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链脲佐菌素诱导的猪糖尿病后胃壁内神经元抑制物质表达的变化。

Changes in expression of inhibitory substances in the intramural neurons of the stomach following streptozotocin- induced diabetes in the pig.

机构信息

Department of Clinical Physiology Faculty of Veterinary Medicine, University of Warmia and Mazury, 10-719 Olsztyn, Poland.

Department of Veterinary Prevention and Feed Hygiene, Faculty of Veterinary Medicine, University of Warmia and Mazury in Olsztyn, 10-718 Olsztyn, Poland.

出版信息

World J Gastroenterol. 2017 Sep 7;23(33):6088-6099. doi: 10.3748/wjg.v23.i33.6088.

Abstract

AIM

Influence of chronic hyperglycemia on chemical coding of enteric neurons in stomach using pig as a model for human diabetic complications.

METHODS

Ten pigs were divided into two groups: diabetic (D group, = 5) and control (C group, = 5). Pigs constituting the experimental group were given streptozotocin (150 mg/kg). Animals were euthanized six weeks after the induction of diabetes. The samples of stomach were collected from animals of both groups. The cryostat sections were processed for double immunofluorescence staining using primary antisera directed towards pan-neuronal marker (Hu C/D) proteins and/or neuronal isoform of nitric oxide synthase (nNOS), vasoactive intestinal peptide (VIP) and galanin (GAL).

RESULTS

In the control group in the myenteric ganglia (MG) of the corpus we have noted 22.28% ± 1.19% of nNOS positive neurons, while in diabetic group we have found 40.74% ± 2.22% of nNOS immunoreactive perikarya (increase by 82.85 %). In turn in the pylorus we have observed 15.91% ± 0.58% nNOS containing neurons in control animals and 35.38% ± 1.54% in the diabetes group (increase by 122.37%). In the MG of the antrum and submucosal ganglion (SG) in the corpus hyperglycemia did not cause statistically significant changes. With regard to VIP-positive cell bodies in the antrum MG in the control animals we have noted 18.38 ± 1.39% and 40.74% ± 1.77% in the experimental group (increase by 121.65%). While in the corpus we have observed 23.20% ± 0.23% in the control and 30.93% ± 0.86% in the diabetes group (increase by 33.31%). In turn in the pylorus VIP positive cells bodies constituted 23.64% ± 1.56% in the control group and 31.20% ± 1.10% in the experimental group (increase by 31.97%). In the submucosal ganglion in the corpus we have noted 43.61% ± 1.06% in the control animals and 37.00% ± 1.77% in the experimental group (decrease by 15.15%). Expression of GAL-positive perikarya showed statistically significant changes only in the MG of the antrum and pylorus. In the antrum GAL positive perykarya constituted 26.53% ± 1.52% in the control and 36.67% ± 1.02% in the experimental animals (increase by 38.22%). While in the pylorus GAL positive neurons in the control group constituted 16.32% ± 0.92% and 17.99% ± 0.38% in the experimental animals (increase by 10.23%).

CONCLUSION

Our results support the hypothesis that in the course of diabetes, long term episodes of high glucose serum level may influence the chemical phenotyping of enteric neurons.

摘要

目的

以猪为模型研究慢性高血糖对胃肠神经元化学编码的影响,模拟人类糖尿病并发症。

方法

将 10 头猪分为两组:糖尿病组(D 组,n = 5)和对照组(C 组,n = 5)。实验组给予链脲佐菌素(150mg/kg)。诱导糖尿病 6 周后处死动物。从两组动物中采集胃标本。使用针对神经元 Pan 标志物(Hu C/D)蛋白和/或神经元型一氧化氮合酶(nNOS)、血管活性肠肽(VIP)和甘丙肽(GAL)的初级抗血清,对冰冻切片进行双重免疫荧光染色。

结果

在对照组胃体的肌间神经节(MG)中,我们发现 22.28%±1.19%的 nNOS 阳性神经元,而在糖尿病组中,我们发现 40.74%±2.22%的 nNOS 免疫反应性胞体(增加 82.85%)。反过来,在幽门部,我们观察到对照组动物中有 15.91%±0.58%的 nNOS 含有神经元,而糖尿病组中则有 35.38%±1.54%(增加 122.37%)。在胃体的胃窦 MG 和黏膜下神经节(SG)中,高血糖未引起统计学上的显著变化。关于胃窦 MG 中的 VIP 阳性胞体,我们在对照组中观察到 18.38%±1.39%,在实验组中观察到 40.74%±1.77%(增加 121.65%)。而在胃体中,我们在对照组中观察到 23.20%±0.23%,在实验组中观察到 30.93%±0.86%(增加 33.31%)。反过来,在幽门部,VIP 阳性细胞体在对照组中构成 23.64%±1.56%,在实验组中构成 31.20%±1.10%(增加 31.97%)。在胃体的黏膜下神经节中,我们在对照组中观察到 43.61%±1.06%,在实验组中观察到 37.00%±1.77%(减少 15.15%)。GAL 阳性胞体的表达仅在胃窦和幽门的 MG 中显示出统计学上的显著变化。在胃窦中,GAL 阳性胞体在对照组中构成 26.53%±1.52%,在实验组中构成 36.67%±1.02%(增加 38.22%)。而在幽门部,对照组中 GAL 阳性神经元构成 16.32%±0.92%,实验组中构成 17.99%±0.38%(增加 10.23%)。

结论

我们的结果支持这样的假设,即在糖尿病过程中,长期的高血糖血清水平可能会影响肠神经元的化学表型。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/29ee/5597500/2ca599c44be9/WJG-23-6088-g001.jpg

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