cell or tissue produces a major protein of the cell a large fraction of the total mRNA
will code for the protein. An example of this are the B cells of the pancreas, which
contain high levels of pro-insulin mRNA. In such cases it is possible to precipitate
polysomes which are actively translating the mRNA, by using antibodies to the
ribosomal proteins; mRNA can then be dissociated from the precipitated ribosomes.
More usually the mRNA required is only a minor component of the total cellular
mRNA. In such cases total mRNA may be fractionated by size using sucrose density
gradient centrifugation. Then each fraction is used to direct the synthesis of proteins
using anin vitrotranslation system (Section 6.7).6.2.8 Subtractive hybridisation
It is often the case that genes are transcribed in a specific cell type or differentially
activated during a particular stage of cellular growth, often at very low levels. It is
possible to isolate those mRNA transcripts bysubtractive hybridisation. Usually the
the mRNA species common to the different cell types are removed, leaving the cell
type or tissue-specific mRNAs for analysis (Fig. 6.8). This may be undertaken by
isolating the mRNA from the so-calledsubtractor cellsand producing a first-strand
cDNA (Section 6.2.5). The original mRNA from the subtractor cells is then degraded
and the mRNA from the target cells isolated and mixed with the cDNA. All the
complementary mRNA–cDNA molecules common to both cell types will hybridise
leaving the unbound mRNA which may be isolated and further analysed. A more rapid
approach of analysing the differential expression of genes has been developed using
the PCR. This technique, termeddifferential display, is explained in greater detail in
Section 6.8.1.6.2.9 Cloning PCR products
While PCR has to some extent replaced cloning as a method for the generation of
large quantities of a desired DNA fragment there is, in certain circumstances, stillSubtractor cells Target cellsmRNAmRNA
unhybridised
cDNA (1st strand)Analyse unhybridised
mRNAmRNAmRNAcDNAFig. 6.8Scheme of analysing specific mRNA molecules by subtractive hybridisation.204 Recombinant DNA and genetic analysis