Identification and Functional Characterization of an N-terminal Oligomerization Domain for Polycystin-2

Shuang Feng,Genevieve M Okenka,Chang-Xi Bai,Andrew J Streets,Linda J Newby,Brett T Dechant,Leonidas Tsiokas,Tomoko Obara,Albert C.M Ong

doi:10.1074/jbc.m803834200

Abstract

Autosomal dominant polycystic kidney disease (ADPKD), the most common inherited cause of kidney failure, is caused by mutations in either PKD1 (85%) or PKD2 (15%). The PKD2 protein, polycystin-2 (PC2 or TRPP2), is a member of the transient receptor potential (TRP) superfamily and functions as a non-selective calcium channel. PC2 has been found to form oligomers in native tissues suggesting that it may form functional homo- or heterotetramers with other subunits, similar to other TRP channels. Our experiments unexpectedly revealed that PC2 mutant proteins lacking the known C-terminal dimerization domain were still able to form oligomers and co-immunoprecipitate full-length PC2, implying the possible existence of a proximal dimerization domain. Using yeast two-hybrid and biochemical assays, we have mapped an alternative dimerization domain to the N terminus of PC2 (NT2-1-223, L224X). Functional characterization of this domain demonstrated that it was sufficient to induce cyst formation in zebrafish embryos and inhibit PC2 surface currents in mIMCD3 cells probably by a dominant-negative mechanism. In summary, we propose a model for PC2 assembly as a functional tetramer which depends on both C- and N-terminal dimerization domains. These results have significant implications for our understanding of PC2 function and disease pathogenesis in ADPKD and provide a new strategy for studying PC2 function.

Highlights

Autosomal dominant polycystic kidney disease (ADPKD),3 the most common inherited human renal disease, has been shown to result from mutations in either PKD1 or PKD2 (1)
PC2 has been included in the transient receptor potential (TRP) superfamily of channels, which broadly function as cellular sensors for multiple stimuli (4, 5)
PC2 can homodimerize via a C-terminal domain, which is distinct from heterodimerization sequences for PC1 or TRPC1 interactions (5, 15)

Summary

EXPERIMENTAL PROCEDURES

Materials—All chemicals were purchased from Sigma unless otherwise stated. Yeast vectors pGBAD-B and pACT2-B were obtained from D. A C-terminal HA-tagged PKD2 mutant construct, R742X, was generated by PCR using the wild-type PKD2Pk plasmid as a template including the HA epitope tag sequence and in-frame stop codon in the reverse primer. Yeast Two-hybrid Assays—Yeast two-hybrid assays were performed in the yeast strain AH109 containing ADE2, HIS3, and LacZ reporter genes under the control of the GAL4 upstream activating sequences (UAS) by co-transforming bait and prey constructs of the entire intracellular N terminus of human PC2 (NT2) or its truncations into yeast cells using a published protocol (20). Sections were stained with 1:1000 DAPI (KPL) solution for 3 min at room temperature, the slides rinsed once with PBS and mounted with fluorescent mounting medium (KPL).

RESULTS

Human PKD2-D511V

DISCUSSION