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Elevated CCL2 causes Leydig cell malfunction in metabolic syndrome
Qingkui Jiang, Constanze C. Maresch, Sebastian Friedrich Petry, Agnieszka Paradowska-Dogan, Sudhanshu Bhushan, Yongsheng Chang, Christine Wrenzycki, Hans-Christian Schuppe, Petr Houska, Michaela F. Hartmann, Stefan A. Wudy, Lanbo Shi, Thomas Linn
Qingkui Jiang, Constanze C. Maresch, Sebastian Friedrich Petry, Agnieszka Paradowska-Dogan, Sudhanshu Bhushan, Yongsheng Chang, Christine Wrenzycki, Hans-Christian Schuppe, Petr Houska, Michaela F. Hartmann, Stefan A. Wudy, Lanbo Shi, Thomas Linn
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Research Article Endocrinology Reproductive biology

Elevated CCL2 causes Leydig cell malfunction in metabolic syndrome

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Abstract

Metabolic syndrome (MetS), which is associated with chronic inflammation, predisposes males to hypogonadism and subfertility. The underlying mechanism of these pathologies remains poorly understood. Homozygous leptin-resistant obese db/db mice are characterized by small testes, low testicular testosterone, and a reduced number of Leydig cells. Here we report that IL-1β, CCL2 (also known as MCP-1), and corticosterone concentrations were increased in the testes of db/db mice relative to those in WT controls. Cultured murine and human Leydig cells responded to cytokine stress with increased CCL2 release and apoptotic signals. Chemical inhibition of CCL2 rescued Leydig cell function in vitro and in db/db mice. Consistently, we found that Ccl2-deficient mice fed with a high-energy diet were protected from testicular dysfunction compared with similarly fed WT mice. Finally, a cohort of infertile men with a history of MetS showed that reduction of CCL2 plasma levels could be achieved by weight loss and was clearly associated with recovery from hypogonadism. Taken together, we conclude that CCL2-mediated chronic inflammation is, to a large extent, responsible for the subfertility in MetS by causing damage to Leydig cells.

Authors

Qingkui Jiang, Constanze C. Maresch, Sebastian Friedrich Petry, Agnieszka Paradowska-Dogan, Sudhanshu Bhushan, Yongsheng Chang, Christine Wrenzycki, Hans-Christian Schuppe, Petr Houska, Michaela F. Hartmann, Stefan A. Wudy, Lanbo Shi, Thomas Linn

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Figure 2

db/db mice showed impaired expression of specific Leydig cell products.

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db/db mice showed impaired expression of specific Leydig cell products....
(A and B) H&E (A) and insulin-like 3 (INSL3) (B) staining on representative testicular sections; scale bar: 20 μm. (C and D) Protein expression of INSL3 (C) and STAR (D), respectively, as analyzed by Western blot. (E) mRNA levels of steroidogenic genes in WT and db/db mice. (F and G) Mean testosterone levels in serum (F) and testicular interstitial fluid (TIF) (G). Data given in C–G were from n = 3–8 mice, 12–24 weeks old, in each group. Data are shown as means ± SEM. Student’s 2-tailed t test was used to compare means between 2 groups. *P < 0.05, **P < 0.01, ***P < 0.001, ****P < 0.0001.

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