Smad Proteins Localization in Chronic Bronchial Asthma Rats Lung Tissue by Lmmunofluorescence and Gene Expression

SUN Zhu-mei; LI Fu-feng; QIAN Peng; ZHAO Jie; WEN Xu-jie

doi:CNKI:11-3495/R.20110823.1117.008

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Smad Proteins Localization in Chronic Bronchial Asthma Rats Lung Tissue by Lmmunofluorescence and Gene Expression

更新时间：2024-01-04

- Smad Proteins Localization in Chronic Bronchial Asthma Rats Lung Tissue by Lmmunofluorescence and Gene Expression
- Chinese Journal of Experimental Traditional Medical Formulae Vol. 17, Issue 20, Pages: 207-210(2011)
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- DOI：CNKI:11-3495/R.20110823.1117.008
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- Published：2011
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SUN Zhu-mei, LI Fu-feng, QIAN Peng, et al. Smad Proteins Localization in Chronic Bronchial Asthma Rats Lung Tissue by Lmmunofluorescence and Gene Expression[J]. Chinese journal of experimental traditional medical formulae, 2011, 17(20): 207-210.
DOI：

SUN Zhu-mei, LI Fu-feng, QIAN Peng, et al. Smad Proteins Localization in Chronic Bronchial Asthma Rats Lung Tissue by Lmmunofluorescence and Gene Expression[J]. Chinese journal of experimental traditional medical formulae, 2011, 17(20): 207-210. DOI： CNKI:11-3495/R.20110823.1117.008.

摘要

目的: 探讨Smads蛋白家族在慢性哮喘大鼠肺组织中的定位表达及其 mRNA变化情况

以反映其在哮喘大鼠气道重建过程的作用。方法: 24只SD大鼠分为正常组和模型组各12只。模型组以10%卵蛋白+10%氮氧化铝生理盐水ip致敏

2周后用2%卵蛋白雾化吸入1 min

隔天1次

引喘

共2周后处死。取肺组织切片(HE染色)作形态学观察;荧光免疫组化法测定Smads蛋白家族在肺组织中的定位;RT-PCR测定Smads蛋白家族 mRNA的变化情况。结果: HE染色显示模型组有较明显出血

肺泡均有一定程度扩张

有慢性炎细胞浸润;荧光免疫组化法显示Smads蛋白家族均在在支气管壁和肺泡壁上表达;RT-PCR测定显示模型组Smad2 mRNA较正常组高表达(P<0.05);模型组Smad7 mRNA较正常组显著低表达(P<0.05);两组Smad4 mRNA之间无差异。结论: Smads蛋白家族与慢性哮喘关系密切

在正常与哮喘模型中都可见Smads蛋白家族的表达

在哮喘发生过程中

受体型Smad2 mRNA表达增加

抑制型Smad7 mRNA表达下降

说明TGF-β/Smad信号途径可能被活化。

Abstract

Objective: To investigate the Smads proteins localization in lung tissue of chronic bronchial asthma rats lung tissue and its mRNA expression

and to explore the TGF-β/Smad signaling pathway

thus in the chronic bronchial asthma. Method: Twenty-four Sprague-Dawley rats were randomly divided into two groups:normal control group was treaded by 0.9% saline; model group treaded by the mixture(10%ovalbumin+10%aluminum hydroxide). HE staining was used to observe the pathomorphological changes;Smad proteins localization in lung tissue was determined by immunofluorescence; Smads mRNA expression was determed by RT-PCR. Result: HE staining showed the model group was obviously bleeding

expanding of lung alveolar andinflammatory cell. The results showed Smads proteins were located in the bronchial wall or alveolar wall by immunofluorescence assay;RT-PCR showed that the Smad2 mRNA expression were higher significantly in model group than that in normal group (P<0.05); Smad7 mRNA expression were significantly lower in model group than that in normal expression (P<0.05); Smad4 mRNA expression was no difference between the two groups. Conclusion: Smads proteins had closely related to chronic asthma

Smad proteins were located in lung tissue of both normal rats and chronic bronchial asthma rats. In the course of asthma

receptor type Smad2 mRNA was increased in expression

inhibitory type Smad7 mRNA was decreased in expression

and thus TGF-β/Smad signaling pathways that might be activated.

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