Structure-Function Studies of Claudin Extracellular Domains by Cysteine-scanning Mutagenesis

Claudins form size- and charge-selective pores in the tight junction that control the paracellular flux of inorganic ions and small molecules. However, the structural basis for ion selectivity of paracellular pores is poorly understood. Here we applied cysteine scanning to map the paracellular pathway of ion permeation across claudin-2-transfected Madin-Darby canine kidney type I cells. Four potential pore-lining amino acid residues in the first extracellular loop were mutated to cysteine and screened for their accessibility to thiol-reactive reagents. All mutants were functional except D65C, which formed dimers by intermolecular disulfide bonding, leading to a loss of charge and size selectivity. This suggests that claudin-2 pores are multimeric and that Asp⁶⁵ lies close to a protein-protein interface. Methanethiosulfonate reagents of different size and charge and the organic mercury derivate, p-(chloromercuri)benzenesulfonic acid, significantly decreased paracellular ion permeation across I66C-transfected cells by a mechanism that suggests steric blocking of the pore. The conductance of wild-type claudin-2 and the other cysteine mutants was only weakly affected. The rate of reaction with I66C decreased dramatically with increasing size of the reagent, suggesting that Ile⁶⁶ is buried deep within a narrow segment of the pore with its side group facing into the lumen. Furthermore, labeling with N-biotinoylaminoethyl methanethiosulfonate showed that I66C was weakly reactive, whereas Y35C was strongly reactive, suggesting that Tyr³⁵ is located at the protein surface outside of the pore.Sheets of polarized epithelia constitute barriers that separate fluid compartments of different chemical composition and mediate exchange of solutes and ions via transcellular and paracellular pathways. A large body of evidence suggests that transport via the paracellular pathway occurs through pores in the tight junctions that are formed by tetraspan membrane proteins, known as claudins (1–3).Our current understanding of paracellular pores is that they are size- and charge-selective water-filled channels that, in contrast to channels for transmembrane transport, are oriented parallel instead of perpendicular to the lipid layer of the cell membrane. Size exclusion experiments suggest a pore diameter of 6.4–8 ? (4, 5). Furthermore, site-directed mutagenesis and overexpression of claudins in epithelial cells identified the first extracellular domain as playing an important role in the charge selectivity of paracellular transport (6–8). The first extracellular domain of claudins contains various basic and acidic amino acids, some of which are conserved in different claudin isoforms, and these could be involved in the mechanism of ion permeation. Several studies have demonstrated homo- or heterotypic interaction of claudins, suggesting that paracellular pores are formed by oligomers of claudins (9–11). Taken together, significant progress has been made in uncovering the nature of the paracellular pathway and mechanisms of selectivity of paracellular ion permeation. However, it is unknown how the extracellular domains of claudins fold to form paracellular pores and which amino acid residues line the pathway of ion diffusion.Epithelia in vivo and epithelial cell lines express characteristic sets of different claudin isoforms that determine paracellular permeability and permselectivity. Claudin-2 is expressed in epithelia with a high capacity for passive paracellular cation transport, such as the epithelium lining the proximal renal tubules (12). The transfection of claudin-2 into high resistance Madin-Darby canine kidney (MDCK)² type I cells converts the tight junction from a “tight” into a “leaky” paracellular barrier by selectively increasing Na⁺ permeability (13, 14), suggesting a physiologic role of claudin-2 in creating paracellular Na⁺ channels. Because of the high signal/noise ratio of the claudin-2-induced permeability, this isoform provides an excellent model to study paracellular transport. We have recently generated a stable expression system of claudin-2 in MDCK I cells under the control of a TetOff promoter. This inducible system allows us to specifically determine the macroscopic conductance and permeability of claudin-2 pores by subtracting background measurements of uninduced cells. Using this expression system, we could recently demonstrate that the cation selectivity of claudin-2 cells is mediated by electrostatic interaction of partially dehydrated permeating cations with aspartate 65 (5). However, further investigations are necessary to study the position and function of this and other residues of the first extracellular domain and to elucidate their role in the transport mechanism of paracellular pores.The substituted cysteine accessibility method (SCAM), developed by the Karlin group, has proved to be a powerful tool in the mapping of the structures of membrane ion channels and transport proteins (15, 16). In SCAM, thiol-reactive reagents are used to covalently modify endogenous cysteines, or cysteines introduced into a protein by site-directed mutagenesis. SCAM can be used to study channel-lining amino acid side chains, the secondary structures of membrane-spanning segments, and the localization of selectivity filters, channel gates, and inhibitor binding sites.Here, we used SCAM to analyze the paracellular pathway of ion permeation across claudin-2 transfected MDCK I cells. Our data show that thiol-reactive reagents strongly block ion transport in at least one of the cysteine mutants that we have generated and, thus, provide a tool to map residues that line the paracellular pore.