Neurosteroid [3α,5α]3-hydroxypregnan-20-one inhibition of chemokine monocyte chemoattractant protein-1 in alcohol-preferring rat brain neurons, microglia, and astroglia

IF 3 Q2 SUBSTANCE ABUSE Alcohol (Hanover, York County, Pa.) Pub Date : 2024-07-11 DOI:10.1111/acer.15404

Samantha Lucenell Chéry, Todd K. O'Buckley, Giorgia Boero, Irina Balan, A. Leslie Morrow

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Abstract

Background

Neuroimmune dysfunction in alcohol use disorder (AUD) is associated with activation of myeloid differentiation primary response 88 (MyD88)-dependent Toll-like receptors (TLR) resulting in overexpression of the chemokine monocyte chemoattractant protein-1 (MCP-1/CCL2). MCP-1 overexpression in the brain is linked to anxiety, higher alcohol intake, neuronal death, and activation of microglia observed in AUD. The neurosteroid [3α,5α][3-hydroxypregnan-20-one (3α,5α-THP) has been reported as an inhibitor of MyD88-dependent TLR activation and MCP-1 overexpression in mouse and human macrophages and the brain of alcohol-preferring (P) rats.

Methods

We investigated how 3α,5α-THP regulates MCP-1 expression at the cellular level in P rat nucleus accumbens (NAc) and central amygdala (CeA). We focused on neurons, microglia, and astrocytes, examining the individual voxel density of MCP-1, neuronal marker NeuN, microglial marker IBA1, astrocytic marker GFAP, and their shared voxel density, defined as intersection. Ethanol-naïve male and female P rats were perfused 1 h after IP injections of 15 mg/kg of 3α,5α-THP, or vehicle. The NAc and CeA were imaged using confocal microscopy following double-immunofluorescence staining for MCP-1 with NeuN, IBA1, and GFAP, respectively.

Results

MCP-1 intersected with NeuN predominantly and IBA1/GFAP negligibly. 3α,5α-THP reduced MCP-1 expression in NeuN-labeled cells by 38.27 ± 28.09% in male and 56.11 ± 21.46% in female NAc, also 37.99 ± 19.53% in male and 54.96 ± 30.58% in female CeA. In females, 3α,5α-THP reduced the MCP-1 within IBA1 and GFAP-labeled voxels in the NAc and CeA. Conversely, in males, 3α,5α-THP did not significantly alter the MCP-1 within IBA1 in NAc or with GFAP in the CeA. Furthermore, 3α,5α-THP decreased levels of IBA1 in both regions and sexes with no impact on GFAP or NeuN levels. Secondary analysis performed on data normalized to % control values indicated that no significant sex differences were present.

Conclusions

These data suggest that 3α,5α-THP inhibits neuronal MCP-1 expression and decreases the proliferation of microglia in P rats. These results increase our understanding of potential mechanisms for 3α,5α-THP modulation of ethanol consumption.

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神经类固醇[3α,5α]3-羟基孕甾-20-酮对酒精偏爱型大鼠脑神经元、小胶质细胞和星形胶质细胞中趋化因子单核细胞趋化蛋白-1的抑制作用。

背景：酒精使用障碍（AUD）的神经免疫功能障碍与依赖于Toll样受体（TLR）的髓样分化初级反应88（MyD88）的激活有关，导致趋化因子单核细胞趋化蛋白-1（MCP-1/CCL2）的过度表达。MCP-1 在大脑中的过度表达与焦虑、酒精摄入量增加、神经元死亡以及在 AUD 中观察到的小胶质细胞活化有关。据报道，神经类固醇[3α,5α][3-hydroxypregnan-20-one (3α,5α-THP)是小鼠、人类巨噬细胞和酒精偏好（P）大鼠大脑中 MyD88 依赖性 TLR 激活和 MCP-1 过度表达的抑制剂：方法：我们研究了 3α,5α-THP如何在细胞水平上调节酒精偏爱型大鼠脑核（NAc）和中央杏仁核（CeA）中 MCP-1 的表达。我们重点研究了神经元、小胶质细胞和星形胶质细胞，检测了 MCP-1、神经元标记物 NeuN、小胶质细胞标记物 IBA1 和星形胶质细胞标记物 GFAP 的单个体节密度以及它们的共同体节密度（定义为交叉点）。在 IP 注射 15 mg/kg 3α、5α-THP 或药物 1 小时后，对乙醇免疫的雄性和雌性 P 大鼠进行灌注。在对MCP-1与NeuN、IBA1和GFAP进行双重免疫荧光染色后，使用共聚焦显微镜对NAc和CeA进行成像：结果：MCP-1主要与NeuN相交，而与IBA1/GFAP相交可忽略不计。3α,5α-THP可使NeuN标记细胞中的MCP-1表达量减少，男性为（38.27 ± 28.09%），女性为（56.11 ± 21.46%）；男性为（37.99 ± 19.53%），女性为（54.96 ± 30.58%）。在女性中，3α,5α-THP 可减少 NAc 和 CeA 中 IBA1 和 GFAP 标记体素内的 MCP-1。相反，在男性中，3α,5α-THP 并未显著改变 NAc 中 IBA1 内的 MCP-1 或 CeA 中 GFAP 的 MCP-1。此外，3α,5α-THP 降低了两个区域和两种性别的 IBA1 水平，但对 GFAP 或 NeuN 水平没有影响。对与对照组%值归一化的数据进行的二次分析表明，不存在显著的性别差异：这些数据表明，3α,5α-THP 可抑制 P 型大鼠神经元 MCP-1 的表达并减少小胶质细胞的增殖。这些结果增加了我们对 3α,5α-THP调节乙醇消耗的潜在机制的了解。

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来源期刊

Alcohol (Hanover, York County, Pa.)

CiteScore

5.40

自引率

0.00%

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