Role of Angiotensin II Type 1a Receptor (AT1aR) of Renal Tubules in Regulating Inwardly Rectifying Potassium Channels 4.2 (Kir4.2), Kir4.1, and Epithelial Na+Channel (ENaC)

Xin Peng Duan; Yu Xiao; Xiao Tong Su; Jun Ya Zheng; Susan Gurley; Jacqueline Emathinger; Chao-Ling Yang; James McCormick; David H. Ellison; Dao Hong Lin; Wen Hui Wang

doi:10.1161/HYPERTENSIONAHA.123.21389

Role of Angiotensin II Type 1a Receptor (AT1aR) of Renal Tubules in Regulating Inwardly Rectifying Potassium Channels 4.2 (Kir4.2), Kir4.1, and Epithelial Na⁺Channel (ENaC)

Xin Peng Duan, Yu Xiao, Xiao Tong Su, Jun Ya Zheng, Susan Gurley, Jacqueline Emathinger, Chao-Ling Yang, James McCormick, David H. Ellison, Dao Hong Lin, Wen Hui Wang

Research output: Contribution to journal › Article › peer-review

Abstract

BACKGROUND: Kir4.2 and Kir4.1 play a role in regulating membrane transport in the proximal tubule (PT) and in the distal-convoluted-tubule (DCT), respectively. METHODS: We generated kidney-tubule-specific-AT1aR-knockout (Ks-AT1aR-KO) mice to examine whether renal AT1aR regulates Kir4.2 and Kir4.1. RESULTS: Ks-AT1aR-KO mice had a lower systolic blood pressure than Agtr1a^flox/flox(control) mice. Ks-AT1aR-KO mice had a lower expression of NHE₃(Na⁺/H⁺-exchanger 3) and Kir4.2, a major Kir-channel in PT, than Agtr1a^flox/floxmice. Whole-cell recording also demonstrated that the membrane potential in PT of Ks-AT1aR-KO mice was lesser negative than Agtr1a^flox/floxmice. The expression of Kir4.1 and Kir5.1, Kir4.1/Kir5.1-mediated K⁺currents of DCT and DCT membrane potential in Ks-AT1aR-KO mice, were similar to Agtr1a^flox/floxmice. However, angiotensin II perfusion for 7 days hyperpolarized the membrane potential in PT and DCT of the control mice but not in Ks-AT1aR-KO mice, while angiotensin II perfusion did not change the expression of Kir4.1, Kir4.2, and Kir5.1. Deletion of AT1aR did not significantly affect the expression of αENaC (epithelial Na⁺channel) and βENaC but increased cleaved γENaC expression. Patch-clamp experiments demonstrated that deletion of AT1aR increased amiloride-sensitive Na⁺-currents in the cortical-collecting duct but not in late-DCT. However, tertiapin-Q sensitive renal outer medullary potassium channel currents were similar in both genotypes. CONCLUSIONS: AT1aR determines the baseline membrane potential of PT by controlling Kir4.2 expression/activity but AT1aR is not required for determining the baseline membrane potential of the DCT and Kir4.1/Kir5.1 activity/expression. However, AT1aR is required for angiotensin II-induced hyperpolarization of basolateral membrane of PT and DCT. Deletion of AT1aR had no effect on baseline renal outer medullary potassium channel activity but increased ENaC activity in the CCD.

Original language	English (US)
Pages (from-to)	126-137
Number of pages	12
Journal	Hypertension
Volume	81
Issue number	1
DOIs	https://doi.org/10.1161/HYPERTENSIONAHA.123.21389
State	Published - Jan 1 2024

Keywords

amiloride
angiotensin II
genotype
knockout mice
perfusion

ASJC Scopus subject areas

Internal Medicine

Access to Document

10.1161/HYPERTENSIONAHA.123.21389

Cite this

Duan, X. P., Xiao, Y., Su, X. T., Zheng, J. Y., Gurley, S., Emathinger, J., Yang, C.-L., McCormick, J., Ellison, D. H., Lin, D. H., & Wang, W. H. (2024). Role of Angiotensin II Type 1a Receptor (AT1aR) of Renal Tubules in Regulating Inwardly Rectifying Potassium Channels 4.2 (Kir4.2), Kir4.1, and Epithelial Na⁺Channel (ENaC). Hypertension, 81(1), 126-137. https://doi.org/10.1161/HYPERTENSIONAHA.123.21389

Duan, XP, Xiao, Y, Su, XT, Zheng, JY, Gurley, S, Emathinger, J, Yang, C-L , McCormick, J , Ellison, DH, Lin, DH & Wang, WH 2024, 'Role of Angiotensin II Type 1a Receptor (AT1aR) of Renal Tubules in Regulating Inwardly Rectifying Potassium Channels 4.2 (Kir4.2), Kir4.1, and Epithelial Na⁺Channel (ENaC)', Hypertension, vol. 81, no. 1, pp. 126-137. https://doi.org/10.1161/HYPERTENSIONAHA.123.21389

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title = "Role of Angiotensin II Type 1a Receptor (AT1aR) of Renal Tubules in Regulating Inwardly Rectifying Potassium Channels 4.2 (Kir4.2), Kir4.1, and Epithelial Na+Channel (ENaC)",

abstract = "BACKGROUND: Kir4.2 and Kir4.1 play a role in regulating membrane transport in the proximal tubule (PT) and in the distal-convoluted-tubule (DCT), respectively. METHODS: We generated kidney-tubule-specific-AT1aR-knockout (Ks-AT1aR-KO) mice to examine whether renal AT1aR regulates Kir4.2 and Kir4.1. RESULTS: Ks-AT1aR-KO mice had a lower systolic blood pressure than Agtr1aflox/flox(control) mice. Ks-AT1aR-KO mice had a lower expression of NHE3(Na+/H+-exchanger 3) and Kir4.2, a major Kir-channel in PT, than Agtr1aflox/floxmice. Whole-cell recording also demonstrated that the membrane potential in PT of Ks-AT1aR-KO mice was lesser negative than Agtr1aflox/floxmice. The expression of Kir4.1 and Kir5.1, Kir4.1/Kir5.1-mediated K+currents of DCT and DCT membrane potential in Ks-AT1aR-KO mice, were similar to Agtr1aflox/floxmice. However, angiotensin II perfusion for 7 days hyperpolarized the membrane potential in PT and DCT of the control mice but not in Ks-AT1aR-KO mice, while angiotensin II perfusion did not change the expression of Kir4.1, Kir4.2, and Kir5.1. Deletion of AT1aR did not significantly affect the expression of αENaC (epithelial Na+channel) and βENaC but increased cleaved γENaC expression. Patch-clamp experiments demonstrated that deletion of AT1aR increased amiloride-sensitive Na+-currents in the cortical-collecting duct but not in late-DCT. However, tertiapin-Q sensitive renal outer medullary potassium channel currents were similar in both genotypes. CONCLUSIONS: AT1aR determines the baseline membrane potential of PT by controlling Kir4.2 expression/activity but AT1aR is not required for determining the baseline membrane potential of the DCT and Kir4.1/Kir5.1 activity/expression. However, AT1aR is required for angiotensin II-induced hyperpolarization of basolateral membrane of PT and DCT. Deletion of AT1aR had no effect on baseline renal outer medullary potassium channel activity but increased ENaC activity in the CCD.",

keywords = "amiloride, angiotensin II, genotype, knockout mice, perfusion",

author = "Duan, {Xin Peng} and Yu Xiao and Su, {Xiao Tong} and Zheng, {Jun Ya} and Susan Gurley and Jacqueline Emathinger and Chao-Ling Yang and James McCormick and Ellison, {David H.} and Lin, {Dao Hong} and Wang, {Wen Hui}",

year = "2024",

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doi = "10.1161/HYPERTENSIONAHA.123.21389",

language = "English (US)",

volume = "81",

pages = "126--137",

journal = "Hypertension",

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publisher = "Lippincott Williams and Wilkins",

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TY - JOUR

T1 - Role of Angiotensin II Type 1a Receptor (AT1aR) of Renal Tubules in Regulating Inwardly Rectifying Potassium Channels 4.2 (Kir4.2), Kir4.1, and Epithelial Na+Channel (ENaC)

AU - Duan, Xin Peng

AU - Xiao, Yu

AU - Su, Xiao Tong

AU - Zheng, Jun Ya

AU - Gurley, Susan

AU - Emathinger, Jacqueline

AU - Yang, Chao-Ling

AU - McCormick, James

AU - Ellison, David H.

AU - Lin, Dao Hong

AU - Wang, Wen Hui

PY - 2024/1/1

Y1 - 2024/1/1

N2 - BACKGROUND: Kir4.2 and Kir4.1 play a role in regulating membrane transport in the proximal tubule (PT) and in the distal-convoluted-tubule (DCT), respectively. METHODS: We generated kidney-tubule-specific-AT1aR-knockout (Ks-AT1aR-KO) mice to examine whether renal AT1aR regulates Kir4.2 and Kir4.1. RESULTS: Ks-AT1aR-KO mice had a lower systolic blood pressure than Agtr1aflox/flox(control) mice. Ks-AT1aR-KO mice had a lower expression of NHE3(Na+/H+-exchanger 3) and Kir4.2, a major Kir-channel in PT, than Agtr1aflox/floxmice. Whole-cell recording also demonstrated that the membrane potential in PT of Ks-AT1aR-KO mice was lesser negative than Agtr1aflox/floxmice. The expression of Kir4.1 and Kir5.1, Kir4.1/Kir5.1-mediated K+currents of DCT and DCT membrane potential in Ks-AT1aR-KO mice, were similar to Agtr1aflox/floxmice. However, angiotensin II perfusion for 7 days hyperpolarized the membrane potential in PT and DCT of the control mice but not in Ks-AT1aR-KO mice, while angiotensin II perfusion did not change the expression of Kir4.1, Kir4.2, and Kir5.1. Deletion of AT1aR did not significantly affect the expression of αENaC (epithelial Na+channel) and βENaC but increased cleaved γENaC expression. Patch-clamp experiments demonstrated that deletion of AT1aR increased amiloride-sensitive Na+-currents in the cortical-collecting duct but not in late-DCT. However, tertiapin-Q sensitive renal outer medullary potassium channel currents were similar in both genotypes. CONCLUSIONS: AT1aR determines the baseline membrane potential of PT by controlling Kir4.2 expression/activity but AT1aR is not required for determining the baseline membrane potential of the DCT and Kir4.1/Kir5.1 activity/expression. However, AT1aR is required for angiotensin II-induced hyperpolarization of basolateral membrane of PT and DCT. Deletion of AT1aR had no effect on baseline renal outer medullary potassium channel activity but increased ENaC activity in the CCD.

AB - BACKGROUND: Kir4.2 and Kir4.1 play a role in regulating membrane transport in the proximal tubule (PT) and in the distal-convoluted-tubule (DCT), respectively. METHODS: We generated kidney-tubule-specific-AT1aR-knockout (Ks-AT1aR-KO) mice to examine whether renal AT1aR regulates Kir4.2 and Kir4.1. RESULTS: Ks-AT1aR-KO mice had a lower systolic blood pressure than Agtr1aflox/flox(control) mice. Ks-AT1aR-KO mice had a lower expression of NHE3(Na+/H+-exchanger 3) and Kir4.2, a major Kir-channel in PT, than Agtr1aflox/floxmice. Whole-cell recording also demonstrated that the membrane potential in PT of Ks-AT1aR-KO mice was lesser negative than Agtr1aflox/floxmice. The expression of Kir4.1 and Kir5.1, Kir4.1/Kir5.1-mediated K+currents of DCT and DCT membrane potential in Ks-AT1aR-KO mice, were similar to Agtr1aflox/floxmice. However, angiotensin II perfusion for 7 days hyperpolarized the membrane potential in PT and DCT of the control mice but not in Ks-AT1aR-KO mice, while angiotensin II perfusion did not change the expression of Kir4.1, Kir4.2, and Kir5.1. Deletion of AT1aR did not significantly affect the expression of αENaC (epithelial Na+channel) and βENaC but increased cleaved γENaC expression. Patch-clamp experiments demonstrated that deletion of AT1aR increased amiloride-sensitive Na+-currents in the cortical-collecting duct but not in late-DCT. However, tertiapin-Q sensitive renal outer medullary potassium channel currents were similar in both genotypes. CONCLUSIONS: AT1aR determines the baseline membrane potential of PT by controlling Kir4.2 expression/activity but AT1aR is not required for determining the baseline membrane potential of the DCT and Kir4.1/Kir5.1 activity/expression. However, AT1aR is required for angiotensin II-induced hyperpolarization of basolateral membrane of PT and DCT. Deletion of AT1aR had no effect on baseline renal outer medullary potassium channel activity but increased ENaC activity in the CCD.

KW - amiloride

KW - angiotensin II

KW - genotype

KW - knockout mice

KW - perfusion

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