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The Role of how in Leg Imaginal Disc Morphogenesis in Drosophila melanogaster Nicole Whyte Craig Woodard July 23, 2004 Background and Significance The processes that lead to the development of animal body parts include complex steps that should be executed accurately to ensure the proper formation. These developmental processes are controlled by the interaction of the genes present in the organism. Genes regulate growth and development by hormonal signaling, including steroid hormones, in simple organisms such as insects to more intricate organisms such as humans. Introduction Drosophila melanogaster are interesting organisms to study. ßFTZ-F1 vs. how Gene Examination of leg development in how mutant fruit flies Drosophila melanogaster Pupariation (Entry into Metamorphosis) Morphogenesis of Adult Body Parts Destruction of Larval body Parts by Programmed Cell Death Leg Morphogenesis in Drosophila melanogaster Structures such as wings and legs in the fruit fly originate from the imaginal disc sacs formed during embryogenesis. Imaginal discs are small packets of cells in the larva which undergo morphogenesis during the metamophosis of the insect. The discs are covered by a single layer of cells called the peripodial epithelium. Third Instar Larva Leg Disc Eversion Adult Cell Shape Changes During Leg Disc Elongation a b Courtesy of Condic et al. 1991. Development 111:23-33 Normal Leg Development QuickTime™ QuickTime™and anda a Sorenson Video decompressor Sorenson Video decompressor are areneeded neededtotosee seethis thispicture. picture. how Gene The how gene found in Drosophila melanogaster encodes a KH RNA binding protein, and is involved in processes such as muscle development. There are different how mutant alleles, some stronger than others. Example: howe44 and howstruthio are strong mutant alleles that results in embryonic death of the flies, while the howr17 is a weak allele. Some of these flies survive to adulthood. how Mutants Show Defects in Leg Development how Mutant Leg Development QuickTime™ and a Video decompressor are needed to see this picture. Experiment What causes the short and crooked leg phenotype seen in how mutants? The experiment included the characterization of leg imaginal disc: length and shape cell shape changes comparison of mutation in each leg disc Materials and Method The animals were kept on standard cornmeal/molasses/yeast medium at 250C or 180C. For the experiment, three strains of animals were used: howe44/TM6B,Hu,Tb,e w; +; howr17/TM6B,Hu,Tb,e Humeral (Hu) Tubby (Tb), Ebony (e) Canton S wild type (CS) Materials and Methods Cont. Experimental animals: howe44/TM6B,Hu,Tb,e F1: X w;+;howr17/TM6B,Hu,Tb,e howe44/ howr17 Control animals: howe44/TM6B,Hu,Tb,e X F1: howe44/ + CS (+/+) Materials and Methods Cont. Zero hour APF prepupae (white, not tubby) animals were collected and maintained at 250C for 6 hours. The leg imaginal discs were dissected out from the animals in PBS Buffer solution at room temperature and fixed in 4% formaldehyde for 18-24 hours at 40C. Then permeabilized for 1-2 hours with 0.5% Triton X-100 (w/v in PBS) at room temeperature. Materials and Methods Cont. The leg imaginal discs were stained with the fluorescent AlexaFluor 488 0.6 µM phalloidin solution for four hours at room temperature. Then rinsed in 0.5% Triton X-100 (w/v in PBS) for 2 hours at room temperature, with 3 changes. The leg imaginal discs were mounted in VectashieldTM and viewed with a Zeiss LSM 510 Meta laser scanning confocal microscope and Nikon SMZ 1500 Stereoscope. Cell Shape in Leg Disc control Stubble Mutant Results Cell Shape in Mutant Animal howe44/ howr17 Phenotypic Differences in 6 hr APF Leg Disc Wild type howe44/ howr17 mutant Peripodial Epithelium in Mutant 6 hr APF Leg Disc howe44/ howr17 Discussion Normal cell shape change occurs in mutants The mutation affects each leg differently The peripodial epithelium is still present around the leg disc which might contribute to the short and bent legs observed Future Work Determine why the leg discs fail to orient properly Examine younger animals to see if there are any defects that explains the observed phenotype Determine what goes wrong in the peripodial epithelium in the how mutants Acknowledgment Dr. Craig Woodard Tina Fortier The Vibrant Fly Lab Team The National Science Foundation And All the People who have inspired my Scientific Career