SEMA7AR148W mutation promotes lipid accumulation and NAFLD progression via increased localization on the hepatocyte surface
Nan Zhao, Xiaoxun Zhang, Jingjing Ding, Qiong Pan, Ming-Hua Zheng, Wen-Yue Liu, Gang Luo, Jiaquan Qu, Mingqiao Li, Ling Li, Ying Cheng, Ying Peng, Qiaoling Xie, Qinglin Wei, Qiao Li, Lingyun Zou, Xinshou Ouyang, Shi-Ying Cai, James L. Boyer, Jin Chai
Nan Zhao, Xiaoxun Zhang, Jingjing Ding, Qiong Pan, Ming-Hua Zheng, Wen-Yue Liu, Gang Luo, Jiaquan Qu, Mingqiao Li, Ling Li, Ying Cheng, Ying Peng, Qiaoling Xie, Qinglin Wei, Qiao Li, Lingyun Zou, Xinshou Ouyang, Shi-Ying Cai, James L. Boyer, Jin Chai
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Research Article Hepatology Metabolism

SEMA7AR148W mutation promotes lipid accumulation and NAFLD progression via increased localization on the hepatocyte surface

Abstract

Genetic polymorphisms are associated with the development of nonalcoholic fatty liver disease (NAFLD). Semaphorin7a (Sema7a) deficiency in mouse peritoneal macrophages reduces fatty acid (FA) oxidation. Here, we identified 17 individuals with SEMA7A heterozygous mutations in 470 patients with biopsy-proven NAFLD. SEMA7A heterozygous mutations increased susceptibility to NAFLD, steatosis severity, and NAFLD activity scores in humans and mice. The Sema7aR145W mutation (equivalent to human SEMA7AR148W) significantly induced small lipid droplet accumulation in mouse livers compared with WT mouse livers. Mechanistically, the Sema7aR145W mutation increased N-glycosylated Sema7a and its receptor integrin β1 proteins in the cell membranes of hepatocytes. Furthermore, Sema7aR145W mutation enhanced its protein interaction with integrin β1 and PKC-α and increased PKC-α phosphorylation, which were both abrogated by integrin β1 silencing. Induction of PKCα_WT, but not PKCα_dominant negative, overexpression induced transcriptional factors Srebp1, Chrebp, and Lxr expression and their downstream Acc1, Fasn, and Cd36 expression in primary mouse hepatocytes. Collectively, our findings demonstrate that the SEMA7AR148W mutation is a potentially new strong genetic determinant of NAFLD and promotes intrahepatic lipid accumulation and NAFLD in mice by enhancing PKC-α–stimulated FA and triglyceride synthesis and FA uptake. The inhibition of hepatic PKC-α signaling may lead to novel NAFLD therapies.

Authors

Nan Zhao, Xiaoxun Zhang, Jingjing Ding, Qiong Pan, Ming-Hua Zheng, Wen-Yue Liu, Gang Luo, Jiaquan Qu, Mingqiao Li, Ling Li, Ying Cheng, Ying Peng, Qiaoling Xie, Qinglin Wei, Qiao Li, Lingyun Zou, Xinshou Ouyang, Shi-Ying Cai, James L. Boyer, Jin Chai

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Figure 5

The Sema7aR145W mutation enhances hepatic FA and TG synthesis and FA uptake by enhancing PKC-α signaling–stimulated expression of transcription factors Srebp1 and Chrebp and nuclear receptor Lxr.

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The Sema7aR145W mutation enhances hepatic FA and TG synthesis and FA upt...
(A) Western blot analysis of the relative levels of Srebp1, Chrebp, Lxr, phosphorylated PKC-α, and PKC-α protein expression in 10-week-old male WT mice (n = 4), Sema7aR145W heterozygous mice (n = 5), and Sema7aR145W homozygous mice (n = 5). Western blot analysis of the relative levels of nuclear Srebp1, Chrebp, and Lxr proteins in primary hepatocytes from WT and Sema7aR145W homozygous mice (B) and in human hepatoma HepG2 cells (C) after transfection with the plasmid for the expression of SEMA7A_WT and SEMA7A_R148W proteins. (D) Representative Western blot of the relative levels of nuclear Srebp1, Chrebp, and Lxr proteins in nuclear extracts and (E) Fasn, Acc1, and Cd36 proteins in whole-cell lysates of primary mouse hepatocytes after transfection with empty vector (CTR) or the plasmid for the expression of PKCα_WT or PKCα_dominant negative (DN) mutant, respectively. All primary mouse hepatocytes were isolated from 12-week-old male WT and Sema7aR145W homozygous mice. Data are representative images or expressed as the mean ± SD of each group from 3 separate experiments. The data were analyzed by 1-way ANOVA with Tukey’s post hoc tests or by Kruskal-Wallis test with Dunn’s post hoc test analysis. *P < 0.05 versus the WT mice, #P < 0.05 versus the Sema7aR145W heterozygous mice, $P < 0.05 versus the primary HO mouse hepatocytes transfected with CTR; n = 3.