Abstract

Protein 4.1 R (4.1 R) was originally identified as an essential component of the red cell membrane cytoskeleton. We have shown that 4.1R plays a role in epithelial morphogenesis and endothelial cell-to-cell junction assemblies. We now propose to characterize the contributions of 4.1 R to tight junction (TJ) biogenesis and membrane polarity in epithelial cells, as well as to adherens junction (AJ) assembly and integrity in endothelial cells. The localization of 4.1 R during epithelial morphogenesis shifts from the nucleus and cytoplasm of non-confluent cells to the lateral membrane of confluent cells, in conjunction with a switch from 4.1R 135 kD, lacking exon 17b, to 4.1 R 160 kD containing exon 17b. In non-confluent nuclei, 4.1R associates with ZO-2. In confluent cells, 4.1R associates with the polarity protein Par3, TJs, and AJs. Dominant negative mutant 4.1R's disrupt TJ integrity and produce an enlarged and flattened morphology. The behavior of 4.1 R during epithelial morphogenesis will be studied in both a model MDCK line and primary epithelial cultures. We shall dissect the mechanisms by which 4.1R associates with partner proteins to form polarized membranes and TJ's using in vitro and in vivo biochemical assays, and fluorescence-based imaging methods. Functional perturbations will be achieved by utilizing siRNA, dominant-negative mutants, and a Tet-off expression system. In AJs, 4.1R co-localizes and associates with the AJ proteins E-cadherin and beta-catenin. Overexpression of 4.1 R reduces E-cadherin localization to the AJs. In order to study AJ's in isolation, we shall use a well-characterized human umbilical vein endothelial cell (HUVEC) primary cell culture. Since HUVEC rarely express TJs, they are more suitable for analyzing the expression and sub-cellular distribution of 4.1 R and proteins with which it associates as they assemble into AJs. We shall delineate the impact of 4.1 R on AJs assembly, using approaches similar to those just described. We shall also test the hypothesis that complementarity may exist between 4.1R and its paralogues (4.1G, N, B), allowing them to compensate for the absence of 4.1 R in knock-out cells. Finally, we shall investigate the relationship between the shift in localization of 4.1 R from nucleus to peripheral membranes and the establishment of contact inhibition in terminally differentiating epithelial cells. These studies should yield new insights about the function of 4.1Rin cellular architecture and achievement of the post-mitotic contact inhibited state. ? ? ?

  Funding Agency

Agency
National Institute of Health (NIH)
Institute
National Heart, Lung, and Blood Institute (NHLBI)
Type
Research Project (R01)
Project #
2R01HL044985-16A1
Application #
7142944
Study Section
Erythrocyte and Leukocyte Biology Study Section (ELB)
Program Officer
Qasba, Pankaj
Project Start
1990-07-01
Project End
2010-07-31
Budget Start
2006-08-01
Budget End
2007-07-31
Support Year
16
Fiscal Year
2006
Total Cost
$424,250
Indirect Cost

  Institution

Name
Dana-Farber Cancer Institute
Department
Type
DUNS #
076580745
City
Boston
State
MA
Country
United States
Zip Code
02215

  Publications

Huang, Shu-Ching; Zhou, Anyu; Nguyen, Dan T et al. (2016) Protein 4.1R Influences Myogenin Protein Stability and Skeletal Muscle Differentiation. J Biol Chem 291:25591-25607
Mattagajasingh, Subhendra N; Huang, Shu-Ching; Benz Jr, Edward J (2009) Inhibition of protein 4.1 R and NuMA interaction by mutagenization of their binding-sites abrogates nuclear localization of 4.1 R. Clin Transl Sci 2:102-11
Huang, Shu-Ching; Liu, Eva S; Chan, Siu-Hong et al. (2005) Mitotic regulation of protein 4.1R involves phosphorylation by cdc2 kinase. Mol Biol Cell 16:117-27
Huang, Shu-Ching; Jagadeeswaran, Ramasamy; Liu, Eva S et al. (2004) Protein 4.1R, a microtubule-associated protein involved in microtubule aster assembly in mammalian mitotic extract. J Biol Chem 279:34595-602
Kontrogianni-Konstantopoulos, A; Frye, C S; Benz Jr, E J et al. (2001) The prototypical 4.1R-10-kDa domain and the 4.1g-10-kDa paralog mediate fodrin-actin complex formation. J Biol Chem 276:20679-87
Mattagajasingh, S N; Huang, S C; Hartenstein, J S et al. (2000) Characterization of the interaction between protein 4.1R and ZO-2. A possible link between the tight junction and the actin cytoskeleton. J Biol Chem 275:30573-85
Kontrogianni-Konstantopoulos, A; Huang, S C; Benz Jr, E J (2000) A nonerythroid isoform of protein 4.1R interacts with components of the contractile apparatus in skeletal myofibers. Mol Biol Cell 11:3805-17
Mattagajasingh, S N; Huang, S C; Hartenstein, J S et al. (1999) A nonerythroid isoform of protein 4.1R interacts with the nuclear mitotic apparatus (NuMA) protein. J Cell Biol 145:29-43
Baklouti, F; Huang, S C; Vulliamy, T J et al. (1997) Organization of the human protein 4.1 genomic locus: new insights into the tissue-specific alternative splicing of the pre-mRNA. Genomics 39:289-302
Baklouti, F; Huang, S C; Tang, T K et al. (1996) Asynchronous regulation of splicing events within protein 4.1 pre-mRNA during erythroid differentiation. Blood 87:3934-41

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