Abstract

Current use of human- or animal-derived phagocytic cell sources required for biomaterials inflammation and foreign body assay is inconvenient, costly, and potentially unnecessary. Equivalence of secondary macrophage-lineage cell lines in these in vitro assays is largely unproven, although many unpublished anecdotes exist regarding their utility in biomaterials toxicity or inflammatory assays. This proposal's overall objective is to establish, using quantitative modem molecular and cell biological methods, the validity of certain macrophage-derived cell line cultures in accurately duplicating phenotypic behavior of human- and animal-derived phagocytes commonly used to model aspects of the biomaterial implant-generated foreign body response. Our working hypothesis is that phenotypic response and foreign body giant cell formation on several model biomaterials using select secondary macrophage-derived cell lines in cultures designed to monitor cell-mediated inflammatory responses on biomaterials will be measurably similar to that observed using host-derived primary macrophages. Studies seek answers to important, long-standing questions surrounding the appropriate use and limitations of macrophage culture systems to analyze the foreign-body response ubiquitous for all implanted biomaterials. New data will be compared against well-developed primary monocyte/macrophage culture assays now common for biomaterials inflammatory assessments with foreign body giant cells. The following Specific Aims are proposed: (1) Determine selected cell-produced cytokines representing the Th1 and Th2 phenotypic responses in cultured secondary macrophage-derived cell lines on several model biomaterials of controlled surface chemistry; (2) Identify short and long term phenotypic stability in culture through changes in cytokine production and responses in macrophage derived cell cultures as a function of surface chemistry; (3) Quantify several distinct known phenotypic features of foreign body giant cell formation as a function of surface chemistry for macrophage-derived cell lines and primary macrophages over time in culture; (4) Establish reliable, quantitative microarray-based gene analysis to accelerate profiling of specific known markers of macrophage activation and inflammatory behavior, specifically for cytokine expression and apoptosis markers; and (5) Exploit an in vitro co culture system containing cultured macrophages and fibroblasts to study affects of macrophage-derived cytokine production on fibroblast production of collagen and fibrous precursors relevant to encapsulation reactions common to foreign bodies in vivo.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Institute of Biomedical Imaging and Bioengineering (NIBIB)
Type
Research Project (R01)
Project #
5R01EB000894-10
Application #
7176127
Study Section
Special Emphasis Panel (ZRG1-SSS-8 (03))
Program Officer
Lee, Albert
Project Start
1998-01-01
Project End
2009-01-31
Budget Start
2007-02-01
Budget End
2009-01-31
Support Year
10
Fiscal Year
2007
Total Cost
$252,697
Indirect Cost

  Institution

Name
University of Utah
Department
Biomedical Engineering
Type
Schools of Engineering
DUNS #
009095365
City
Salt Lake City
State
UT
Country
United States
Zip Code
84112

  Publications

Chamberlain, Lisa M; Holt-Casper, Dolly; Gonzalez-Juarrero, Mercedes et al. (2015) Extended culture of macrophages from different sources and maturation results in a common M2 phenotype. J Biomed Mater Res A 103:2864-74
Gustafson, Heather Herd; Holt-Casper, Dolly; Grainger, David W et al. (2015) Nanoparticle Uptake: The Phagocyte Problem. Nano Today 10:487-510
Wang, Yuwei; Grainger, David W (2013) Developing siRNA therapies to address osteoporosis. Ther Deliv 4:1239-46
Wang, Yuwei; Tran, Kenny K; Shen, Hong et al. (2012) Selective local delivery of RANK siRNA to bone phagocytes using bone augmentation biomaterials. Biomaterials 33:8540-7
Wang, Yuwei; Grainger, David W (2012) RNA therapeutics targeting osteoclast-mediated excessive bone resorption. Adv Drug Deliv Rev 64:1341-57
Diekjiirgen, Dorina; Astashkina, Anna; Grainger, David W et al. (2012) Cultured primary macrophage activation by lipopolysaccharide depends on adsorbed protein composition and substrate surface chemistry. J Biomater Sci Polym Ed 23:1231-54
Holt, Dolly J; Grainger, David W (2012) Senescence and quiescence induced compromised function in cultured macrophages. Biomaterials 33:7497-507
Holt, Dolly J; Grainger, David W (2011) Multinucleated giant cells from fibroblast cultures. Biomaterials 32:3977-87
Wang, Yuwei; Panasiuk, Alexandra; Grainger, David W (2011) Small interfering RNA knocks down the molecular target of alendronate, farnesyl pyrophosphate synthase, in osteoclast and osteoblast cultures. Mol Pharm 8:1016-24
Wang, Yuwei; Grainger, David W (2010) siRNA knock-down of RANK signaling to control osteoclast-mediated bone resorption. Pharm Res 27:1273-84

Showing the most recent 10 out of 23 publications