proteins may be detected by polyacrylamide gel electrophoresis or by immunological
detection usingwestern blotting. Recently oligonucleotide PCR primers have been
designed to incorporate a promoter for RNA polymerase and a ribosome-binding site.
When the so-calledexpression PCR(E-PCR) is carried out the amplified products are
denatured and transcribed by RNA polymerase after which they are translatedin vitro.
The advantage of this system is that large amounts of specific RNA are synthesised thus
increasing the yield of specific proteins (Fig. 6.35).6.7.1 Production of fusion proteins
For a foreign gene to be expressed in a bacterial cell, it must have particular promoter
sequences upstream of the coding region, to which the RNA polymerase will bind
prior to transcription of the gene. The choice of promoter is vital for correct and
efficient transcription since the sequence and position of promoters are specific to a
particular host such asE. coli(Section 5.5.4). It must also contain a ribosome-binding
site, placed just before the coding region. Unless a cloned gene contains both of these
sequences, it will not be expressed in a bacterial host cell. If the gene has been
produced via cDNA from a eukaryotic cell, then it will certainly not have any such
sequences. Consequently, expression vectors have been developed which contain
promoter and ribosome-binding sites positioned just before one or more restrictionPrimer 1 Primer 2T7
promoterStart
codonRestrictionRBS UTR
cloning siteStop codon5
3 5 3 Amplify gene by PCR with primers 1 and 2PCR product with potential for protein productionTranscription and translationRestriction cloning siteFig. 6.35Expression PCR (E-PCR). This technique amplifies a target sequence with one promoter that
contains a transcriptional promoter, ribosome binding site (RBS), untranslated leader region (UTR) and start
codon. The other primer contains a stop codon. The amplified PCR products may be used in transcription
and translation to produce a protein.236 Recombinant DNA and genetic analysis