Abstract
Alzheimer’s disease is the most common form of age-related dementia. At least 15 mutations in the human gene PRESENILIN 2 (PSEN2) have been found to cause familial Alzheimer’s disease (fAD). Zebrafish possess an orthologous gene, psen2, and present opportunities for investigation of PRESENILIN function related to Alzheimer’s disease. The most prevalent and best characterized fAD mutation in PSEN2 is N141I. The equivalent codon in zebrafish psen2 is N140. We used genome editing technology in zebrafish to target generation of mutations to the N140 codon. We isolated two mutations: psen2N140fs, (hereafter “N140fs”), causing truncation of the coding sequence, and psen2T141_L142delinsMISLISV, (hereafter “T141_L142delinsMISLISV”), that deletes the two codons immediately downstream of N140 and replaces them with seven codons coding for amino acid residues MISLISV. Thus, like almost every fAD mutation in the PRESENILIN genes, this latter mutation does not truncate the gene’s open reading frame. Both mutations are homozygous viable although N140fs transcripts are subject to nonsense-mediated decay and lack any possibility of coding for an active γ-secretase enzyme. N140fs homozygous larvae initially show grossly normal melanotic skin pigmentation but subsequently lose this as they grow while retaining pigmentation in the retinal pigmented epithelium. T141_L142delinsMISLISV homozygotes retain faint skin melanotic pigmentation as adults, most likely indicating that the protein encoded by this allele retains weak γ-secretase activity. Null mutations in the human PRESENILIN genes do not cause Alzheimer’s disease so these two mutations may be useful for future investigation of the differential effects of null and fAD-like PRESENILIN mutations on brain aging.
Highlights
The first two transmembrane domains (TMDs) of PRESENILIN 2 (PSEN2) are thought to be necessary for endoplasmic reticulum (ER) localisation [11] while a conserved sequence near the N-terminal is bound by Adaptor Complex AP-1 to direct PSEN2 protein to late endosomes / lysosomes [10]
The zebrafish PRESENILIN 2 is required for normal adult melanotic skin pigmentation progeny of the mosaic, mutation-carrying G0 fish may be heterozygous for such random mutations
The second mutation is a deletion of 7 nucleotides causing a frameshift that does truncate the coding sequence, N140fs, due to a premature termination codon (PTC) at the 142nd codon position
Summary
Alzheimer’s disease (AD) is a progressive neurodegenerative disorder, and is the most common form of age-related dementia, accounting for 50–75% of dementia cases worldwide [1]. The first two transmembrane domains (TMDs) of PSEN2 are thought to be necessary for ER localisation [11] while a conserved sequence near the N-terminal is bound by Adaptor Complex AP-1 to direct PSEN2 protein to late endosomes / lysosomes [10]. The C-terminal fragment of SILV is processed by the γ-secretase complex to release an intracellular domain fragment [25] into endosomal precursors to form amyloid fibrils These become melanosomes [27,28]. While homology-directed repair (HDR) after CRISPR Cas cleavage at the relevant site in zebrafish psen was not successful, we did find products of non-homologous end joining (NHEJ) that will prove useful in future analyses We identified both a frameshift mutation and a reading frame-preserving indel mutation close to the N141-equivalent codon of zebrafish psen (N140). We discovered that the γ-secretase activity of Psen (unlike that of Psen1) appears essential for melanotic pigment formation in the skin of zebrafish adults but not in their retinal pigmented epithelium
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