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The ARH adaptor protein regulates endocytosis of the ROMK potassium secretory channel in mouse kidney
Liang Fang, … , James B. Wade, Paul A. Welling
Liang Fang, … , James B. Wade, Paul A. Welling
Published October 19, 2009
Citation Information: J Clin Invest. 2009;119(11):3278-3289. https://doi.org/10.1172/JCI37950.
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Research Article Nephrology

The ARH adaptor protein regulates endocytosis of the ROMK potassium secretory channel in mouse kidney

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Abstract

Renal outer medullary potassium (ROMK) channels are exquisitely regulated to adjust renal potassium excretion and maintain potassium balance. Clathrin-dependent endocytosis plays a critical role, limiting urinary potassium loss in potassium deficiency. In renal disease, aberrant ROMK endocytosis may contribute to potassium retention and hyperkalemia. Previous work has indicated that ROMK endocytosis is stimulated by with-no-lysine (WNK) kinases, but the endocytotic signal and the internalization machinery have not been defined. Here, we found that ROMK bound directly to the clathrin adaptor molecule autosomal recessive hypercholesterolemia (ARH), and this interaction was mediated by what we believe to be a novel variant of the canonical “NPXY” endocytotic signal, YxNPxFV. ARH recruits ROMK to clathrin-coated pits for constitutive and WNK1-stimuated endocytosis, and ARH knockdown decreased basal rates of ROMK endocytosis, in a heterologous expression system, COS-7 cells. We found that ARH was predominantly expressed in the distal nephron where it coimmunoprecipitated and colocalized with ROMK. In mice, the abundance of kidney ARH protein was modulated by dietary potassium and inversely correlated with changes in ROMK. Furthermore, ARH-knockout mice exhibited an altered ROMK response to potassium intake. These data suggest that ARH marks ROMK for clathrin-dependent endocytosis, in concert with the demands of potassium homeostasis.

Authors

Liang Fang, Rita Garuti, Bo-Young Kim, James B. Wade, Paul A. Welling

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Figure 8

L-WNK1 stimulates ROMK endocytosis through an ARH-dependent mechanism.

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L-WNK1 stimulates ROMK endocytosis through an ARH-dependent mechanism.
R...
ROMK endocytosis was measured by biotinylation in COS-7 cells expressing either WT ARH (myc tagged, left column) or the dominant-negative ARH (myc-ARH1–187) (right column) in the presence (+) or absence (-) of exogenous L-WNK1 (amino acids 1–491). (A) Representative experiment showing surface biotinylated ROMK channels that have become internalized after a 5-minute chase compared with the total surface pool (detected by immunoblot with anti-ROMK antibodies). (B) Quantification of ROMK endocytosis in cells cotransfected either WT ARH or ARH1–187 and empty vector (white bars) or the active fragment of L-WNK1 (black bars) (n = 3). In the presence of WT ARH, L-WNK1 stimulated ROMK endocytosis. (*P < 0.001). The response was completely suppressed by the dominant-negative ARH. Dominant-negative ARH also suppressed constitutive ROMK endocytosis (#P < 0.05).

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ISSN: 0021-9738 (print), 1558-8238 (online)

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