LRG1 is an adipokine that mediates obesity-induced hepatosteatosis and insulin resistance
Sijia He, … , Juli Bai, Lily Q. Dong
Sijia He, … , Juli Bai, Lily Q. Dong
Published November 2, 2021
Citation Information: J Clin Invest. 2021;131(24):e148545. https://doi.org/10.1172/JCI148545.
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Research Article Endocrinology Metabolism

LRG1 is an adipokine that mediates obesity-induced hepatosteatosis and insulin resistance

Abstract

Dysregulation in adipokine biosynthesis and function contributes to obesity-induced metabolic diseases. However, the identities and functions of many of the obesity-induced secretory molecules remain unknown. Here, we report the identification of leucine-rich alpha-2-glycoprotein 1 (LRG1) as an obesity-associated adipokine that exacerbates high fat diet–induced hepatosteatosis and insulin resistance. Serum levels of LRG1 were markedly elevated in obese humans and mice compared with their respective controls. LRG1 deficiency in mice greatly alleviated diet-induced hepatosteatosis, obesity, and insulin resistance. Mechanistically, LRG1 bound with high selectivity to the liver and promoted hepatosteatosis by increasing de novo lipogenesis and suppressing fatty acid β-oxidation. LRG1 also inhibited hepatic insulin signaling by downregulating insulin receptor substrates 1 and 2. Our study identified LRG1 as a key molecule that mediates the crosstalk between adipocytes and hepatocytes in diet-induced hepatosteatosis and insulin resistance. Suppressing LRG1 expression and function may be a promising strategy for the treatment of obesity-related metabolic diseases.

Authors

Sijia He, Jiyoon Ryu, Juanhong Liu, Hairong Luo, Ying Lv, Paul R. Langlais, Jie Wen, Feng Dong, Zhe Sun, Wenjuan Xia, Jane L. Lynch, Ravindranath Duggirala, Bruce J. Nicholson, Mengwei Zang, Yuguang Shi, Fang Zhang, Feng Liu, Juli Bai, Lily Q. Dong

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Figure 4

Identification of liver as a major target tissue of LRG1.

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Identification of liver as a major target tissue of LRG1. (A) Binding of...
(A) Binding of SEAP or SEAP-LRG1 to frozen tissue sections prepared from male C57BL/6J mice (scale bar: 1000 μm for brain and liver, 500 μm for muscle, kidney, and heart). (B) Binding of SEAP-LRG1 to liver tissue with or without preincubation of purified Myc-His-tagged recombinant LRG1 (scale bar: 1000 μm). (C) Biodistribution of LRG1 in vivo 16 hours after i.v. injection. Organs isolated from mice injected with Vivo tag680 (Tag) or Vivo Tag680-LRG1(Tag-LRG1) were subjected to Epi-luminescence imaging (n = 3/group). The color bar indicates the intensity of florescence signal based on radiance values (photons/second/cm2/steradian). (D) Quantification of LRG1 in vivo biodistribution 16 hours after i.v. injection, data were calculated based on radiance values of each tissue (photons/second/cm2/steradian). (E) Epi-luminescence imaging measurement of biodistribution of LRG1 in vivo 48 hours after i.v. injection (n = 3 per group). (F) Quantification of LRG1 in vivo biodistribution 48 hours after i.v. injection. Data in A, B, C, and E are representative of 3 independent experiments. Data in D and F represent mean ± SEM. Unpaired 2-tailed t test, *P ≤ 0.05, **P ≤ 0.01, ***P ≤ 0.001.