Oligomicroarray-based primary study of gene expression profile changes in Barrett’s esophagus

Wang Xingwei1; Sun Yonggang1; Xu Mei1; Fang Dianchun1; Gao Hengjun2; Xu Jiangtao2; 1Gastroenterology Research Center; Southwest Hospital; Third Military Medical University; Chongqing 400038; China 2 National Engineering Center for Shanghai Biochip Technology; Shanghai 201203; China

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Oligomicroarray-based primary study of gene expression profile changes in Barrett’s esophagus

Updated：2026-03-12

- Oligomicroarray-based primary study of gene expression profile changes in Barrett’s esophagus
- Oligomicroarray-based primary study of gene expression profile changes in Barrett’s esophagus
- 解放军医学杂志（英文版） 2008年第5期页码：251-257
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  中图分类号： R735.1
- 纸质出版：2008
- Accepted：
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Oligomicroarray-based primary study of gene expression profile changes in Barrett’s esophagus[J]. 解放军医学杂志（英文版）, 2008,(5):251-257.

[1].Oligomicroarray-based primary study of gene expression profile changes in Barrett’s esophagus[J].Journal of Medical Colleges of PLA,2008(05):251-257.
Oligomicroarray-based primary study of gene expression profile changes in Barrett’s esophagus[J]. 解放军医学杂志（英文版）, 2008,(5):251-257. DOI：

[1].Oligomicroarray-based primary study of gene expression profile changes in Barrett’s esophagus[J].Journal of Medical Colleges of PLA,2008(05):251-257. DOI：

摘要

Abstract

Objective: To analyze the differential expression genes （DEGs） between Barrett’s esophagus （BE） and normal esophagus mucosa and explore the target genes related to the development and progression of BE. Methods: The total RNAs of matched BE and normal esophagus mucosa of BE patients were isolated using one step Trizol method. Matched RNAs were qualified using 10 g/L agarose gel electrophoresis. cRNAs were synthesized

fluorescence labeled and purified after total RNAs were purified. The RNAs of BE and normal esophagus mucosa were hybridized with Agilent oligomicroarray （30 968 probes）. The fluorescence intensity features were detected by Agilent scanner and quantified by feature extraction software. Results: （1） The total RNA

reverse transcription product and fluorescence labeled cRNA were all of high quality; （2） There were 142 up-regulated genes and 284 down-regulated genes among 2-fold DEGs. Conclusion: Microarray-based studies are feasible in endoscopically obtained tissues. Many BE-associated genes are screened by the high-throughput gene chip. The development and progression of BE is a complicated process involving multiple genes and multiple procedures

and functional study of these genes may help to identify the key genes or pathways involved in the pathogenesis and development of BE.

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