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Tri-culture modeling of neuroinflammation, neurodegeneration, and neuroprotection
Abstract
The
study of neurodegenerative diseases, such as Alzheimer's disease (AD),
has long been a complex and challenging task. One of the major hurdles
in understanding these diseases is the difficulty in recapitulating the
complex interactions between neurons, astrocytes, and microglia in a
laboratory setting. In recent years, researchers have made significant
progress in developing triculture models that combine these three cell
types, allowing for a more accurate representation of the cellular
context of the human brain. This commentary discusses the recent
advancements and importance of using tri-culture model systems in
clarifying the pathophysiology of AD and discusses the recent article by
Kim et al. (2024) published in the Journal of Alzheimer's Disease.
The human brain contains over 100 billion neurons(Actually, you're out-of-date, it's 80 billion), each with unique morphology, function, and connectivity.1–3
Understanding the interactions and coordination between these cells
during physiological and pathological states is crucial for elucidating
the mechanisms underlying neurodegenerative diseases, such as
Alzheimer's disease (AD). Neuroinflammation is a hallmark of many
neurodegenerative diseases, including AD, and is mediated by microglia,
which play a critical role in the initiation and progression of
neurodegenerative diseases. The relation between microglia and
neuroinflammation is bi-directional.4–6
These findings have led researchers to study these complex processes in
detail and how it contributes to neurodegeneration using model systems
combining neurons, astrocytes and microglia.
While
microglial monocultures have been a cost effective and valuable tool
for studying the responses of these cells to specific inflammatory
stimuli or toxins, it has several limitations. One of the main drawbacks
is that they do not accurately reflect the in vivo state, where
microglia interact with other cell types in a complex and dynamic
manner. Therefore, monocultures may not fully capture the microglial
behavior and function in the context of disease leading researchers to
recognize the need to move beyond monocultures and study microglia in
more complex and physiologically relevant settings. Co-cultures, which
involve the simultaneous culture of microglia with other cell types,
have been developed as means to better mimic the in vivo niche and gain a
more comprehensive understanding of microglial function in disease.
To
model the cellular context of the human brain, Haenseler et al.
co-cultured induced pluripotent stem cell (iPSC)-derived microglia with
cortical neurons and reported characteristic microglial features,
including expression of microglia-specific markers, dynamic
ramifications, and phagocytic capacity, along with enhanced homeostatic
gene expression and anti-inflammatory cytokine profiles compared to
monocultures.7 However, studies have shown that microglia are influenced by the secreted molecules from neurons and astrocytes.8
Since then, several groups have developed more advanced triculture
models that better mimic the in vivo environment. For example, Park et
al. developed a 3D tri-culture model system where neurons and astrocytes
were differentiated from human neural progenitor cells first, followed
by the addition of adult immortalized human microglia cells mimicking
different stages of AD.9
This model demonstrated amyloid-β (Aβ) aggregation, phosphorylated tau
formation, and increased proinflammatory chemokine/cytokine expression
accompanied by microglial recruitment and marked neuron/astrocyte loss,
suggesting its validity as a tool to investigate neuroinflammatory
mechanisms underlying AD pathophysiology.9
In another study, Guttikonda et al. employed a tri-culture system
comprising human iPSC-derived neurons, microglia, and astrocytes to
investigate the role of complement C3 in AD, revealing a bidirectional
signaling between microglia and astrocytes that led to increased C3
levels under pathological conditions.10
Bassil et al. developed a long-term triculture platform using human
iPSC-derived neurons, microglia, and astrocytes, which allowed them to
replicate the key features of AD, including Aβ plaques, dystrophic
neurites, synaptic loss, dendrite retraction, axon fragmentation,
phosphorylated tau induction, and neuronal cell death.11
By adding soluble Aβ species to the system, they found that
iPSC-derived microglia were able to provide neuroprotection by
internalizing and compacting Aβ, not only through generating but also
surrounding plaques.11
Despite
their potential, these models can be limited by their complexity and
high cost, making them inaccessible to many researchers. Goshi et al.
developed a tri-culture model using primary cortical cells from neonatal
rats, which could also mimic in vivo neuroinflammatory responses.12
This model is suggested to be more accurate than traditional mono- and
co-cultures as it captured CNS response to lipopolysaccharide exposure
and glial scarring in a scratch assay, and neuronal rescue from
glutamate-induced excitotoxicity, making it a valuable tool for studying
neuroinflammation in vitro.12
To further advance the knowledge in the context of Aβ induced
neurodegeneration and associated neuroinflammatory responses, the same
group of researchers report the use of primary rat cortical tri-culture
model to study the internalization of Aβ by microglia in the presence of
neurons and astrocytes in the latest issue of the Journal of Alzheimer's Disease.13
They have used the model to characterize neural and microglial response
to Aβ exposure compared to neuronal-astrocyte co-culture and microglial
monoculture. They exposed the cultures to fluorescently labeled Aβ
(FITC-Aβ) particles and using epifluorescence microscopy, live cell
imaging and cytokine profiling, they report that the tri-culture model
comprising microglia was able to clear the FITC-Aβ particles more
efficiently than that observed in the co-culture model.13
This will be important given the growing body of evidence that Aβ
clearance by microglia in CNS as well as macrophages (the counterparts
of microglia) in the peripheral system, plays crucial role in the
clearance of Aβ and the progression of neurodegeneration in AD.14–17 These findings align with previous research, including studies by Baxter et al.,18
which showed that the loss of normal microglial function in disease
states can be rescued by co-culturing with astrocytes and neurons, the
study by Phadke et al.,19
demonstrating that microglia could suppress neuronal activity and alter
synaptic function in a tri-culture model system and the study by
Luchena et al.20
reporting that microglia are less inflammatory, astrocytes are less
reactive, and neurons display a more mature morphology, in the
tri-culture system making it a powerful tool to study neuroinflammation
and neurodegeneration in the context of AD and other neurodegenerative
diseases. While the study by Kim et al. provides valuable insights into
the interactions between microglia and neurons in the context of Aβ
exposure, it is crucial to consider the potential influence of genetic
variations on these responses. Future studies should also address the
response of these cells to tau proteins and should incorporate genetic
factors such as APP, PSEN, APOE, TREM2, etc. to provide a more comprehensive understanding of the variability in neuronal and microglial responses.
Moreover,
while rodent microglia may not perfectly replicate the human disease
context, these studies can still offer valuable insights into the
fundamental mechanisms underlying neuroinflammation, neurodegeneration,
and neuroprotection during disease progression and could be pivotal in
high-throughput screening efforts for target identification, assay
development, and therapeutic drug discovery. By understanding the basic
mechanisms, researchers can then extrapolate their findings to the human
context, potentially leading to the development of new therapeutic
strategies for the treatment of neurodegenerative diseases. In
conclusion, these tri-culture model systems offer a promising platform
for modeling and testing mechanisms associated with microglia in the
presence of neurons and astrocytes, providing a more accurate
representation of the cellular context of the human brain and AD.
However, it is essential to exercise caution when interpreting results,
taking into account the origin and condition of cells used, to ensure
that findings are accurately translated to the human context.
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