Abstract

The long-term goal of this project is to elucidate mechanisms underlying assembly of the enterocyte brush border, the sole site of nutrient absorption, and the primary surface of interaction with bacteria and bacterial products that accumulate in the intestinal lumen. Found at the apex of the enterocyte, the brush border contains up to one thousand tightly packed microvilli: actin bundle-supported membrane protrusions that extend off the cell surface to a nearly identical length. The functional consequence of this arrangement is an immense capacity for housing membrane-associated nutrient processing and host defense machinery that is required for maintaining gut homeostasis. Despite being positioned at a critical physiological interface in the GI tract, there s little information on how microvillar actin bundles are nucleated, how microvillar length is controlled, or how microvilli achieve perfectly tight packing during enterocyte differentiation. Using the CACO- 2BBE cell culture model to explore the physical remodeling of the enterocyte apical surface during differentiation, our laboratory made a series of exciting discoveries that provide insight on fundamental mechanisms of brush border formation. During the early stages of brush border assembly, we observe that microvilli cluster together and interact at their tips toform 'tepee' shaped structures. As differentiation proceeds, the observed 'tepees' grow larger by incorporating more microvilli. Electron microscopy of these structures revealed, for the first time that adjacent microvilli in these tepees are physically connected to each other by thread-like links. These observations suggest that the tight packing of microvilli during brush border assembly may be driven by adhesion complexes that are inherent to these protrusions. We also identified a member of the cadherin superfamily, protocadherin-24 (PCDH24), which exhibits striking enrichment at the tips of microvilli. Interestingly, knockdown of PCDH24 also gives rise to defects in microvillar clustering. Based on these and other preliminary findings, we propose that PCDH24 creates inter-microvillar adhesion links at microvillar tips, which are required for the tight packing of these protrusions during brush border assembly.
The Aims proposed herein will begin to test this hypothesis by investigating: (1) the targeting and requirement for PCDH24 during brush border assembly, (2) the adhesion capacity of PCDH24, and (3) the mechanism underlying the microvillar tip localization of PCDH24. Given our expertise in defining the biological and physical underpinnings of brush border function, our group is well positioned to test this hypothesis and generate insight on this fundamental aspect of GI epithelial biology.

Public Health Relevance

The epithelial cells that line the intestinal tract build hundreds of cylindrical protrusions on their apical surface;these 'microvilli'extend into the gut lumen, increasing the amount of apical membrane surface area available for nutrient absorption. Despite occupying a critical physiological interface in the gut, there is little information on how microvillar protrusions are built and/or maintained. The proposed work will elucidate molecular mechanisms underlying the construction of microvilli during the differentiation of intestinal epithelial cells and provide insight on the basis of human diseases characterized by loss of microvilli.

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Institute of Diabetes and Digestive and Kidney Diseases (NIDDK)
Type
High Priority, Short Term Project Award (R56)
Project #
1R56DK095811-01
Application #
8543896
Study Section
Clinical, Integrative and Molecular Gastroenterology Study Section (CIMG)
Program Officer
Grey, Michael J
Project Start
2012-09-20
Project End
2013-08-31
Budget Start
2012-09-20
Budget End
2013-08-31
Support Year
1
Fiscal Year
2012
Total Cost
$328,338
Indirect Cost
$110,838

  Institution

Name
Vanderbilt University Medical Center
Department
Anatomy/Cell Biology
Type
Schools of Medicine
DUNS #
004413456
City
Nashville
State
TN
Country
United States
Zip Code
37212

  Publications

Crawley, Scott W; Weck, Meredith L; Grega-Larson, Nathan E et al. (2016) ANKS4B Is Essential for Intermicrovillar Adhesion Complex Formation. Dev Cell 36:190-200
Crawley, Scott W; Shifrin Jr, David A; Grega-Larson, Nathan E et al. (2014) Intestinal brush border assembly driven by protocadherin-based intermicrovillar adhesion. Cell 157:433-446
Knowles, Byron C; Roland, Joseph T; Krishnan, Moorthy et al. (2014) Myosin Vb uncoupling from RAB8A and RAB11A elicits microvillus inclusion disease. J Clin Invest 124:2947-62
Shifrin Jr, David A; Crawley, Scott W; Grega-Larson, Nathan E et al. (2014) Dynamics of brush border remodeling induced by enteropathogenic E. coli. Gut Microbes 5:504-16
Mazerik, Jessica N; Kraft, Lewis J; Kenworthy, Anne K et al. (2014) Motor and tail homology 1 (Th1) domains antagonistically control myosin-1 dynamics. Biophys J 106:649-58
Crawley, Scott W; Mooseker, Mark S; Tyska, Matthew J (2014) Shaping the intestinal brush border. J Cell Biol 207:441-51
Hoshino, Daisuke; Kirkbride, Kellye C; Costello, Kaitlin et al. (2013) Exosome secretion is enhanced by invadopodia and drives invasive behavior. Cell Rep 5:1159-68
Shifrin Jr, David A; Demory Beckler, Michelle; Coffey, Robert J et al. (2013) Extracellular vesicles: communication, coercion, and conditioning. Mol Biol Cell 24:1253-9