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B.20. SEX- LINKED RECESSIVE LETHAL TEST IN DROSOPHILA MELANOGASTER
1. METHOD
Please notice that only European Community’s legislation published in the paper editions of the Official Journal of the European Communities is deemed authentic.
When preparing this document, care has been taken to ensure correctness of the text; nevertheless possibility of errors cannot be completely excluded, so differences
may exist between this version and the one agreed and published in the paper edition of the Official Journal. In case of doubt the reader is advised to consult the
Official Journal.
This method can be found in Dir 88/303/EEC (OJ L 133 1988).
A complete list of Annex V Testing Methods and the corresponding OJ can be downloaded from a previous page in this site.
1.1. Introduction
See General Introduction Part B.
1.2. Definition
See General Introduction Part B.
1.3. Reference substances
None.
1.4. Principles of the test method
T he sex-linked recessive lethal (SLRL) test using Drosophila melanogaster detects the occurrence of
mutations, both point mutations and small deletions, in the germ line of the insect. This test is a
forward mutation assay capable of screening for mutations at about 800 loci on the X-chromosome;
this represents about 80% of all X-chromosal loci. The X-chromosome represents approximately onefifth of the entire haploid genome.
Mutations in the X-chromosome of Drosophila melanogaster are phenotypically expressed in males
carrying the mutant gene. When the mutation is lethal in the hemizygous condition, its presence is
inferred from the absence of one class of male offspring out of the two that are normally produced by a
heterozygous female. The SLRL test takes advantage of these facts by means of specially marked and
arranged chromosomes.
1.5. Quality criteria
None.
1.6. Description of the test method
Preparations
Stocks
Males of a well-defined wild-type stock and females of the Muller-5 stock may be used. Other
appropriately marked female stocks with multiple inverted X-chromosomes may also be used.
Test substance
Test substances should be dissolved in water. Substances which are insoluble in water may be
dissolved or suspended in appropriate vehicles (e.g. a mixture of ethanol and Tween-60 or 80), then
diluted in water or saline prior to administration. Dimethylsulphoxide (DMSO) should be avoided as a
vehicle.
Number of animals
The test should be designed with a predetermined sensitivity and power. The spontaneous mutant
frequency observed in the appropriate control will influence strongly the number of treated
chromosomes that must be analysed.
Route of administration
Exposure may be oral, by injection or by exposure to gases or vapours. Feeding of the test substance
may be done in sugar solution. When necessary, substances may be dissolved in a 0,7% NaCl solution
and injected into the thorax or abdomen.
Use of negative and positive controls
Negative (vehicle) and positive controls should be included. However, if appropriate laboratory
historical control data are available, no concurrent controls are needed.
Please notice that only European Community’s legislation published in the paper editions of the Official Journal of the European Communities is deemed authentic.
When preparing this document, care has been taken to ensure correctness of the text; nevertheless possibility of errors cannot be completely excluded, so differences
may exist between this version and the one agreed and published in the paper edition of the Official Journal. In case of doubt the reader is advised to consult the
Official Journal.
This method can be found in Dir 88/303/EEC (OJ L 133 1988).
A complete list of Annex V Testing Methods and the corresponding OJ can be downloaded from a previous page in this site.
Exposure levels
Three exposure levels should be used. For a preliminary assessment one exposure level of the test
substance may be used, that exposure level being either the maximum tolerated concentration or that
producing some indication of toxicity. For non-toxic substances exposure to the maximum practicable
concentration should be used.
Procedure
Wild-type males (three to five days old) are treated with the test substance and mated individually to an
excess of virgin females from the Muller-5 stock or from another appropriately marked (with multiple
inverted X-chromosomes) stock. The females are replaced with fresh virgins every two to three days to
cover the entire germ cell cycle. The offspring of these females are scored for lethal effects
corresponding to the effects on mature sperm, mid or late-stage spermatids, early spermatids,
spermatocytes and spermatogonia at the time of treatment.
Heterozygous F1 females from the above crosses are allowed to mate individually (i.e. one female per
vial) with their brothers. In the F2 generation, each culture is scored for the absence of wild-type males.
If a culture appears to have arisen from an F1 female carrying a lethal in the parental X-chromosome
(i.e. no males with the treated chromosome are observed) daughters of that female with the same
genotype should be tested to ascertain whether the lethality is repeated in the next generation.
2. DATA
Data should be tabulated to show the number of X-chromosomes tested, the number of non-fertile
males and the number of lethal chromosomes at each exposure concentration and for each mating
period for each male treated. Numbers of clusters of different sizes per male should be reported. These
results should be confirmed in a separate experiment.
Appropriate statistical methods should be used in evaluation sex-linked recessive lethal tests.
Clustering of recessive lethals originating from one male should be considered and evaluated in an
appropriate statistical manner.
3. REPORTING
3.1. Test report
The test report shall, if possible, contain the following information;
-stock: Drosophila stocks or strains used, age of insects, number of males treated, number of sterile
males, number of F2 cultures established, number of F2 cultures without progeny, number of
chromosomes carrying a lethal detected at each germ cell stage,
-criteria for establishing the size of treated groups,
-test conditions. detailed description of treatment and sampling schedule, exposure levels, toxicity data,
negative (solvent) and positive controls, if appropriate,
-criteria for scoring lethal mutations,
-exposure/effect relationship where possible,
-evaluation of data,
-discussion of results,
-interpretation of results.
3.2. Evaluation and interpretation
See General Introduction Part B.
4. REFERENCES
See General Introduction Part B.
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