Ischemic heart disease is the primary cause of death in both men and women globally. Ischemic heart conditions, including angina and myocardial infarction, are characterized by loss of blood flow to the heart tissue and reduced cardiac function, both reducing quality of life and increasing mortality. Improved recovery of cardiac function following a myocardial infarction has been observed in several studies upon the injection of high concentrations of endothelial progenitor cells (EPCs) to the ischemic area. Multiple types of EPCs have been shown to play pivotal roles in the formation of new blood vessels, and are promising candidates for accelerated and increased repair of ischemic tissues. Follow up studies indicate both high purity and quantity of EPCs are critical to recovery of function, yet current technologies for sorting of EPCs are incapable of isolating these cells in the purity and speed required for widespread clinical use. This research grant will develop a novel technique for the isolation of EPCs which yields a high-purity isolate at high throughput. The developed technology, Antigen Specific Lysis (ASL), is capable of being performed in a typical research lab setting where batches exceeding 200 mL (>1010 cells) are completed in under an hour. The proposed work will develop high speed selection modalities for the isolation of high purity, functional EPCs. ASL uses targeted coatings to selectively protect EPCs while all other cells are lysed. Preliminary results demonstrate 1) antibody- initiator conjugates are capable of selectively forming a ~100 nm polymer coating on the exterior of only antigen expressing cells, 2) these coatings stabilize cells in harsh environments (5% SDS), and 3) viable cells are released at high purity (>99% purity for antigen positive cells spiked into blood). This research grant drives new advances in wavelength specific polymerization and degradation for the selective protection of targeted cells and the subsequent release of cells with increased viability and proliferative capacity. Sequential selection for CD133+ and CD34+ cells is expected, yielding a >99% pure population of EPCs. This system will also have the capability to process multiple, smaller batches at one time using only standard disposable labware for cell- contacting materials. Finally, the functional properties of clinically-relevant EPC populations isolated fluorescently or by ASL will be evaluated through in vitro and in vivo assays. ASL shows considerable promise as a powerful isolation technique that can be applied both clinically for the treatment of acute myocardial infarctions and in individual research settings for the analysis of rare cellular species in blood. This project is significant because in-lab isolation of large volums of cells will enable the widespread use of EPC therapy for improved cardiac function following acute myocardial infarctions. Future directions of this work include the use of ASL in the isolation of other rare cell populations (other progenitor cells, circulating tumor cells) emergingin clinical research, diagnostics, prognostics, and treatment.

Public Health Relevance

This project develops a new approach to isolating a rare type of cell capable of repairing heart damage. This approach promises to deliver cells with fewer contaminants, faster, and at a lower cost than is possible today. This technology is also expected to both accelerate and reduce the cost of research across a broad spectrum of biological and medical sciences.

Agency
National Institute of Health (NIH)
Institute
National Heart, Lung, and Blood Institute (NHLBI)
Type
Research Project (R01)
Project #
1R01HL127682-01
Application #
8864515
Study Section
Instrumentation and Systems Development Study Section (ISD)
Program Officer
Lee, Albert
Project Start
2015-07-15
Project End
2019-04-30
Budget Start
2015-07-15
Budget End
2016-04-30
Support Year
1
Fiscal Year
2015
Total Cost
$592,359
Indirect Cost
$108,614
Name
University of Kentucky
Department
Engineering (All Types)
Type
Schools of Engineering
DUNS #
939017877
City
Lexington
State
KY
Country
United States
Zip Code
40506
Lilly, Jacob L; Gottipati, Anuhya; Cahall, Calvin F et al. (2018) Comparison of eosin and fluorescein conjugates for the photoinitiation of cell-compatible polymer coatings. PLoS One 13:e0190880
Wu, Pei-Jung; Lilly, Jacob L; Arreaza, Roberto et al. (2017) Hydrogel Patches on Live Cells through Surface-Mediated Polymerization. Langmuir 33:6778-6784
Lilly, Jacob L; Berron, Brad J (2016) The Role of Surface Receptor Density in Surface-Initiated Polymerizations for Cancer Cell Isolation. Langmuir 32:5681-9
Romero, Gabriela; Lilly, Jacob J; Abraham, Nathan S et al. (2015) Protective Polymer Coatings for High-Throughput, High-Purity Cellular Isolation. ACS Appl Mater Interfaces 7:17598-602