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Affinity techniques polymerase chain reaction

To get the solution, we use three techniques polymerase chain reaction (PCR), electrophoresis, and separation through affinity. The machinery behind all this is supramolecular chemistry, with the recognition of synthons and co-synthons (called hybridization in biochemistry ). [Pg.1006]

The principle of in vitro selection is governed by a number of the same principles that apply to the Darwinian theory of evolution, as shown in Figure 2. First, the random sequence DNA is prepared by automated solid-phase synthesis. A mixture of four types of nucleotide is added in a stepwise condensation reaction process. When necessary, this DNA library may be converted to an RNA library by in vitro transcription or to a peptide library by in vitro translation. Second, the prepared DNA, RNA, or peptide library is subjected to affinity selection, and the molecules that bind to a target molecule are selected. Because only a very small part of the library is selected in each selection, the selected fraction is then amplified by a polymerase chain reaction (PCR) or a reverse transcription PCR (RT-PCR) technique. Successive selection and amplification cycles bring about an exponential increase in the abundance of the targeting DNA, RNA, or peptide until it dominates the population. [Pg.195]


See other pages where Affinity techniques polymerase chain reaction is mentioned: [Pg.881]    [Pg.1022]    [Pg.1028]    [Pg.277]    [Pg.385]    [Pg.802]    [Pg.373]    [Pg.1022]    [Pg.1028]    [Pg.139]    [Pg.1441]    [Pg.85]    [Pg.417]    [Pg.723]    [Pg.1089]    [Pg.159]    [Pg.352]    [Pg.54]    [Pg.1916]    [Pg.214]    [Pg.49]    [Pg.167]    [Pg.185]   
See also in sourсe #XX -- [ Pg.198 , Pg.200 ]




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