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 Homo- and heterotetrameric architecture of the epithelial Ca2+ channels TRPV5 and  TRPV6 Hoenderop JG; Voets T; Hoefs S; Weidema F; Prenen J; Nilius B; Bindels RJEMBO J  2003[Feb]; 22 (4): 776-85The molecular assembly of the epithelial Ca(2+) channels (TRPV5 and TRPV6) was  investigated to determine the subunit stoichiometry and composition. Immunoblot  analysis of Xenopus laevis oocytes expressing TRPV5 and TRPV6 revealed two  specific bands of 75 and 85-100 kDa, corresponding to the core and glycosylated  proteins, respectively, for each channel. Subsequently, membranes of these  oocytes were sedimented on sucrose gradients. Immuno blotting revealed that TRPV5  and TRPV6 complexes migrate with a mol. wt of 400 kDa, in line with a tetrameric  structure. The tetrameric stoichiometry was confirmed in an electrophysiological  analysis of HEK293 cells co-expressing concatemeric channels together with a  TRPV5 pore mutant that reduced Cd(2+) sensitivity and voltage-dependent gating.  Immuno precipitations using membrane fractions from oocytes co-expressing TRPV5  and TRPV6 demonstrated that both channels can form heteromeric complexes.  Expression of all possible heterotetrameric TRPV5/6 complexes in HEK293 cells  resulted in Ca(2+) channels that varied with respect to Ca(2+)-dependent  inactivation, Ba(2+) selectivity and pharmacological block. Thus,  Ca(2+)-transporting epithelia co-expressing TRPV5 and TRPV6 can generate a  pleiotropic set of functional heterotetrameric channels with different Ca(2+)  transport kinetics.|Animals[MESH]|Calcium Channels/*chemistry/metabolism[MESH]|Calcium/*metabolism[MESH]|Epithelium/chemistry/*metabolism[MESH]|Kidney/chemistry/metabolism[MESH]|Mice[MESH]|Precipitin Tests[MESH]|Protein Structure, Tertiary[MESH]|TRPV Cation Channels[MESH]
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