PDZK1: I. A major scaffolder in brush borders of proximal tubular cells

被引:137
作者
Gisler, SM
Pribanic, S
Bacic, D
Forrer, P
Gantenbein, A
Sabourin, LA
Tsuji, A
Zhao, ZS
Manser, E
Biber, J
Murer, H
机构
[1] Univ Zurich, Inst Physiol, Dept Physiol & Biochem, CH-8057 Zurich, Switzerland
[2] Univ Ottawa, Neurosci Res Inst, Ottawa, ON, Canada
[3] Univ Ottawa, Dept Cellular & Mol Med, Ottawa, ON, Canada
[4] Kanazawa Univ, Fac Pharmaceut Sci, Kanazawa, Ishikawa 920, Japan
[5] Natl Univ Singapore, Inst Mol & Cell Biol, Glaxo IMCB Lab, Singapore 117548, Singapore
关键词
renal transport of phosphate; NaPi-IIa; NaPi-I; PDZK1; NHERF-1; D-AKAP2; PDZ proteins; MAP17; URAT1; CFEX; yeast two-hybrid;
D O I
10.1046/j.1523-1755.2003.00266.x
中图分类号
R5 [内科学]; R69 [泌尿科学(泌尿生殖系疾病)];
学科分类号
1002 ; 100201 ;
摘要
Background. In proximal tubular cells, PDZK1 (NaPi-Cap1) has been implicated in apical expression of the Na+-dependent phosphate cotransporter (NaPi-IIa) via interaction with its C-terminus. PDZK1 represents a multidomain protein consisting of four PDZ domains and thus is believed to have a broader specificity besides NaPi-IIa. Methods. We subjected single PDZ domains derived from PDZK1 either to yeast two-hybrid screens or yeast trap assays. Different pull-down assays and blot overlays were applied to corroborate the PDZK1-mediated interactions in vitro. Co-localization of interacting proteins with PDZK1 in proximal tubular cells was assessed by immunohistochemistry. Results. In the yeast screens, the most abundant candidate protein to interact with PDZK1 was the membrane-associated protein of 17 kD (MAP17). Besides MAP17, C-terminal parts of following transporters were also identified: NaPi-IIa, solute carrier SLC17A1 (NaPi-I), Na+/H+ exchanger (NHE-3), organic cation transporter (OCTN1), chloride-formate exchanger (CFEX), and urate-anion exchanger (URAT1). In addition, other regulatory factors were found among the clones, such as a protein kinase A (PKA)-anchoring protein (D-AKAP2) and N+/H+ exchanger regulator factor (NHERF-1). All interactions of itemized proteins with PDZK1 were affirmed by in vitro techniques. Apart from PDZK1, strong in vitro interactions of NHERF-1 were also observed with the solute transporters (excluding MAP17) and D-AKAP2. All identified proteins were immunolocalized in proximal tubular cells, wherein all membrane proteins co-localized with PDZK1 in brush borders. Conclusion. We hypothesize that PDZK1 and NHERF-1 establish an extended network beneath the apical membrane to which membrane proteins and regulatory components are anchored.
引用
收藏
页码:1733 / 1745
页数:13
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