Abstract
Pathological hallmarks of Alzheimer’s disease (AD) include deposition and accumulation of amyloid- β (Aβ), neurofibrillary tangle formation, and neuronal loss. Pathogenesis of presymptomatic disease stages remains elusive, although studies suggest that the early structural and functional alterations likely occur at neuronal dendritic spines. Presymptomatic alterations may also affect different CNS cell types. However, specific contributions of these cell types as cause or consequence of pathology are difficult to study in vivo. There is a shortage of relatively simple, well-defined, and validated in vitro models that allow a straightforward interpretation of results and recapitulate aspects of pathophysiology. For instance, dissecting the AD-related processes (e.g., neurotoxicity vs. synaptotoxicity) may be difficult with the common cell-based systems such as neuronal cell lines or primary neurons. To investigate and characterize the impact of reactive astrocytes on neuronal morphology in the context of AD-related cues, we modified an in vitro co-culture assay of primary mouse neurons and primary mouse astrocytes based on the so-called Banker “sandwich” co-culture assay. Here, we provide a simple and modular assay with fully differentiated primary mouse neurons to study the paracrine interactions between the neurons and the astrocytes in the co-culture setting. Readouts were obtained from both cell types in our assay. Astrocyte feeder cells were pre-exposed to neuroinflammatory conditions by means of Aβ42, Aβ40, or lipopolysaccharide (LPS). Non-cell autonomous toxic effects of reactive astrocytes on neurons were assessed using the Sholl analysis to evaluate the dendritic complexity, whereas synaptic puncta served as a readout of synaptotoxicity. Here, we show that astrocytes actively contribute to the phenotype of the primary neurons in an AD-specific context, emphasizing the role of different cell types in AD pathology. The cytokine expression pattern was significantly altered in the treated astrocytes. Of note, the impact of reactive astrocytes on neurons was highly dependent on the defined cell ratios. Our co-culture system is modular, of low cost, and allows us to probe aspects of neurodegeneration and neuroinflammation between the two major CNS cell types, neurons, and astrocytes, under well-defined experimental conditions. Our easy-to-follow protocol, including work-flow figures, may also provide a methodological outline to study the interactions of astrocytes and neurons in the context of other diseases in the future.
Highlights
Alzheimer’s disease (AD) is the most prevalent form of dementia in the elderly and its incidence will significantly increase in the upcoming decades, with an estimated number of 66–76 million by 2030 and 115–136 million by 2050, respectively (Prince et al, 2013; Cummings et al, 2018)
Astrocytes were derived from the tissue dissection of cortices, while neurons were derived from the tissue dissection of hippocampi
To study the effects on the neuronal phenotype, and track changes occurring in astrocytes upon experimental manipulation, we applied the following modifications to the assay: a) glass coverslips on the dish bottom were equipped with three wax dots arranged in a triangular fashion; b) primary mouse astrocytes were plated as a feeder layer on these wax dot-coverslips serving as a physical barrier between feeder layer and neurons; c) pre-treatment of astrocytes with compounds induced a reactive astrocyte phenotype; and d) from an independent experiment, the neurons differentiated for 14 days in a co-culture were inverted over the pre-treated astrocytes for 24 h to model the indirect effects of Aβ42 and LPS on mediated neurons via astrocytes
Summary
Alzheimer’s disease (AD) is the most prevalent form of dementia in the elderly and its incidence will significantly increase in the upcoming decades, with an estimated number of 66–76 million by 2030 and 115–136 million by 2050, respectively (Prince et al, 2013; Cummings et al, 2018). Recent observations indicate that neuroinflammation represents a disease element promoting that promotes AD development and progression (De Strooper and Karran, 2016). In pre-clinical AD models, microglia and astrocytes were shown to produce a variety of pro-inflammatory cytokines, suggestive of chronic neuroinflammation, which is apparent even before the development of full-blown disease features (Guillot-Sestier et al, 2015; Heneka et al, 2015; De Strooper and Karran, 2016). Existing shortages of the appropriate pre-clinical models leave the exact disease onset, linearity of disease events, and mechanistic drivers of progression in AD unknown (De Strooper and Karran, 2016; Drummond and Wisniewski, 2017). AD mouse models mimic features of AD pathogenesis to a certain degree, such as Aβ plaque deposition, without presenting the whole pathological disease profile (Drummond and Wisniewski, 2017)
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