Assembly of Tight Junction Strands: Claudin-10b and Claudin-3 Form Homo-Tetrameric Building Blocks that Polymerise in a Channel-Independent Manner

C Hempel; J Protze; E Altun; B Riebe; A Piontek; A Fromm; I M Lee; T Saleh; D Günzel; G Krause; J Piontek

doi:10.1016/j.jmb.2020.02.034

Assembly of Tight Junction Strands: Claudin-10b and Claudin-3 Form Homo-Tetrameric Building Blocks that Polymerise in a Channel-Independent Manner

J Mol Biol. 2020 Mar 27;432(7):2405-2427. doi: 10.1016/j.jmb.2020.02.034. Epub 2020 Mar 4.

Authors

C Hempel¹, J Protze², E Altun¹, B Riebe¹, A Piontek², A Fromm¹, I M Lee¹, T Saleh¹, D Günzel¹, G Krause², J Piontek³

Affiliations

¹ Charité - Universitätsmedizin Berlin, Institute of Clinical Physiology, Hindenburgdamm 30, 12203 Berlin, Germany.
² Leibniz-Forschungsinstitut für Molekulare Pharmakologie (FMP), Robert-Rössle-Straße 10, 13125 Berlin, Germany.
³ Charité - Universitätsmedizin Berlin, Institute of Clinical Physiology, Hindenburgdamm 30, 12203 Berlin, Germany. Electronic address: joerg.piontek@charite.de.

PMID: 32142789
DOI: 10.1016/j.jmb.2020.02.034

Abstract

Tight junctions regulate paracellular permeability size and charge selectively. Models have been proposed for the molecular architecture of tight junction strands and paracellular channels. However, they are not fully consistent with experimental and structural data. Here, we analysed the architecture of claudin-based tight junction strands and channels by cellular reconstitution of strands, structure-guided mutagenesis, in silico protein docking and oligomer modelling. Prototypic channel- (Cldn10b) and barrier-forming (Cldn3) claudins were analysed. Förster resonance energy transfer (FRET) assays indicated multistep claudin polymerisation, starting with cis-oligomerization specific to the claudin subtype, followed by trans-interaction-triggered cis-polymerisation. Alternative protomer interfaces were modelled in silico and tested by cysteine-mediated crosslinking, confocal- and freeze fracture EM-based analysis of strand formation. The analysed claudin mutants included also mutations causing the HELIX syndrome. The results indicated that protomers in Cldn10b and Cldn3 strands form similar antiparallel double rows, as has been suggested for Cldn15. Mutually stabilising -hydrophilic and hydrophobic - cis- and trans-interfaces were identified that contained novel key residues of extracellular segments ECS1 and ECS2. Hydrophobic clustering of the flexible ECS1 β1β2 loops together with ECS2-ECS2 trans-interaction is suggested to be the driving force for conjunction of tetrameric building blocks into claudin polymers. Cldn10b and Cldn3 are indicated to share this polymerisation mechanism. However, in the paracellular centre of tetramers, electrostatic repulsion may lead to formation of pores (Cldn10b) and electrostatic attraction to barriers (Cldn3). Combining in vitro data and in silico modelling, this study improves mechanistic understanding of paracellular permeability regulation by elucidating claudin assembly and its pathologic alteration as in HELIX syndrome.

Keywords: barrier; modelling; oligomerisation; paracellular permeability; pore.

Publication types

Research Support, Non-U.S. Gov't

MeSH terms

Animals
Cell Membrane Permeability
Claudin-3 / chemistry*
Claudin-3 / genetics
Claudin-3 / metabolism
Claudins / chemistry*
Claudins / genetics
Claudins / metabolism
HEK293 Cells
Humans
Ion Channels
Mice
Mutation
Protein Conformation
Protein Multimerization*
Syndrome
Tight Junctions / chemistry*
Tight Junctions / metabolism

Substances

Claudin-3
Claudins
Cldn3 protein, mouse
Ion Channels
claudin 10