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一种在气道活检匀浆中进行基因转录谱分析的新方法显示,哮喘患者中钠-钾-氯共转运体(NKCC1)的表达增加。

A novel method of gene transcript profiling in airway biopsy homogenates reveals increased expression of a Na+-K+-Cl- cotransporter (NKCC1) in asthmatic subjects.

作者信息

Dolganov G M, Woodruff P G, Novikov A A, Zhang Y, Ferrando R E, Szubin R, Fahy J V

机构信息

Genelabs Technologies, Inc., Redwood City, California 94063, USA.

出版信息

Genome Res. 2001 Sep;11(9):1473-83. doi: 10.1101/gr.191301.

DOI:10.1101/gr.191301
PMID:11544191
Abstract

Comprehensive and systematic analysis of airway gene expression represents a strategy for addressing the multiple, complex, and largely untested hypotheses that exist for disease mechanisms, including asthma. Here, we report a novel real-time PCR-based method specifically designed for quantification of multiple low-abundance transcripts using as little as 2.5 fg of total RNA per gene. This method of gene expression profiling has the same specificity and sensitivity as RT-PCR and a throughput level comparable to low-density DNA microarray hybridization. In this two-step method, multiplex RT-PCR is successfully combined with individual gene quantification via real-time PCR on generated cDNA product. Using this method, we measured the expression of 75 genes in bronchial biopsies from asthmatic versus healthy subjects and found expected increases in expression levels of Th2 cytokines and their receptors in asthma. Surprisingly, we also found increased gene expression of NKCC1--a Na+-K+-Cl- cotransporter. Using immunohistochemical method, we confirmed increased protein expression for NKCC1 in the asthmatic subject with restricted localization to goblet cells. These data validate the new transcriptional profiling method and implicate NKCC1 in the pathophysiology of mucus hypersecretion in asthma. Potential applications for this method include transcriptional profiling in limited numbers of laser captured cells and validation of DNA microarray data in clinical specimens.

摘要

对气道基因表达进行全面系统的分析,是应对包括哮喘在内的多种复杂且大多未经检验的疾病机制假说的一种策略。在此,我们报告一种基于实时PCR的新方法,该方法专门设计用于定量多个低丰度转录本,每个基因仅需2.5 fg的总RNA。这种基因表达谱分析方法具有与逆转录聚合酶链反应(RT-PCR)相同的特异性和灵敏度,以及与低密度DNA微阵列杂交相当的通量水平。在这个两步法中,多重RT-PCR通过对生成的互补DNA(cDNA)产物进行实时PCR成功地与单个基因定量相结合。使用这种方法,我们测量了哮喘患者与健康受试者支气管活检组织中75个基因的表达情况,发现哮喘患者中Th2细胞因子及其受体的表达水平出现预期的升高。令人惊讶的是,我们还发现钠-钾-氯协同转运蛋白1(NKCC1)的基因表达增加。使用免疫组织化学方法,我们证实哮喘患者中NKCC1的蛋白表达增加,且其定位局限于杯状细胞。这些数据验证了新的转录谱分析方法,并表明NKCC1参与哮喘中黏液高分泌的病理生理过程。该方法的潜在应用包括对有限数量的激光捕获细胞进行转录谱分析,以及在临床标本中验证DNA微阵列数据。

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