Summary

Summary Polymerase Chain Reaction

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Course
Introduction To Genetics (BLGY1232)

Institution
University Of Leeds (UoL)

Detailed notes summarising PCR

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Uploaded on February 21, 2022
Number of pages 4
Written in 2018/2019
Type Summary

pcr
biology
genetics

Institution
University of Leeds (UoL)
Education
University of Leeds
Course
Introduction To Genetics (BLGY1232)

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Introduction to Genetics

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1. Class notes - Introduction to genetics
2. Class notes - Meiosis
3. Class notes - bacterial genetics transduction
4. Class notes - Bacterial genetics
5. Class notes - Genome size and complexity
6. Class notes - Regulating development in plants
7. Class notes - Regulating development in complex animals
8. Class notes - Programming of development
9. Class notes - Gene amplification and rearrangement
10. Class notes - Rna processing
11. Class notes - Eukaryotic transcription
12. Summary - Gene expression
13. Summary - Screening tratement and therapies
14. Summary - Genetics and disease
15. Summary - Locating genes underlying human phenotypes
16. Summary - Locating genes underlying human phenotypes
17. Summary - Human genetics
18. Summary - Polymerase chain reaction
19. Summary - Dna sequencing and future of dna sequencing
20. Summary - Gene cloning and sequencing
21. Summary - Mutation and recombination
22. Summary - Gene mutation
23. Summary - Genetic material
24. Summary - Interactions between genes
25. Summary - Sex determination and sex linkage
26. Summary - Chromosomes
27. Summary - Dihybrid crosses
28. Summary - Monohybrid crosses
29. Summary - Inheritance
30. Summary - Post transcriptional initation control and regulatory rnas
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BLGY1232 PCR

The 21st century: the “post-genomic” age
 The completion of an increasing number of genome sequencing projects has
ushered in the “post-genomic age”  We now have access to genome sequence
information via the internet, and this has enabled a new set of experimental
approaches
 Comparative genome studies - comparing the organisation of genomes, and the
sequences of homologous genes from different organisms provides us with
information about the evolutionary relationship between extant species, and the
ways in which new gene functions have evolved as ancestral genes become
duplicated and subject to divergent selection over evolutionary time  globin
gene evolution;

 It is now possible to purify any gene for which sequence information is available,
without the need for the “cut-ligate-screen” procedures of gene cloning, by
using the POLYMERASE CHAIN REACTION (PCR)
 PCR utilises the property of DNA polymerase: this enzyme will extend an
oligonucleotide primer annealed to a single-stranded DNA template
 Allows the selective amplification of any gene from a genome, without the need
for cut-paste-screen cloning, provided that sufficient sequence information is
available
1. Isolate DNA from the organism of choice, and denature its DNA by heating at
95 C for 30 seconds. This will render it single-stranded.
2. Anneal primers at 45-60 C for 30 secs - Now add two oligonucleotide primers:
25-30 base synthetic DNA sequences that anneal to sequences (i) at either end of
the sequence to be amplified (ii) on the opposite strands of the DNA:

3. Now add DNA polymerase and the 4 dNTP monomers, and the primers will be
extended from their free 3’-OH ends. NOTE: the 3’-ends of the 2 primers must
“point inwards”  This produces 2 DNA strands, where previously there was 1.
4. Repeat this 30 times, and you generate 2 30 copies of the sequence lying
between the two primers.

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