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Technical Advances |








From the Departments of Pathology*
and Internal
Medicine,
Justus-Liebig-University Giessen,
Giessen, Germany
Differential gene expression can be investigated effectively by
cDNA arrays. Because tissue homogenates result inevitably in an average
expression of a bulk of different cells, we aimed to combine
mRNA profiling with cell-type-specific microdissection. Using a
polymerase chain reaction (PCR)-based preamplification
technique, the expression profile was shown to be preserved. We
modified the existing protocol enabling to apply the total amount of
extracted RNA from microdissected cells. A mean amplification factor of
nearly 1000 allowed to reduce the demand of initial RNA to
10 ng.
This technique was used to investigate intrapulmonary arteries from
mouse lungs (
500 cell equivalents). Using filters with 1176
spots, three independent experiments showed a high consistency
of expression for the preamplified cDNAs. These profiles differed
primarily from those of total lung homogenates. Additionally,
in experimental hypoxia-induced pulmonary hypertension,
amplified cDNA from intrapulmonary vessels of these lungs was compared
to cDNA from vessels dissected from normoxic lungs. Validation by an
alternative method was obtained by linking microdissection with
real-time polymerase chain reaction (PCR). As suggested by the array
data, nine selected genes with different factors of
up-regulation were fully confirmed by the PCR technique. Thus,
a rapid protocol is presented combining microdissection and array
profiling that demands low quantities of initial RNA to assess reliably
cell-type-specific gene regulation even within nonneoplastic complex
tissues.
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