Difference between revisions of "Measuring Lifespan in Drosophila"
From Bridges Lab Protocols
Davebridges (Talk | contribs) (wrote initial protocol based on Broughton et al) |
(No difference)
|
Latest revision as of 14:51, 30 November 2012
Generating Experimental Flies
Setting up Tissue Specific shRNA Expression Experiment
- Generate a large amount of the driver line, since you will need these as both controls and one for each shRNA being tested. See Maintenance of Fly Stocks for details.
- Order and propagate the shRNA lines.
Parental Crosses
- Set up parental cross of Driver/+ vs shRNA/+. If either the driver or the shRNA is homozygous then, you will not get all of the potential controls, but the experiment will still work as long of the alleles is heterozygous.
- Place 10 Females with 3-10 Male flies in a parental cross vial.
- To determine how many parental crosses are needed presume that 10 females will generate XXX flies and calculate backwards.
- After ~10 days remove parental flies to prevent mixing of parental with progenies.
Analysis of Progeny
- Collect eclosed progeny over a 8h period after they have started hatching.
- Separate progeny based on gender and genotype, placing 10 flies in a vial. The goal should be 150-250 flies per genotype/gender
- Transfer flies to a new vial twice weekly under anaesthesia maintaining 10 flies per vial.
- Check for deaths 5-6 times per week.