, function and ultimately affect cell processes such as proliferation and metabolic state that are important in health and disease. We need to understand the impact of specific RNA modifications in biological processes and how they respond to chemical or drug exposure or with pathology. In order to facilitate such studies, sensitive, robust and readily adoptable methods to detect and quantify RNA modifications are needed, which is the goal of this proposed study.

Project Terms:
abstracting; Adopted; Affect; analytical method; Anterior; base; Biological; Biological Assay; Biological Markers; Biological Process; biological systems; Brain; brain cell; Cannabinoids; Cell physiology; Cells; Cerebral cortex; Chemical Exposure; Chemicals; Chemistry; Chronic; Communities; Complex; Computer software; computerized data processing; Cues; Detection; Development; Diagnostic; Disease; Drug abuse; Drug Exposure; drug of abuse; Epigenetic Process; Functional RNA; Gene Expression; Gene Expression Regulation; Goals; Health; High Pressure Liquid Chromatography; Human; induced pluripotent stem cell; insight; instrumentation; Investigation; Legal; liquid chromatography mass spectrometry; Liquid substance; Mass Spectrum Analysis; Measures; Mental disorders; Messenger RNA; Metabolic; Methods; Methylation; Modification; Molecular; nervous system disorder; Nervous system structure; Neuroglia; Neurons; Nicotine; novel; Nucleosides; Pathology; Pattern; Pharmaceutical Preparations; Play; Prosencephalon; public health relevance; Reporting; Research; Resolution; RNA; RNA Degradation; RNA Stability; Role; Sample Size; Specificity; Speed (motion); Staging; Structure; Substance abuse problem; Substance of Abuse; Technical Expertise; Technology; Testing; tool

Phase II

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Start Date: 00/00/00    Completed: 00/00/00
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