Abstract

? To-date most real time imaging procedures have been used to detect cancer cells in vivo. The application of these methods may not be appropriate for stem cells for several reasons. First, the tracking systems include the expression in the cells to be tracked of a foreign protein that has the potential of altering stem cell behavior such as proliferation, differentiation, and migration. Second, the production of the foreign protein, often to reach many fold over the levels of other proteins in the cell, requires that the cell devote a significant portion of its energy to its synthesis. Although this is not likely to be a problem for cancer cells which generally express very high levels of hexokinase and glucose transporters for making ATP by glycolysis, stem cells are less robust and could be debilitated. For effective tissue repair, stem cells must migrate and proliferate in regions of previously damaged tissues that are often hypoxic and nutrient depleted. ? ? The additional need to synthesize a foreign protein from a constitutive promoter that cannot readily be down regulated will place an energy burden on the cells when they need to cope with an inadequate environment and may decrease the number of cells that can successfully populate the damaged tissue. Consequently, for marking stem cells, it would be of great advantage to have a system that does not place a large energy burden on the cells that are being imaged. ? ? The ultimate goal of the research proposed here is to develop an innocuous means of marking stem cells so that they can be tracked in vivo and in real time without their potential for homing, proliferation and differentiation being altered by the marking system. The current proposal describes a novel nucleic acid structure that will be expressed in cells to mark them so they can be tracked in vivo by available imaging technology. We call the markers """"""""Intracellular MultiAptamer Genetic Tags"""""""" (IMAGEtags). The basic innovation in the proposed IMAGEtag design is the expression in living cells of aptamers that can be used to track the cells in vivo by a noninvasive procedure. Cells that express IMAGEtags will be detected by virtue of the concentrated ligands bound to the aptamers. (End of Abstract) ? ?

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Institute of Biomedical Imaging and Bioengineering (NIBIB)
Type
Research Project (R01)
Project #
5R01EB005075-02
Application #
6950729
Study Section
Special Emphasis Panel (ZHL1-CSR-K (S1))
Program Officer
Zhang, Yantian
Project Start
2004-09-20
Project End
2008-07-31
Budget Start
2005-08-01
Budget End
2006-07-31
Support Year
2
Fiscal Year
2005
Total Cost
$229,834
Indirect Cost

  Institution

Name
Iowa State University
Department
Biochemistry
Type
Schools of Earth Sciences/Natur
DUNS #
005309844
City
Ames
State
IA
Country
United States
Zip Code
50011

  Publications

Ray, J; Shin, I; Ilgu, M et al. (2016) IMAGEtags: Quantifying mRNA Transcription in Real Time with Multiaptamer Reporters. Methods Enzymol 572:193-213
Ilgu, Muslum; Ray, Judhajeet; Bendickson, Lee et al. (2016) Light-up and FRET aptamer reporters; evaluating their applications for imaging transcription in eukaryotic cells. Methods 98:26-33
Shin, Ilchung; Ray, Judhajeet; Gupta, Vinayak et al. (2014) Live-cell imaging of Pol II promoter activity to monitor gene expression with RNA IMAGEtag reporters. Nucleic Acids Res 42:e90
Boushaba, Khalid; Levine, Howard; Hamilton, Marit Nilsen (2009) A mathematical feasibility argument for the use of aptamers in chemotherapy and imaging. Math Biosci 220:131-42