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Development and characterization of a novel method to analyze global gene expression profiles in endothelial cells derived from primary tissues.

Development and characterization of a novel method to analyze global gene expression profiles in endothelial cells derived from primary tissues. Research Abstract Details 

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  • Development and characterization of a novel method to analyze global gene expression profiles in endothelial cells derived from primary tissues. Abstract Text:

    xiangyang baiXiangyang Bai,mei huangMei Huang,jingyi wuJingyi Wu,xiaoyuan huangXiaoyuan Huang,lingling yanLingling Yan,yunping luYunping Lu,shixuan wangShixuan Wang,gang xuGang Xu,jianfeng zhouJianfeng Zhou,ding maDing Ma,xiangyang baiXiangyang Bai,mei huangMei Huang,jingyi wuJingyi Wu,xiaoyuan huangXiaoyuan Huang,lingling yanLingling Yan,yunping luYunping Lu,shixuan wangShixuan Wang,gang xuGang Xu,jianfeng zhouJianfeng Zhou,ding maDing Ma,

    Homogenous cells separated directly from clinical samples with laser capture microdissection (LCM) contain their original transcript messages, which accurately reflects the physiological and pathological changes of the cell before fixation. Analysis of such samples provides a direct understanding of in vivo physiological and pathological processes. The development of modern large-scale analytical techniques have given us a chance to determine the entire transcript profile of interesting cells. Therefore, LCM and gene expression microarray analysis are becoming common tools across a broad range of disciplines, particularly in the basic and clinical biomedical sciences. However, the combination of these technologies is limited in the study of vascular endothelial cell (VEC) since the precise location and separation of VECs is not easily realized and the requirement for relatively large amount of intact RNA for labeling and hybridization is not easily available. In this report, we describe an approach for tissue fixation and isolation of RNA from laser-captured cells retrieved from frozen sections, which had previously been subjected to immunohistochemistry and subsequently subjected to linear amplification and gene expression microarray analysis. Our results demonstrate that nanogram quantities of total RNA isolated from about 3,000 VECs can be amplified and that the amplified RNA can generate enough signal intensity for GeneChip analysis. analysis. Am. J. Hematol., 2008. (c) 2007 Wiley-Liss, Inc.

    Development and characterization of a novel method to analyze global gene expression profiles in endothelial cells derived from primary tissues. Publishing Authors By Initials

    x baiX Bai,m huangM Huang,j wuJ Wu,x huangX Huang,l yanL Yan,y luY Lu,s wangS Wang,g xuG Xu,j zhouJ Zhou,d maD Ma,x baiX Bai,m huangM Huang,j wuJ Wu,x huangX Huang,l yanL Yan,y luY Lu,s wangS Wang,g xuG Xu,j zhouJ Zhou,d maD Ma,

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    Development and characterization of a novel method to analyze global gene expression profiles in endothelial cells derived from primary tissues. Journal Published:

    PUBLICATION TYPE: Journal Article

    Journal: American journal of hematology

    VOLUME: 83

    Page Numbers: 26-33

    Journal Abbreviation: Am. J. Hematol.

    ISSN: 0361-8609

    DAY: 21

    MONTH: Jan

    YEAR: 2008

    Development and characterization of a novel method to analyze global gene expression profiles in endothelial cells derived from primary tissues. Information

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    LANGUAGE: eng

    NlmUniqueID: 7610369

    Development and characterization of a novel method to analyze global gene expression profiles in endothelial cells derived from primary tissues. Keywords Mesh Terms:

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    Grant and Affiliation Information for Development and characterization of a novel method to analyze global gene expression profiles in endothelial cells derived from primary tissues.

    AFFILIATION: Cancer Biology Research Center, Tongji Hospital, Tongji Medical College, Huazhong University of Science and Technology, Wuhan, Hubei 430030, China.

    Country: United States

    United States Research PublicationUnited States Research Publication

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    MEDLINETA: Am J Hematol

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