Aldehyde dehydrogenase 2 preserves kidney function by countering acrolein-induced metabolic and mitochondrial dysfunction
Szu-Yuan Li, Ming-Tsun Tsai, Yu-Ming Kuo, Hui-Min Yang, Zhen-Jie Tong, Hsiao-Wei Cheng, Chih-Ching Lin, Hsiang-Tsui Wang
Szu-Yuan Li, Ming-Tsun Tsai, Yu-Ming Kuo, Hui-Min Yang, Zhen-Jie Tong, Hsiao-Wei Cheng, Chih-Ching Lin, Hsiang-Tsui Wang
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Research Article Metabolism Nephrology

Aldehyde dehydrogenase 2 preserves kidney function by countering acrolein-induced metabolic and mitochondrial dysfunction

Abstract

The prevalence of chronic kidney disease (CKD) varies by race because of genetic and environmental factors. The Glu504Lys polymorphism in aldehyde dehydrogenase 2 (ALDH2), commonly observed among East Asian people, alters the enzyme’s function in detoxifying alcohol-derived aldehydes, affecting kidney function. This study investigated the association between variations in ALDH2 levels within the kidney and the progression of kidney fibrosis. Our clinical data indicate that diminished ALDH2 levels are linked to worse CKD outcomes, with correlations between ALDH2 expression, estimated glomerular filtration rate, urinary levels of acrolein — an aldehyde metabolized by ALDH2 — and fibrosis severity. In mouse models of unilateral ureteral obstruction and folic acid nephropathy, reduced ALDH2 levels and elevated acrolein were observed in kidneys, especially in ALDH2 Glu504Lys–knockin mice. Mechanistically, acrolein modifies pyruvate kinase M2, leading to its nuclear translocation and coactivation of HIF-1α, shifting cellular metabolism to glycolysis, disrupting mitochondrial function, and contributing to tubular damage and the progression of kidney fibrosis. Enhancing ALDH2 expression through adeno-associated virus vectors reduced acrolein and mitigated fibrosis in both WT and Glu504Lys-knockin mice. These findings underscore the potential therapeutic significance of targeting the dynamic interaction between ALDH2 and acrolein in CKD.

Authors

Szu-Yuan Li, Ming-Tsun Tsai, Yu-Ming Kuo, Hui-Min Yang, Zhen-Jie Tong, Hsiao-Wei Cheng, Chih-Ching Lin, Hsiang-Tsui Wang

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Figure 5

Assessment of Acr-PCs, fibrosis markers, inflammatory cytokines, and kidney damage markers in Aldh2*1/*2 and Aldh2*2/*2 mice compared with Aldh2*1 mice after FAN.

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Assessment of Acr-PCs, fibrosis markers, inflammatory cytokines, and kid...
WT, Aldh2*1/*2, and Aldh2*2/*2 mice (n = 5 for each group) were intraperitoneally administered folic acid (FA) (225 mg/kg in 300 mM NaHCO3) and sacrificed on day 28. (A) The upper panel displays the gross appearance of representative kidneys, while the lower panel presents the statistical analysis of the kidney-to-body weight ratio. (B) H&E and periodic acid–Schiff (PAS) staining are shown in the first and second panels to assess morphological changes in kidney tissues. Sirius red staining to evaluate the kidney fibrosis area on day 28 after FA injection is depicted in the third panel. Immunohistochemistry for Acr-PC in kidney tissues is presented in the fourth panel. Scale bar: 50 μm. The upper panel displays Western blot analysis of (C) Acr-PCs, (D) collagen 1, α–smooth muscle actin (α-SMA), and ALDH2 in kidney tissues of mice, with quantification of these proteins shown in the lower panel. mRNA expression of (E) Col1a1, Acta2, (F) Havcr1, Lcn2, and (G) Il6 and Il1b in kidney tissues of mice was assessed using quantitative reverse transcription PCR analysis. Data are presented as mean ± SD. Statistical significance was determined using Kruskal-Wallis tests, and 2-tailed P values are shown. *P < 0.05, **P < 0.01, ***P < 0.001 compared with the WT group. Acr-PCs, acrolein-protein conjugates; ALDH2, aldehyde dehydrogenase 2; WT, wild-type; FAN, folic acid nephropathy; Acta2, actin alpha 2; Aldh2, aldehyde dehydrogenase 2; Col1a1, collagen type I alpha 1 chain; Havcr1, hepatitis A virus cellular receptor 1 homolog; Il6, interleukin-6, Il1b, interleukin-1β; Lcn2, lipocalin-2.