Abstract

Currently, there are no suitable microscopy tools available that would allow researchers to follow the vast number of newly discovered, diverse non-protein coding (nc)RNAs around the cell as they fulfill their numerous biological functions, let alone at the single molecule level. The proposed project will fundamentally overcome this limitation by developing a novel probe concept optimized for detecting single small ncRNA molecules inside living cells. It is expected that our """"""""molecular Christmas tree"""""""" probe technology will subsequently be transferable to other biopolymers. When developing a new cell microscopy technique, real-world field testing on a biological system for the purpose of determining performance parameters is essential. Among recently discovered ncRNAs are those associated with the new gene regulatory paradigm of RNA interference (RNAi), where in one pathway micro-RNAs (miRNAs) act to repress endogenous genes in all multicellular eukaryotes, including humans. A founding class member is let-7, or lethal-7, which is an evolutionarily conserved miRNA from C. elegans to humans. It has been found to regulate expression of disease-related transcriptional effectors, among them the High Mobility Group AT-hook 2 (HMGA2) protein involved in transcriptional regulation and associated with various cancers as well as diet-induced obesity. Expression of HMGA2 mRNA is controlled by an unusual seven let-7a-1 binding sites. As a proof-of-principle for our intracellular probe technology we will detect the assembly of let-7 miRNA, HMGA2 mRNA and RNAi proteins into single active micro-RNA-protein (miRNP) complexes, by pursuing the following milestones in collaboration with the groups of Sunney Xie (Harvard U.) and David Bartel (Whitehead Institute/MIT): (1) We will design, synthesize and test single molecule detection in cultured cells on a fully controllable sample. The necessary signal-to-noise threshold (amplification level) for intracellular detection of single assembled miRNP complexes is reached once a sufficient number of labeled let-7a probes are loaded onto a single target and slowly diffuse together in a complex. (2) We will test the developed probe technology on the real-world Let-7a/HMGA2 mRNA probe/target system and uniquely address numerous outstanding questions concerning the cell biology of miRNAs. (3) We will define the scope and limitations of our """"""""molecular Christmas tree"""""""" probe technology. That is, in parallel to Aims 1 and 2 we will ask: Is multiplexing (i.e., the detection of multiple targets in parallel) possible? Can multiple tandem repeat sequences in a DNA target be detected? Can protein assembly, particularly that occurring during protein misfolding diseases such as Alzheimer's and prion diseases, be detected by our novel """"""""molecular Christmas tree"""""""" probe concept? What are the lower limits for DNA repeat sequence and protein polymerization detection and can these limits be further pushed? Can multiple different biopolymers be detected in parallel and how does this affect detection limits? ? ? ?

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Institute of General Medical Sciences (NIGMS)
Type
Research Project (R01)
Project #
5R01GM081025-02
Application #
7476308
Study Section
Special Emphasis Panel (ZRG1-BST-R (51))
Program Officer
Deatherage, James F
Project Start
2007-08-01
Project End
2011-07-31
Budget Start
2008-08-01
Budget End
2009-07-31
Support Year
2
Fiscal Year
2008
Total Cost
$245,413
Indirect Cost

  Institution

Name
University of Michigan Ann Arbor
Department
Chemistry
Type
Schools of Arts and Sciences
DUNS #
073133571
City
Ann Arbor
State
MI
Country
United States
Zip Code
48109

  Publications

Pitchiaya, Sethuramasundaram; Heinicke, Laurie A; Park, Jun I et al. (2017) Resolving Subcellular miRNA Trafficking and Turnover at Single-Molecule Resolution. Cell Rep 19:630-642
Tsekouras, Konstantinos; Custer, Thomas C; Jashnsaz, Hossein et al. (2016) A novel method to accurately locate and count large numbers of steps by photobleaching. Mol Biol Cell 27:3601-3615
Rinaldi, Arlie J; Suddala, Krishna C; Walter, Nils G (2015) Native purification and labeling of RNA for single molecule fluorescence studies. Methods Mol Biol 1240:63-95
Pitchiaya, Sethuramasundaram; Heinicke, Laurie A; Custer, Thomas C et al. (2014) Single molecule fluorescence approaches shed light on intracellular RNAs. Chem Rev 114:3224-65
Ma, Jiong; Liu, Zhen; Michelotti, Nicole et al. (2013) High-resolution three-dimensional mapping of mRNA export through the nuclear pore. Nat Commun 4:2414
Pitchiaya, Sethuramasundaram; Krishnan, Vishalakshi; Custer, Thomas C et al. (2013) Dissecting non-coding RNA mechanisms in cellulo by Single-molecule High-Resolution Localization and Counting. Methods 63:188-99
Pitchiaya, Sethuramasundaram; Androsavich, John R; Walter, Nils G (2012) Intracellular single molecule microscopy reveals two kinetically distinct pathways for microRNA assembly. EMBO Rep 13:709-15
Androsavich, John R; Chau, B Nelson; Bhat, Balkrishen et al. (2012) Disease-linked microRNA-21 exhibits drastically reduced mRNA binding and silencing activity in healthy mouse liver. RNA 18:1510-26
Hoerter, John A H; Krishnan, Vishalakshi; Lionberger, Troy A et al. (2011) siRNA-like double-stranded RNAs are specifically protected against degradation in human cell extract. PLoS One 6:e20359
Rawlings, Renata A; Krishnan, Vishalakshi; Walter, Nils G (2011) Viral RNAi suppressor reversibly binds siRNA to outcompete Dicer and RISC via multiple turnover. J Mol Biol 408:262-76

Showing the most recent 10 out of 17 publications