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通过对表达谱进行生物学筛选鉴定出哈钦森-吉尔福德早衰综合征成纤维细胞中锚蛋白G的过表达。

Ankyrin G overexpression in Hutchinson-Gilford progeria syndrome fibroblasts identified through biological filtering of expression profiles.

作者信息

Wang Jian, Robinson John F, O'Neil Caroline H, Edwards Jane Y, Williams Christina M, Huff Murray W, Pickering J Geoffrey, Hegele Robert A

机构信息

Vascular Biology Research Group, Robarts Research Institute, 100 Perth Drive, London, ON, Canada, N6A 5K8.

Department of Medicine, University of Western Ontario, London, ON, Canada.

出版信息

J Hum Genet. 2006;51(11):934-942. doi: 10.1007/s10038-006-0042-0. Epub 2006 Oct 11.

Abstract

Hutchinson-Gilford progeria syndrome (HGPS; MIM 176670) is a rare disease characterized by accelerated aging. In this study, light and immunofluorescence microscopy were used to assess morphological changes, measures of cell growth kinetics and gene expression profiles in HGPS cells and normal fibroblasts in culture. A filtering strategy was developed based on differentially expressed transcripts seen consistently across three culture stages based on cell passage number. This filtering strategy produced a list of 66 unique differentially expressed genes, of which approximately 40% were upregulated in HGPS cells compared to normal fibroblasts. The increased mRNA expression in HGPS cells that was seen for one gene defined using this strategy--namely ANK3--was validated using quantitative reverse-transcriptase amplification, Western analysis and immunofluorescence microscopy, all of which showed significantly increased ankyrin G expression. These findings demonstrate differences in morphology, growth kinetics and mRNA expression profiles in HGPS cells compared to normal fibroblasts in culture, including increased expression of ANK3/ankyrin G. Furthermore, other genes that co-clustered with ANK3 might provide mechanistic clues regarding senescence in cultured HGPS cells.

摘要

哈钦森-吉尔福德早衰综合征(HGPS;MIM 176670)是一种以加速衰老为特征的罕见疾病。在本研究中,使用光学显微镜和免疫荧光显微镜评估培养的HGPS细胞和正常成纤维细胞的形态变化、细胞生长动力学指标及基因表达谱。基于根据细胞传代次数在三个培养阶段持续出现的差异表达转录本,开发了一种筛选策略。该筛选策略产生了一份包含66个独特差异表达基因的列表,其中与正常成纤维细胞相比,约40%的基因在HGPS细胞中上调。使用此策略确定的一个基因——即ANK3——在HGPS细胞中增加的mRNA表达,通过定量逆转录扩增、蛋白质免疫印迹分析和免疫荧光显微镜进行了验证,所有这些均显示锚蛋白G的表达显著增加。这些发现表明,与培养的正常成纤维细胞相比,HGPS细胞在形态、生长动力学和mRNA表达谱方面存在差异,包括ANK3/锚蛋白G表达增加。此外,与ANK3共聚类的其他基因可能为培养的HGPS细胞衰老提供机制线索。

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