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Polymerase chain reaction Insertion/deletion

Fig. 5.2.6 Long-distance polymerase chain reaction (PCR) to detect large deletions and insertions in the low-density lipoprotein receptor (LDLR). The structure of the LDLR gene is shown from exon 1 through 18. The five fragments produced by the five long-distance PCRs are outlined. PCR1 covers exons 1-5, PCR2 exons 6-13, PCR3 exons 15-18, PCR 4 exons 2-10, and PCR5 exons 12-18... Fig. 5.2.6 Long-distance polymerase chain reaction (PCR) to detect large deletions and insertions in the low-density lipoprotein receptor (LDLR). The structure of the LDLR gene is shown from exon 1 through 18. The five fragments produced by the five long-distance PCRs are outlined. PCR1 covers exons 1-5, PCR2 exons 6-13, PCR3 exons 15-18, PCR 4 exons 2-10, and PCR5 exons 12-18...
Key Words 5 fluorogenic assay fluorogenic probes TaqMan allelic discrimination high-throughput genotyping insertion/deletion polymorphisms polymerase chain reaction. [Pg.165]

In addition to PCR, there are many other technologies to amplify nucleic acids. For example, ligation-based amplification or ligase chain reaction uses sequence-directed oligonucleotide primers and thermostable DNA ligase to assay point mutations, deletions, or insertions in DNA. Strand-displacement amplification uses the inherent strand-displacement activity of DNA polymerases to conduct DNA amplification at a constant temperature. Transcription-based methods such as nucleic acid sequence-based amplification (NASBA) involve in vitro RNA transcription. NASBA and most other transcription-based... [Pg.105]


See other pages where Polymerase chain reaction Insertion/deletion is mentioned: [Pg.198]    [Pg.390]    [Pg.2]    [Pg.209]    [Pg.262]    [Pg.312]    [Pg.567]    [Pg.165]    [Pg.165]    [Pg.367]    [Pg.312]    [Pg.564]    [Pg.81]    [Pg.311]   


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Chain insertion reactions

Delete

Deletions

Deletions/insertions

Insertion reactions

Reaction polymerase

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