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Open AccessJournal ArticleDOI

A rapid and simple PCR-based method for isolation of cDNAs from differentially expressed genes.

Boris P. Sokolov, +1 more
- 25 Sep 1994 - 
- Vol. 22, Iss: 19, pp 4009-4015
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TLDR
A simple and rapid PCR-based protocol to both detect and isolate cDNA fragments of up to 3000 base pairs from differentially expressed genes in two easy steps is reported.
Abstract
Recently two techniques have been reported which use arbitrarily primed RT-PCR amplification of cDNA fragments from subsets of mRNAs to detect cDNA fragments from differentially expressed mRNAs. Here we report a simple and rapid PCR-based protocol to both detect and isolate cDNA fragments of up to 3000 base pairs from differentially expressed genes in two easy steps. To generate cDNAs from most mRNAs, the first step consisted of reverse transcription using a fully degenerated 6-mer oligonucleotide as primer. The second step consisted of PCR amplification of internal regions of the cDNAs with two or three longer primers with arbitrary but defined sequences. DNA fragments were easily displayed by agarose gel electrophoresis and then excised for direct use in cloning, sequencing, and Northern blot analysis. By repeating the PCR amplification (second step) on the same cDNA templates (first step) ten times with different sets of primers, over 170 discrete cDNA fragments were obtained from a single tissue. By combining the two-step procedure with 3'-RNA-anchored cDNA extension, additional DNA fragments can be generated from the same mRNA. The new procedure was used here to define 3600 bp of a new brain-specific mRNA.

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Identification by Differential Display of Transcripts Regulated during Hematopoietic Differentiation

TL;DR: Three cDNA transcripts display differential expression during cytokine‐induced maturation of CD34+ cells and represent novel hematopoietic cDNAs that should prove of value for the study of human blood cells and their disorders.
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Photomorphogenesis in Phycomyces: differential display of gene expression by PCR with arbitrary primers.

TL;DR: A method based on the polymerase chain reaction with arbitrary primers to investigate the role of differential gene expression during photophorogenesis in Phycomyces demonstrated the feasibility of this approach by the isolation of a cDNA segment for the heat-shock protein HSP100 that is induced by blue light at the onset of sporangiophore development.
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Transcriptional analysis of the response of poultry species to respiratory pathogens.

TL;DR: The adoption of a conceptually simple approach to understand the genetic and biochemical responses of host cells during infection with respiratory pathogens, such as avian pneumovirus, suggests that a molecular description of host-pathogen interactions in terms of differential gene expression will provide key insights on the molecular basis of disease pathogenesis, pathogen virulence, and host immunity.
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Identification of Avian Sarcoplasmic Reticulum Ca2+-ATPase (SERCA3) as a Novel 1,25(OH)2D3 Target Gene in the Monocytic Lineage☆

TL;DR: A new target gene, a chick ATP-dependent Ca(2+) pump, ChkSERCA3 is identified, which was restricted to the hematopoietic cell lineage, spleen, lung, intestine, and brain, whereas no expression was detected in embryos, further supporting the critical role for intracellular calcium in highly specialized cells such as osteoclasts.
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