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Microencapsulation of Leydig cells Team: Bryan Baxter Tim Eng Joe Zechlinski April Zehm BME 400 October 14, 2005
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Client: Dr. Craig Atwood Dr. Sivan Vadakkadath Meethal Miguel Gallego VA Hospital Advisor: Assistant Professor Kristyn Masters Department of Biomedical Engineering
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Overview Problem Statement Problem Statement Background Background Design Specifications Design Specifications Recap of previous work Recap of previous work New directions New directions
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Problem Statement Develop method of encapsulating cells to allow hormone release while providing a physical barrier to the host’s immune system Develop method of encapsulating cells to allow hormone release while providing a physical barrier to the host’s immune systemMotivation Potential alternative to less desirable treatments Potential alternative to less desirable treatments –Organ transplant –Hormone injections –Cellular grafts
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Microcapsules Provide physical barrier to immune system Provide physical barrier to immune system Consist of hydrogels Consist of hydrogels Implanted in vivo Implanted in vivo Time-released hormone therapy Time-released hormone therapy (Uludag et al., 2000)
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Client Research Microencapsulation applications Microencapsulation applications –Anti-aging therapy –Reproductive disorders Cells and hormones of interest Cells and hormones of interest –Leydig and Sertoli cells –Testosterone, inhibin, activin, FSH, LH (Ownby, 1999)(Adapted from Morohashi, 1997)
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Design Specifications Biocompatibility Biocompatibility –Material properties –Crosslinking procedure Repeatability of results Repeatability of results Immunoprotection Immunoprotection –Controlled pore size (MWCO) Degradation Degradation –Mechanical –Biological
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Previous work Polyethylene glycol (PEG) – –Diacrylated synthetic polymer – –UV-crosslinked – –Water-in-oil emulsification
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Previous work Bioprinter – –Modified Epson R200 inkjet printer – –Piezoelectric droplet generation – –Linux platform, software interface
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Microsphere Production Microfluidic devices Microfluidic devices –Increased precision and control on microscale Sample and sheath flow rates determine size and quantity of microcapsules –Minimal reagents used (Jeong et al., 2005)
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Cell culture Cell line Cell line –MA-10 cells (mouse cancer Leydig cells) –Produce testosterone Cell passaging Cell passaging –Split proliferating cells –Hemocytometry –Cryofreezing (Saltzman, 2004.)
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PEG hydrogels on the macroscale Current Experiments: Current Experiments: –Acrylation procedure –Hydrogel swelling/PEG crosslinking Planned Experiments: Planned Experiments: –Combine with MA-10 cell suspension 12.5x
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Viability/Hormone studies Live/Dead® assay Live/Dead® assay –Metabolism (green live) –Membrane integrity (red dead) Testosterone assay Testosterone assay –Competitive sandwich ELISA (ALPCO Diagnostics) (http://respiratory-research.com)
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References Jeong, W., et al. 2005. Continuous fabrication of biocatalyst immobilized microparticles using photopolymerization and immiscible liquids in microfluidic systems. Langmuir 21: 3738-3741. Machluf M, Orsola A, Boorjian S, Kershen R, and Atala A. 2003. Microencapsulation of leydig cells: a system for testosterone supplementation. Endocrinology 144:4975- 4979. Morohashi, K. 1997. The ontogenesis of the steroidogenic tissues. Genes to Cells 2: 95- 106. Ownby. 1999. Histology: male reproductive system. http://www.cvm.okstate.edu/instruction/mm_curr/histology/MR/HiMRp3.htm. Accessed February 12, 2005. Saltzman, W. 2004. Tissue engineering : engineering principles for the design of replacement organs and tissues. New York : Oxford University Press. Uludag H, De Vos P, and Tresco PA. 2000. Technology of mammalian cell encapsulation. Advanced Drug Delivery Reviews 42:29-64. http://chemfinder.cambridgesoft.com http://respiratory-research.com http://web.indstate.edu/thcme/mwking/glycans.html http://www.cybercolloids.net/library/alginate/structure.php
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