Xenografted human iPSC-derived neurons with the familial Alzheimer's disease APP.sup.V717I mutation reveal dysregulated transcriptome signatures linked to synaptic function and implicate LINGO2 as a disease signaling mediator

Alzheimer's disease (AD) is the most common cause of dementia, and disease mechanisms are still not fully understood. Here, we explored pathological changes in human induced pluripotent stem cell (iPSC)-derived neurons carrying the familial AD APP.sup.V717I mutation after cell injection into th...

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Bibliographic Details
Published inActa neuropathologica Vol. 147; no. 1
Main Authors Qu, Wenhui, Lam, Matti, McInvale, Julie J, Mares, Jason A, Kwon, Sam, Humala, Nelson, Mahajan, Aayushi
Format Journal Article
LanguageEnglish
Published Springer 01.06.2024
Subjects
Advertising executives
Alzheimer's disease
Brain
Comparative analysis
Diseases
Genes
Genetic aspects
Neurons
Physiological aspects
RNA
Stem cells
Target marketing
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ISSN0001-6322
DOI10.1007/s00401-024-02755-5

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Summary:Alzheimer's disease (AD) is the most common cause of dementia, and disease mechanisms are still not fully understood. Here, we explored pathological changes in human induced pluripotent stem cell (iPSC)-derived neurons carrying the familial AD APP.sup.V717I mutation after cell injection into the mouse forebrain. APP.sup.V717I mutant iPSCs and isogenic controls were differentiated into neurons revealing enhanced A.sub.42 production, elevated phospho-tau, and impaired neurite outgrowth in APP.sup.V717I neurons. Two months after transplantation, APP.sup.V717I and control neural cells showed robust engraftment but at 12 months post-injection, APP.sup.V717I grafts were smaller and demonstrated impaired neurite outgrowth compared to controls, while plaque and tangle pathology were not seen. Single-nucleus RNA-sequencing of micro-dissected grafts, performed 2 months after cell injection, identified significantly altered transcriptome signatures in APP.sup.V717I iPSC-derived neurons pointing towards dysregulated synaptic function and axon guidance. Interestingly, APP.sup.V717I neurons showed an increased expression of genes, many of which are also upregulated in postmortem neurons of AD patients including the transmembrane protein LINGO2. Downregulation of LINGO2 in cultured APP.sup.V717I neurons rescued neurite outgrowth deficits and reversed key AD-associated transcriptional changes related but not limited to synaptic function, apoptosis and cellular senescence. These results provide important insights into transcriptional dysregulation in xenografted APP.sup.V717I neurons linked to synaptic function, and they indicate that LINGO2 may represent a potential therapeutic target in AD.
ISSN:0001-6322
DOI:10.1007/s00401-024-02755-5