Abstract

The University of Iowa Flow Cytometry Facility, established in 1979, supports a broad base of campus research projects. The Facility has grown to include nine instruments used by 23 departments across five colleges. Serving a diverse group of investigators requires instruments capable of accommodating a wide range of experiments. High-speed, multi-color cell sorting is a major component of this service. The Facility has only housed three cell sorters over its 30- year history, each used consecutively. The instruments were replaced only when they became obsolete in terms of scientific merit or difficult to maintain because of lack of spare parts and/or manufacturer support. This indicates that public funds have been used responsibly and wisely in support of healthcare-related research at the University of Iowa. The Facility's current cell sorter, scheduled to be obsolete after 2010, is a 2002 Becton Dickinson FACS DiVa. It serves as a work horse for cloning, isolating cells expressing fluorescent protein markers, multi-color cell sorting of rare cell populations, sorting based on cell cycle, and stem cell sorting of side populations. This Shared Instrumentation Application requests funds for a Becton Dickinson FACS Aria high-speed, multi-color cell sorter to replace the current instrument and to increase the number of colors, sensitivity, and capacity it provides to investigators. The Facility's long-term goal is to remain as close to state of the art as possible in support of its investigators'research. A replacement cell sorter is absolutely necessary given the wide spectrum of institutions and investigators that will be impacted if there is no access to cell sorting. Becton Dickinson discontinued sales of the FACS Vantage SE/DiVa family of instruments in 2007, DiVa software upgrades in 2008, and service contracts after 2010 (see attached letter). When parts and software to support the instrument become difficult to obtain after 2010, the current instrument will be mothballed. Secondly, the other two publicly accessible cell sorters that were previously available in the state of Iowa were retired in 2008. One of those instruments was housed at Iowa State University, and the other was housed in the University Of Iowa Department Of Pathology. The Flow Cytometry Facility now has the only operational cell sorter at an Iowa Board of Regents institution and must provide service to a larger number of investigators. If this sorter is not replaced, investigators will not be able to execute their funded research.

Public Health Relevance

University of Iowa researchers use flow cytometry, a fluorescence-based tool, to study human diseases such as prostate and breast cancer, lymphoma, cancer metastasis, autoimmune disease, neurodegenerative disease, influenza, SARS infection, cellular effects of PCB pollutants, and Stem cell therapies. The cells that may hold the key to understanding and treating these diseases are usually present in minuscule numbers and cannot be readily examined. Sorting by flow cytometry allows the investigators to obtain large amounts of these important cells which can then be examined.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Center for Research Resources (NCRR)
Type
Biomedical Research Support Shared Instrumentation Grants (S10)
Project #
1S10RR027219-01
Application #
7790807
Study Section
Special Emphasis Panel (ZRG1-CB-J (30))
Program Officer
Tingle, Marjorie
Project Start
2009-09-01
Project End
2010-08-31
Budget Start
2009-09-01
Budget End
2010-08-31
Support Year
1
Fiscal Year
2009
Total Cost
$499,900
Indirect Cost

  Institution

Name
University of Iowa
Department
Internal Medicine/Medicine
Type
Schools of Medicine
DUNS #
062761671
City
Iowa City
State
IA
Country
United States
Zip Code
52242

  Publications

Mock, Donald M; Nalbant, Demet; Kyosseva, Svetlana V et al. (2018) Development, validation, and potential applications of biotinylated red blood cells for posttransfusion kinetics and other physiological studies: evidenced-based analysis and recommendations. Transfusion 58:2068-2081
Gorman, Jacob V; Colgan, John D (2018) Acute stimulation generates Tim-3-expressing T helper type 1 CD4 T cells that persist in vivo and show enhanced effector function. Immunology 154:418-433
McGowan, Stephen E; McCoy, Diann M (2017) Glucocorticoids Retain Bipotent Fibroblast Progenitors during Alveolar Septation in Mice. Am J Respir Cell Mol Biol 57:111-120
Barr, Jennifer Y; Goodfellow, Renee X; Colgan, Diana F et al. (2017) Early B Cell Progenitors Deficient for GON4L Fail To Differentiate Due to a Block in Mitotic Cell Division. J Immunol 198:3978-3988
Peters, Anna L; Beuger, Boukje; Mock, Donald M et al. (2016) Clearance of stored red blood cells is not increased compared with fresh red blood cells in a human endotoxemia model. Transfusion 56:1362-9
Schaut, Robert G; Lamb, Ian M; Toepp, Angela J et al. (2016) Regulatory IgDhi B Cells Suppress T Cell Function via IL-10 and PD-L1 during Progressive Visceral Leishmaniasis. J Immunol 196:4100-9
Shrestha, Rajiv P; Horowitz, Joseph; Hollot, Christopher V et al. (2016) Models for the red blood cell lifespan. J Pharmacokinet Pharmacodyn 43:259-74
McGowan, Stephen E; McCoy, Diann M (2015) Fibroblast growth factor signaling in myofibroblasts differs from lipofibroblasts during alveolar septation in mice. Am J Physiol Lung Cell Mol Physiol 309:L463-74
Borcherding, Nicholas; Kusner, David; Kolb, Ryan et al. (2015) Paracrine WNT5A Signaling Inhibits Expansion of Tumor-Initiating Cells. Cancer Res 75:1972-82
Richer, Martin J; Pewe, Lecia L; Hancox, Lisa S et al. (2015) Inflammatory IL-15 is required for optimal memory T cell responses. J Clin Invest 125:3477-90

Showing the most recent 10 out of 13 publications