The N and C termini of ZO-1 are surrounded by distinct proteins and functional protein networks

Christina M Van Itallie; Angel Aponte; Amber Jean Tietgens; Marjan Gucek; Karin Fredriksson; James Melvin Anderson

doi:10.1074/jbc.M113.466193

The N and C termini of ZO-1 are surrounded by distinct proteins and functional protein networks

J Biol Chem. 2013 May 10;288(19):13775-88. doi: 10.1074/jbc.M113.466193. Epub 2013 Apr 3.

Authors

Christina M Van Itallie¹, Angel Aponte, Amber Jean Tietgens, Marjan Gucek, Karin Fredriksson, James Melvin Anderson

Affiliation

¹ Laboratory of Tight Junction Structure and Function, NHLBI, National Institutes of Health, Bethesda, MD 20892, USA. Christina.vanitallie@nih.gov

Abstract

Background: Biotin ligase tagging with ZO-1 was applied to identify a more complete tight junction proteome.

Results: Identical but also different proteins and functional networks were identified near the N and C ends of ZO-1.

Conclusion: The ends of ZO-1 are embedded in different functional subcompartments of the tight junction.

Significance: Biotin tagging with ZO-1 expands the tight junction proteome and defines subcompartments of the junction. The proteins and functional protein networks of the tight junction remain incompletely defined. Among the currently known proteins are barrier-forming proteins like occludin and the claudin family; scaffolding proteins like ZO-1; and some cytoskeletal, signaling, and cell polarity proteins. To define a more complete list of proteins and infer their functional implications, we identified the proteins that are within molecular dimensions of ZO-1 by fusing biotin ligase to either its N or C terminus, expressing these fusion proteins in Madin-Darby canine kidney epithelial cells, and purifying and identifying the resulting biotinylated proteins by mass spectrometry. Of a predicted proteome of ∼9000, we identified more than 400 proteins tagged by biotin ligase fused to ZO-1, with both identical and distinct proteins near the N- and C-terminal ends. Those proximal to the N terminus were enriched in transmembrane tight junction proteins, and those proximal to the C terminus were enriched in cytoskeletal proteins. We also identified many unexpected but easily rationalized proteins and verified partial colocalization of three of these proteins with ZO-1 as examples. In addition, functional networks of interacting proteins were tagged, such as the basolateral but not apical polarity network. These results provide a rich inventory of proteins and potential novel insights into functions and protein networks that should catalyze further understanding of tight junction biology. Unexpectedly, the technique demonstrates high spatial resolution, which could be generally applied to defining other subcellular protein compartmentalization.

Keywords: Adherens Junction; Mass Spectrometry (MS); Membrane; Proteomics; Tight Junctions; ZO-1.

Publication types

Research Support, N.I.H., Intramural

MeSH terms

Adherens Junctions / metabolism
Animals
Biotin / metabolism
Biotinylation
Carbon-Nitrogen Ligases / metabolism
Cell Line
Chromatography, Affinity
Dogs
Humans
Molecular Sequence Annotation
Protein Interaction Mapping
Protein Interaction Maps
Protein Structure, Tertiary
Protein Transport
Recombinant Fusion Proteins / metabolism
Tight Junction Proteins / isolation & purification
Tight Junction Proteins / metabolism*
Tight Junctions / metabolism
Zonula Occludens-1 Protein / metabolism*

Substances

Recombinant Fusion Proteins
TJP1 protein, human
Tight Junction Proteins
Zonula Occludens-1 Protein
Biotin
Carbon-Nitrogen Ligases

Grants and funding

Intramural NIH HHS/United States