Nucleic Acids Research, Vol 25, Issue 13 2598-2602, Copyright © 1997 by Oxford University Press
OD von Stein, WG Thies and M Hofmann
A novel method combining elements of suppression subtractive hybridization
with high throughput differential screening permits the efficient and rapid
cloning of rarely transcribed differentially expressed genes. The
experimental strategy virtually excludes the possibility of isolating false
positive clones. The potential of the method is demonstrated by the
isolation of 625 differentially expressed cDNAs from the metastatic
adenocarcinoma cell line Bsp73-ASML when subtracted from its non-metastatic
counterpart Bsp73-1AS. Northern analysis of 72 randomly selected clones
demonstrated that 68 were differentially expressed with respect to
Bsp73-ASML, indicating a true positive rate of 94%. Additionally, a large
proportion of these clones represented rare transcripts as determined by
the exposure time required to detect a signal. Sequence data indicated that
of the 625 clones obtained, 92 clones scored perfect or near perfect
matches with already known genes. Two hundred and eighty one clones scored
between 60 and 95% homology to known human and mouse genes, whereas 252
clones scored no match with any sequences in the public databases. The
method we describe is ideally suited whenever subtle changes in gene
expression profiles need to be determined.
ARTICLES
A high throughput screening for rarely transcribed differentially expressed genes
Institut fur Genetik (IGEN) and 1 Institute fur Toxikologie (ITOX), Forschungszentrum Karlsruhe, PO Box 3640, 76021 Karlsruhe, Germany.
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