Real-time quantitative RT-PCR after laser-assisted cell picking

被引:519
|
作者
Fink, L
Seeger, W
Ermert, L
Hänze, J
Stahl, U
Grimminger, F
Kummer, W
Bohle, RM
机构
[1] Univ Giessen, Dept Pathol, D-35392 Giessen, Germany
[2] Univ Giessen, Dept Internal Med, D-35390 Giessen, Germany
[3] Univ Giessen, Dept Pediat, D-35390 Giessen, Germany
[4] Univ Giessen, Inst Anat & Cell Biol, D-35390 Giessen, Germany
关键词
D O I
10.1038/3327
中图分类号
Q5 [生物化学]; Q7 [分子生物学];
学科分类号
071010 ; 081704 ;
摘要
The present study describes a technique for quantitation of mRNA in a few isotypic cells obtained from an intact organ structure by combining laser-assisted cell picking and real-time PCR. The microscopically controlled lasering of selected cells in stained tissue sections was applied to lung alveolar macrophages, which are unique in that they can alternatively be gathered as a pure cell population from intact lungs by bronchoalveolar lavage as a reference technique. TNF-α was chosen as the transcriptionally inducible target gene to be quantified in alveolar macrophages of control rat lung, as well as low- and high-challenge lungs stimulated by endotoxin and IFN-γ nebulization. Online fluorescence detection for quantitation of the number of amplified copies was based on 5' nuclease activity of Taq polymerase cleaving a sequence-specific dual-labeled fluorogenic hybridization probe. A pseudogene-free sequence of PBGD served as an internal calibrator for comparative quantitation of target. A quick procedure and minimized loss of template were achieved by avoiding RNA extraction, DNase digestion and nested-PCR. Using this approach, we demonstrated dose-dependent manifold upregulation of the ratio of TNF-α mRNA copies per one copy of PBGD mRNA in alveolar macrophages of the challenged lungs. The quantitative data obtained from laser-picked alveolar macrophages were well matched with those of lavaged alveolar macrophages carried out in parallel. We suggest that this new combination of laser-assisted cell picking and real-time PCR has great promise for quantifying mRNA expression in a few single cells or oligocellular clusters in intact organs, allowing assessment of transcriptional regulation in defined cell populations.
引用
收藏
页码:1329 / 1333
页数:5
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