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LT12 Yeast Genetics R83,22   Add to cart

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LT12 Yeast Genetics

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Yeast Genetics: transgenics and uses (cell cycle etc.(

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  • April 10, 2016
  • 4
  • 2014/2015
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Yeast Genetics

Characteristics

Budding yeast: Saccharomyces cerevisiae Fission yeast: Saccharomyces pombe
 2 hour doubling time  Budding and fission yeast share many
 3-4 days for colony from single cell experimental similarities but are
 Growth on chemically defined media evolutionarily distant.
(down to specific amino acids)  They separated over 400 million years
 Store frozen at -70oC ago.
 Total length of genome: 12.1 x 106 bp  Total length of genome: 14 x 106 bp
 Around 6,000 ORFs  Around 5,000 ORFs
 Lots of non-coding RNAs




Mating types

Mutagenesis

 Mutagenise and screen haploid yeast
 Replica plate potentially lethal phenotypes
 Very often – mutants are normally lethal/sterile – haploid, no need to do breeding
schemes
 Design screen – choose phenotype that is viable or lethal only under certain
conditions

Transgenesis

 Similar process to bacteria
 Selectable bacterial marker/bacterial origin of
replication
 Selectable yeast marker/yeast 2 micron origin 
selectable markers normally based on mutants unable
to synthesis specific amino acid
 Multiple cloning sites

, Cloning by functional complementation

 ARG2 gene – gene involved in arginine
biosynthesis pathway
 Infect yeast cells with a library of genes
(read notes)




Targeted Mutagenesis

 Homologous recombination extremely efficient in yeast
 Only 25bp of homologous sequence required
 Targeting constructs and systematic gene disruption
- Recombination between homologous regions 1 and 2 replaces
MFG1 coding sequence with URA3 cassette
- Constructs generated very efficiently for any gene by PCR

Genome-wide tagged mutation libraries

 All 6000 yeast ORFs have been targeted and tagged
 4500 ORFS not required for viability under standard
conditions – screen for phenotypes for competitive
ability in yeast –loci that confer increased fitness
- Place 10 cells of each of the 6000 strains in a flask –
subject flask to various stressful conditions
- Tagged strains can be subjected to competition and
% of each strain determined by DNA extraction and
microchip analysis

Ageing of pool maintained in stationary phase containing 3000 S. pombe mutants

 Maintain yeast cells at stationary phase – don’t grow but can die
 Samples collected at various time points – DNA extraction, PCR, sequencing of
barcodes follows
 Sequencing data; no. of reads per tag/mutant – determine presence and proportion
of mutants in different samples




Epistasis Analysis

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