Abstract

Hyaluronan (HA), a secreted polymeric glycosaminoglycan component of extracellular matrices, is essential for cell growth and migration during normal development. Elevated production of HA is associated with several pathological states, including cancer. Studies of human prostate tumor biopsies have demonstrated that HA, not present in normal adult prostate, is dramatically overproduced as a function of disease severity in prostate cancer patients. Tumor cell associated HA is observed in the most invasive cancers and correlates to reduced prognosis for the patient. Overproduction and manipulation of cell surface HA polymers is regulated by the action of hyaluronan synthase enzymes (HAS) and hyaluronidases. Degradation of HA by hyaluronidases produces small oligosaccharide fragments, which are active angiogenic stimuli. The long term goals of the laboratory are to understand how HA accumulation occurs, and how HA synthases and hyaluronidases function in concert to facilitate tumor progression in a physiologically relevant model system. The following specific aims are proposed.
Aim 1 : Determine the relative importance of HA biosynthetic enzymes and HA precursors in promoting HA production and tumorigenesis. The overexpression of HA synthases promotes tumor growth and is likely responsible for HA accumulation. It is unclear how elevated HA synthesis occurs, since HA production directly competes with energy metabolism in the tumor cells. An androgen-stimulated gene, UDP-glucose dehydrogenase, provides the limiting precursor for HA synthase. Coexpression of UDP-glucose dehydrogenase and HA synthase synergistically elevates HA synthesis, so we will assess the independent and concerted impact of these enzymes on tumor promotion.
Aim 2 : Investigate how a balance between HA biosynthesis and degradation in prostate tumor cells regulates phenotype. HA synthase is expected to promote maximal tumor growth only in the presence of hyaluronidase. We have stably selected tumor cell lines for differential expression and coexpression of HA synthase and hyaluronidase. We will use these unique tools to correlate the amount and molecular size of HA produced by the cells with their tumorigenic and metastatic potential following direct prostatic injection.
Aim 3 : Use an inducible system to evaluate the role of HA in tumor growth, regression, and apoptosis. Tetracycline inducible constructs will be used to upregulate HA synthesis in non-tumorigenic prostate tumor cells and to inhibit HA synthesis in highly aggressive prostate tumor cells in an experimentally controlled fashion. The chronological importance of HA in tumorigenesis and its mode of action will be evaluated by eliminating HA production in an established orthotopic tumor and determining vascular density and relative percentages of proliferating and apoptotic cells in tumor sections. ? ? ?

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Cancer Institute (NCI)
Type
Research Project (R01)
Project #
5R01CA106584-03
Application #
7218008
Study Section
Tumor Microenvironment Study Section (TME)
Program Officer
Woodhouse, Elizabeth
Project Start
2005-07-01
Project End
2010-04-30
Budget Start
2007-05-01
Budget End
2008-04-30
Support Year
3
Fiscal Year
2007
Total Cost
$205,583
Indirect Cost

  Institution

Name
University of Nebraska Lincoln
Department
Biochemistry
Type
Schools of Earth Sciences/Natur
DUNS #
555456995
City
Lincoln
State
NE
Country
United States
Zip Code
68588

  Publications

Simpson, Melanie A; Weigel, Janet A; Weigel, Paul H (2012) Systemic blockade of the hyaluronan receptor for endocytosis prevents lymph node metastasis of prostate cancer. Int J Cancer 131:E836-40
Hyde, Annastasia S; Farmer, Erin L; Easley, Katherine E et al. (2012) UDP-glucose dehydrogenase polymorphisms from patients with congenital heart valve defects disrupt enzyme stability and quaternary assembly. J Biol Chem 287:32708-16
Kovar, Joy L; Xu, Xinshe; Draney, Dan et al. (2011) Near-infrared-labeled tetracycline derivative is an effective marker of bone deposition in mice. Anal Biochem 416:167-73
Bharadwaj, Alamelu G; Goodrich, Nathaniel P; McAtee, Caitlin O et al. (2011) Hyaluronan suppresses prostate tumor cell proliferation through diminished expression of N-cadherin and aberrant growth factor receptor signaling. Exp Cell Res 317:1214-25
Huang, Dali; Casale, George P; Tian, Jun et al. (2010) Udp-glucose dehydrogenase as a novel field-specific candidate biomarker of prostate cancer. Int J Cancer 126:315-27
Kovar, Joy L; Volcheck, William; Sevick-Muraca, Eva et al. (2009) Characterization and performance of a near-infrared 2-deoxyglucose optical imaging agent for mouse cancer models. Anal Biochem 384:254-62
Wei, Qin; Galbenus, Robert; Raza, Ashraf et al. (2009) Androgen-stimulated UDP-glucose dehydrogenase expression limits prostate androgen availability without impacting hyaluronan levels. Cancer Res 69:2332-9
Zhang, Ling; Bharadwaj, Alamelu G; Casper, Andrew et al. (2009) Hyaluronidase activity of human Hyal1 requires active site acidic and tyrosine residues. J Biol Chem 284:9433-42
Bharadwaj, Alamelu G; Kovar, Joy L; Loughman, Eileen et al. (2009) Spontaneous metastasis of prostate cancer is promoted by excess hyaluronan synthesis and processing. Am J Pathol 174:1027-36
Simpson, Melanie A; Lokeshwar, Vinata B (2008) Hyaluronan and hyaluronidase in genitourinary tumors. Front Biosci 13:5664-80

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