电针抑制PDK1/Akt/HCN4通路改善大鼠神经源性尿潴留。

Zheng-Fei Li, Ren Zhang, Guo-Rui Zhao, Yao Kuang
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引用次数: 0

摘要

目的:观察电针(EA)对神经源性尿潴留大鼠的治疗作用,以3-磷酸依赖性蛋白激酶1(PDK1)/蛋白激酶B(Akt)/超极化激活的环核苷酸门控阳离子通道4(HCN4)通路为研究对象,探讨电针治疗神经源性尿液潴留的潜在机制。方法:雌性SD大鼠随机分为假手术组、模型组、电针组、PDK1抑制剂组、HCN4阻滞剂组和电针+HCN4阻断剂组,每组20只。采用改良Hassan Shaker脊髓横断法建立骶髓损伤模型。电针(2Hz/15Hz,0.5mA)分别作用于“中脊”(CV3)和“中寮”(BL33)20min,每日1次,持续10d。PDK1抑制剂组大鼠腹膜内注射OSU-03012(20mg/kg),HCN4阻断剂组大鼠腹腔内注射伊伐布雷定(10mg/kg),两组均每隔一天注射一次,持续10天。采用多通道生理记录仪检测大鼠尿动力学指标采用肌条试验检测逼尿肌兴奋性HE染色观察膀胱的形态学变化。免疫荧光双染色法检测HCN4与膀胱Cajal间质细胞特异性标志物C-Kit的共表达。采用蛋白质印迹法检测膀胱组织中PDK1/Akt/HCN4通路蛋白和与膀胱收缩功能相关的热休克蛋白27(HSP27)的表达。结果:与假手术组相比,模型组大鼠出现尿功能障碍、泄漏点压降低、逼尿肌自发收缩频率分离、C-Kit阳性细胞荧光强度、HCN4+/C-Kit+共表达,HCN4和p-HSP27/HSP27蛋白在膀胱组织中的表达(PPP+/C-Kit+)以及HCN4、p-HSP27/HSP27蛋白的表达降低(PPC结论:电针可改善神经源性尿潴留大鼠的尿功能障碍,这可能与其抑制PDK1/Akt通路的激活、促进HCN4介导的逼尿肌兴奋性收缩和尿电信号激活有关。
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Electroacupuncture inhibits PDK1/Akt/HCN4 pathway to improve neurogenic urinary retention in rats.

Objectives: To observe the therapeutic effect of electroacupuncture (EA) on neurogenic urinary retention rats, so as to explore the underlying mechanism of EA in treating neurogenic urinary retention by focusing on 3-phosphoinositide-dependent protein kinase 1 (PDK1)/protein kinase B (Akt)/hyperpolarization activated cyclic nucleotide-gated cation channel 4 (HCN4) pathway.

Methods: Female SD rats were randomly divided into sham operation, model, EA, PDK1 inhibitor, HCN4 blocker and EA + HCN4 blocker groups, with 20 rats in each group. The model of sacral spinal cord injury was established by modified Hassan Shaker spinal cord transection method. EA (2 Hz/15 Hz, 0.5 mA) was applied to "Zhongji" (CV3) and "Zhongliao" (BL33) for 20 min, once daily for 10 days. Rats of the PDK1 inhibitor group received intraperitoneal injection of OSU-03012 (20 mg/kg), and rats of the HCN4 blocker group received intraperitoneal injection of ivabradine (10 mg/kg), both once every other day for 10 days. The urodynamic indexes of rats were detected by multi-channel physiological recorder;muscle strip test was used to detect detrusor excitability;the morphological changes of bladder were observed by HE staining. Immunofluorescence double staining was used to detect the co-expression of HCN4 and C-Kit, a specific marker of interstitial cells of Cajal in bladder. Western blot was used to detect the expression of PDK1/Akt/HCN4 pathway proteins in bladder tissue and heat shock protein 27 (HSP27), a protein related to bladder contraction function.

Results: Compared with the sham operation group, the rats in the model group showed urinary dysfunction, decreased leak point pressure, isolated detrusor spontaneous contraction frequency, fluorescence intensity of C-Kit positive cells, HCN4+/C-Kit+ co-expression, HCN4 and p-HSP27/HSP27 protein expression in bladder tissue (P<0.05), and increased maximum bladder capacity and comp-liance, minimum tension during contraction of isolated detrusor, PDK1 and p-Akt/Akt protein expression in bladder tissue (P<0.05). Meanwhile, the above index were all reversed after EA and PDK1 inhibitor intervention (P<0.05). In comparison with the EA group, the rats had severe urinary dysfunction, the urine leakage point pressure, spontaneous contraction frequency, fluorescence intensity of C-Kit positive cells, the co-expression of HCN4+/C-Kit+, and the protein expression of HCN4 and p-HSP27/HSP27 were decreased (P<0.05), the maximum bladder capacity and compliance, the minimum tension during contraction of isolated detrusor, and the protein expression of PDK1 and p-Akt/Akt in bladder tissue were increased (P<0.05) in both HCN4 blocker and EA+HCN4 blocker groups. HE staining showed exfoliated bladder epithelium and disordered layers, vacuolization of bladder wall cells, with infiltration of neutrophils in mucosal and muscular layers in the model group, which were relatively milder in the EA and PDK1 inhibitor groups, but worse in the HCN4 blocker and EA + HCN4 blocker groups.

Conclusions: EA can improve the urinary dysfunction in rats with neurogenic urinary retention, which may be related to its effect in inhibiting the activation of PDK1/Akt pathway, promo-ting HCN4-mediated detrusor excitatory contraction and urinary electrical signal activation.

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