Zebrafish as a Model to Investigate the Disease Mechanisms of Infantile Neuronal Ceroid Lipfuscinosis Nicole Brant and Dr. Wendy Boehmler, Department of.

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Zebrafish as a Model to Investigate the Disease Mechanisms of Infantile Neuronal Ceroid Lipfuscinosis Nicole Brant and Dr. Wendy Boehmler, Department of Biology, York College of Pennsylvania eurons%20confocal%20mu1a%20dcx.jpg Introduction Infantile neuronal ceroid lipfuscinosis (INCL) is a devastating neurodegenerative disorder that destroys neurons in certain tissues of the central nervous system such as the thalamus, cortex, and cerebellum. INCL is caused by a mutation in the PPT1 gene which encodes palmitoyl protein thioesterase 1. PPT1 is a lysosomal enzyme that plays a major role in the degradation of lipid-modified proteins. How PPT1 deficiency leads to selective central nervous system degeneration is unclear. Neurons have an altered endoplasmic reticulum morphology. Microarray analyses on INCL brain tissues shows an upregulation of inflammatory genes. The post-mitotic nature of neurons may contribute to their selective degeneration. While the gene mutation has been identified, there is still a need to investigate the neurobiology of the disease course throughout early development and to assess potential therapeutic treatments. Mouse models of INCL have provided significant clues to the biological basis of the disease, however such studies can be slow, laborious, and expensive to perform. Zebrafish, a small vertebrate, are becoming the organism of choice for modeling diseases and for drug discovery. The genome is fully sequenced. Breeding pairs can produce hundreds of embryos. Embryos develop ex utero, develop rapidly, and are transparent Objectives 1.Determine if there is expression of the PPT1 gene in adult zebrafish tissues. 2.Determine if there is spatial and temporal expression of the PPT1 gene during zebrafish development. Methods Searches of expressed sequence tag databases ( led to the identification of a potential zebrafish PPT1 homolog (Gene Accession number NM213339). RT-PCR was conducted using RNA collected from adult zebrafish and embryos. Figure 1: RT-PCR analysis of PPT1 from adult zebrafish. The PPT1 gene was amplified from adult zebrafish brain, gut, and muscle RNA. The primers used encompassed the predicted ATG start codon and stop codon to produce an amplicon of 1033 base pairs (bp). Primer sequences: forward 5’AGATTGAATAATGGCTCCACC3’ and reverse 5’TATCTGAGACGGTAGTTACGA3’. Conclusion 1.The data presented here represents the first analysis of temporal and spatial expression of the PPT1 gene in developing zebrafish embryos. 2.PPT1 is also expressed in adult zebrafish in the brain, gut, and muscle. 3.Sequence comparisons and syntenic analysis supports the identification of a novel zebrafish PPT1 homolog. Future Experiments Perform a morpholino knockdown of PPT1 gene to assess any gross morphological abnormalities in development. Literature Cited Cooper, Jonathan D., Russel, Claire and Mitchison, Hannah, M Progress towards understanding disease mechanisms in small vertebrate models of neuronal ceroid lipofuscinosis. Biochimica et Biophysica Acta Woods, I. G., Wilson, C., Friedlander, B., Chang, P., Reyes, D. K., Nix, R., Kelly, P. D., Chu, F., Postlethwait, J. H., and W. S. Talbot The zebrafish gene map defines ancestral vertebrate chromosomes. Genome Research 15: Gene Name Zebrafish Chromosome Human Chromosome PPT1191 dnajc8191 flj mhcuaa191 trh3191 tpm3b191 ctps191 hdac1191 flj rbb4191 fuca1191 bmp8191 col9a2191 ilf2191 sfpq191 pum1191 cap1191 rpl11191 Figure 4: Comparison of zebrafish and human PPT1. Human and zebrafish PPT1 amino acid sequences were aligned using CLUSTALW. Dashes in sequences allow optimal alignment for amino acid insertions/deletions. Identical amino acids are highlighted by asterisks and conserved are highlighted by dots. Collected tissues from the brain, eye, gut, heart, and muscle and 24, 48, and 72 hours post fertilization (hpf) embryos PCR Denature for 30 sec. at 94 o C Annealing for 30 sec. at 48 o C Elongation for 1 min. at 72 o C 30 cycles RNA isolation with phenol/chloroform extraction Reverse Transcription cDNA Zebrafish PPT1 gene was successfully cloned into a pDrive and sequenced Results Figure 2: RT-PCR analysis of PPT1 from 24, 48, and 72 hpf embryos. The PPT1 gene was amplified from 24, 48, and 72 hpf embryo RNA. Primers encompassed the entire gene to produce the predicted 1033bp amplicon. Table 1: Markers and Genes Syntenic with PPT1 Genes in Zebrafish and Humans. A whole-mount in situ hybridization was performed on 24, 48, and 72 hpf embryos. Figure 3: Expression of the palmitoyl protein thioesterase 1 gene. Lateral views of 24 (A, D), 48 (B, E), and 72 (C, F) hpf embryos. Note the sense probe (A, B, C) and the antisense probe (D, E, F). B-brain, E-eye, SC-spinal cord Collected 24, 48, and 72 hpf embryos, stored them in MeOH, made the sense and antisense probes and reagents Staining and washing, stored embryos and took pictures Permeabilization of the embryos and hybridization of the RNA probe Washes Incubation with anti- DIG antibody alkaline phosphase Washes A 24 hpfD 24 hpf E 48 hpfB 48 hpf F 72 hpfC 72 hpf B E SC B E B E Acknowledgements I would like to thank Dr. Boehmler for all of her time and guidance.