Abstract
Amyloid β (Aβ) forms aggregates in the Alzheimer’s disease brain and is well known for its pathological roles. Recent studies show that it also regulates neuronal physiology in the healthy brain. Whether Aβ also regulates glial physiology in the normal brain, however, has remained unclear. In this article, we describe the discovery of a novel signaling pathway activated by the monomeric form of Aβ in vitro that plays essential roles in the regulation of microglial activity and the assembly of neocortex during development in vivo. We find that activation of this pathway depends on the function of amyloid precursor (APP) and the heterotrimeric G protein regulator Ric8a in microglia and inhibits microglial immune activation at transcriptional and post-transcriptional levels. Genetic disruption of this pathway during neocortical development results in microglial dysregulation and excessive matrix proteinase activation, leading to basement membrane degradation, neuronal ectopia, and laminar disruption. These results uncover a previously unknown function of Aβ as a negative regulator of brain microglia and substantially elucidate the underlying molecular mechanisms. Considering the prominence of Aβ and neuroinflammation in the pathology of Alzheimer’s disease, they also highlight a potentially overlooked role of Aβ monomer depletion in the development of the disease.
Introduction
Aβ, a core component of amyloid plaques in the Alzheimer’s disease brain, is well known to form oligomers under disease conditions. Studies have shown that the oligomers formed by Aβ are highly toxic, with wide-ranging effects including inhibition of neurotransmitter release, depletion of synaptic vesicle pools, disruption of postsynaptic organization and function, and impairment of multiple forms of synaptic plasticity (Gulisano et al., 2018; He et al., 2019; Kim et al., 2013; Lauren et al., 2009; Lazarevic et al., 2017; Parodi et al., 2010; Puzzo et al., 2008; Shankar et al., 2008; Walsh et al., 2002; Yang et al., 2015; Zott et al., 2019). These effects likely significantly underpin the pathogenic role of Aβ in Alzheimer’s disease and contribute to neuron loss and cognitive decline in patients. Besides its pathological roles, recent studies show that Aβ is also produced in the healthy brain by neurons in a neural activity-dependent manner and regulates the normal physiology of neurons (Cirrito et al., 2005; Fogel et al., 2014; Galanis et al., 2021; Garcia-Osta and Alberini, 2009; Gulisano et al., 2018; Gulisano et al., 2019; Morley et al., 2010; Palmeri et al., 2017; Puzzo et al., 2008; Zhou et al., 2022). For example, consistent with studies showing that Aβ monomers and low molecular weight oligomers positively regulate synaptic function and plasticity, administration of these molecules in vivo has been found to improve learning and memory in animals (Fogel et al., 2014; Garcia-Osta and Alberini, 2009; Gulisano et al., 2018; Gulisano et al., 2019; Morley et al., 2010; Palmeri et al., 2017; Puzzo et al., 2008). Furthermore, recent studies have shown that Aβ monomers directly promote synapse formation and function and homeostatic plasticity, processes crucial to normal cognitive function (Galanis et al., 2021; Kamenetz et al., 2003; Zhou et al., 2022). Together, these findings have provided crucial insights into the physiological roles that Aβ plays in regulating normal neuronal function in the brain. However, it remains unclear if Aβ also regulates the physiology of glia, nonneuronal cells that also play important roles in normal brain function.
Microglia and astrocytes, two of the major glial cell types in the brain, are known to play critical roles in the normal development, function, and plasticity of the brain circuitry (Barres, 2008; Schafer and Stevens, 2015). They coordinately regulate, among others, the spatiotemporally specific expression of immune cytokines in the brain that regulate numerous processes of brain circuit development, function, and plasticity (Zipp et al., 2023). For example, in the thalamus, a key relay station in the visual pathway, populations of astrocytes have been found to activate the expression of interleukin-33 in a neural activity-dependent manner, induce activity-dependent elimination of supernumerary synapses, and promote the maturation of the visual circuitry in early postnatal life (Vainchtein et al., 2018). In the adult hippocampus, in contrast, astrocytes have been found to activate the expression of interleukin-33 under neuronal activity blockade and induce homeostatic synaptic plasticity that maintains circuit activity balance (Wang et al., 2021). In the striatum and the neocortex, not only have astrocytes but also have microglia been observed to activate the expression of TNFα upon changes in neural circuit activity and induce homeostatic synaptic plasticity that dampens circuit perturbation (Heir et al., 2024; Lewitus et al., 2016; Stellwagen and Malenka, 2006). In the clinic, the induction of microglial release of cytokines such as TNFα also underpins the application of repetitive transcranial magnetic stimulation, a noninvasive brain stimulation technique frequently used to induce cortical plasticity and treat pharmaco-resistant depression (Eichler et al., 2023). In neurodegenerative diseases such as Alzheimer’s disease, glial activation and brain cytokine elevation are also key pathologic factors in disease development (Colonna and Butovsky, 2017; Patani et al., 2023). Furthermore, elevated TNFα expression by microglia also underlies interneuron deficits and autism-like phenotype linked to maternal immune activation (Yu et al., 2022). Thus, the precise regulation of glial cytokine expression in the brain plays a key role in the normal development and function of the brain and its dysregulation is linked to common neurodevelopmental and neurodegenerative diseases. However, how glial cytokine expression is mechanistically regulated by cell-cell communication in the brain have remained largely unknown.
In this article, we report the discovery of a novel microglial signaling pathway activated in vitro by Aβ, the neuron-produced peptide at the center of Alzheimer’s disease, that plays a crucial role in precisely regulating the levels of microglial cytokine expression and activity and ensuring the proper assembly of neuronal laminae during cerebral cortex development. We first came across evidence for this pathway in our study of the function of ric8a. ric8a encodes a guanine nucleotide exchange factor (GEF) and molecular chaperone for several classes of heterotrimeric G proteins, which become severely destabilized upon ric8a loss of function (Gabay et al., 2011; Papasergi-Scott et al., 2018; Tall et al., 2003). We found that deletion of ric8a during cortical development resulted in cortical basement membrane degradation, neuronal ectopia, and laminar disruption. However, unlike in classic models of cobblestone lissencephaly, these phenotypes resulted not from ric8a deficiency in brain neural cell types, but from deficiency in microglia. Ric8a-regulated Gα proteins are known to bind to the cytoplasmic domain of the amyloid precursor protein (APP) and mediate key branches of APP signaling in several cell types (Fogel et al., 2014; Milosch et al., 2014; Nishimoto et al., 1993; Ramaker et al., 2013). The ric8a cortical phenotypes also resemble those in triple or double mutants of APP family and pathway genes (Guenette et al., 2006; Herms et al., 2004), suggesting functional interactions. Indeed, we found that app deficiency in brain microglia also underpins ectopia formation in app family gene mutants. Furthermore, we found that APP and Ric8a form a pathway in microglia that is specifically activated by the monomeric form of Aβ and that this pathway normally inhibits the transcriptional and post-transcriptional expression of immune cytokines by microglia.
Results
Cortical ectopia in ric8a-emx1-cre mutants results from non-neural deficiency
To study of the function of ric8a, a GEF as well as molecular chaperone for Gα proteins (Gabay et al., 2011; Papasergi-Scott et al., 2018; Tall et al., 2003), in neocortical development, we deleted a conditional ric8a allele (Ma et al., 2012; Ma et al., 2017) using emx1-cre, a cre line designed to target dorsal forebrain neural progenitors in mice (Gorski et al., 2002). We found it result in ectopia formation exclusively in the lateral cortex of the perinatal mutant brain (Fig. 1a-d). Birth-dating showed that the ectopia consisted of both early and late-born neurons (Supplemental Fig. 1). Consistent with this observation, neurons in the ectopia also stained positive for both Ctip2 and Cux1, genes specific to lower and upper-layer neurons, respectively. Interestingly, in cortical areas without ectopia, radial migration of early- and late-born neurons appeared largely normal as shown by birth-dating as well as Cux1 and Ctip2 staining (Supplemental Fig. 2). This suggests that cell-autonomous defects in neurons are unlikely the cause of the ectopia. At E16.5, clear breaches in the pial basement membrane of the developing cortex were already apparent (Supplemental Fig. 3). However, unlike classic models of cobblestone lissencephaly, where radial glial fibers typically retract, radial glial fibers in ric8a mutants instead extended beyond the breaches. This argues against radial glial cell adhesion defects since they would be predicted to retract. Furthermore, in areas without ectopia, we also observed normal localization of Cajal-Retzius cells, expression of Reelin, and splitting of the preplate, arguing against primary defects in Cajal-Retzius cells. In cobblestone lissencephaly, studies show that ectopia result from primary defects in radial glial maintenance of the pial basement membrane (Beggs et al., 2003; Graus-Porta et al., 2001; Moore et al., 2002; Satz et al., 2010). In ric8a mutants, we observed large numbers of basement membrane breaches at E14.5, almost all associated with ectopia (Supplemental Fig. 4). In contrast, at E13.5, although we also observed significant numbers of breaches, none was associated with ectopia. This indicates that basement membrane breaches similarly precede ectopia in ric8a mutants. However, at E12.5, despite a complete lack of basement membrane breaches, we observed increased numbers of laminin-positive debris across the lateral cortex, both beneath basement membrane segments with intact laminin staining and beneath segments with disrupted laminin staining, the latter presumably sites of future breach (Supplemental Fig. 5). As a major basement membrane component, the increased amounts of laminin debris suggest increased degradative activity within the developing cortex. Thus, these results indicate that excessive basement membrane degradation, but not defective maintenance, is likely a primary cause of cortical ectopia in ric8a mutants.
To determine the cell type(s) genetically responsible for cortical basement membrane degradation and ectopia in ric8a mutants, we employed a panel of cre lines (Fig. 1e-h’). To target Cajal-Retzius cells, we employed wnt3a-cre (Yoshida et al., 2006) but found ric8a deletion using wnt3a-cre did not result in ectopia. To target postmitotic excitatory and inhibitory neurons, we employed nex-cre (Goebbels et al., 2006) and dlx5/6-cre (Stenman et al., 2003) respectively but similarly found neither result in ectopia. These results point to ric8a requirement in cell types other than post-mitotic neurons. To test the involvement of neural progenitors, we employed nestin-cre (Graus-Porta et al., 2001). Previous studies show that deletion of β1 integrin and related genes by emx1-cre and nestin-cre results in similar ectopia phenotypes (Belvindrah et al., 2006; Graus-Porta et al., 2001; Huang et al., 2006; Niewmierzycka et al., 2005). To our surprise, deletion of ric8a by nestin-cre did not result in ectopia (Ma et al., 2017) (Fig. 1g-g’). Since nestin-cre-mediated deletion in neural progenitors is inherited by post-mitotic neurons and astrocytes, this indicates that the combined deletion of ric8a from all these cell types does not lead to ectopia. The onset of nestin-cre expression is, however, developmentally slightly later than that of emx1-cre (Gorski et al., 2002). To assess the potential contribution of this temporal difference, we employed foxg1-cre, a cre line expressed in forebrain neural progenitors starting from E10.5 (Hebert and McConnell, 2000). We found that ric8a deletion using foxg1-cre still failed to produce ectopia (Fig. 1h-h’). Thus, these results strongly argue against the interpretation that ric8a deficiency in neural cell lineages is responsible for basement membrane degradation and ectopia in ric8a mutants.
During embryogenesis, the neural tube undergoes epithelial-mesenchymal transition giving rise to neural crest cells (Leathers and Rogers, 2022). This process involves region-specific basement membrane breakdown that resembles the ric8a mutant phenotype. To determine if ectopic epithelial-mesenchymal transition plays a role, we examined potential changes in neuro-epithelial cell fates in the mutant cortex. We found that cortical neural progenitors expressed Pax6, Nestin, and Vimentin normally (Supplemental Fig. 6). Cell proliferation in the ventricular zone was also normal. Furthermore, although ric8a regulates asymmetric cell division in invertebrates (Afshar et al., 2004; Couwenbergs et al., 2004; David et al., 2005; Hampoelz et al., 2005; Wang et al., 2005), we observed no significant defects in mitotic spindle orientation at the ventricular surface. Additionally, no ectopic expression of neural crest markers or Wnt pathway activation was observed (Supplemental Fig. 7). Altogether, these results further indicate that non-neural-cell deficiency is responsible for ectopia formation in ric8a mutants.
Microglial ric8a deficiency is responsible for ectopia formation
To assess the role of non-neural cell types, we turned our attention to microglia since RNA-seq studies show that brain microglia express emx1 at a significant level (Zhang et al., 2014). To determine if emx1-cre is expressed and active in microglia, we isolated microglia from ric8a-emx1-cre mutants. We found that emx1-cre mediated ric8a deletion resulted in altered cytokine expression in microglia (Supplemental Fig. 8a-b). This indicate that emx1-cre is expressed and active in microglia and deletes ric8a. In further support of this interpretation, we found that when crossed to a reporter, emx1-cre resulted in the expression of reporter gene in microglia (Supplemental Fig. 8c-c”). It also resulted in the reduction of ric8a mRNA levels in in microglia in ric8a-emx1-cre mutants (Supplemental Fig. 8d). To determine the specific significance of ric8a deletion from microglia alone, we next employed a microglia-specific cx3cr1-cre (Yona et al., 2013). Like emx1-cre mutants, ric8a-cx3cr1-cre mutant microglia also showed elevated cytokine secretion and transcription in comparison to control microglia upon stimulation by lipopolysaccharide (LPS) (Fig. 2a-b). Similar results were also obtained with stimulation by polyinosinic-polycytidylic acid (poly I:C), an intracellular immune activator. Thus, these results indicate that ric8a deficiency in microglia results in broad increases in microglial sensitivity to immune stimulation.
To determine if microglial ric8a deficiency alone is sufficient to cause cortical ectopia in vivo, we examined ric8a-cx3cr1-cre mutants but found that it did not affect either basement membrane integrity or cortical layering (Fig. 2c). We reasoned that this may be related to the fact that ric8a mutant microglia only show heightened activity upon stimulation but not under basal unstimulated conditions (Fig. 2a-b) but elevated microglial activity may be needed for basement membrane degradation and ectopia formation. To test this possibility, we employed in utero LPS administration to activate microglia during cortical development. We found that over 50% of ric8a-cx3cr1-cre mutant neonates showed ectopia when administered LPS at E11.5-12.5 (10 of 19 mutant neonates examined) (Fig. 2d). In contrast, no cortical ectopia were observed in any of the 32 littermate controls that were similarly administered LPS. This indicates that only the combination of microglial ric8a deficiency and immune activation leads to ectopia formation. In emx1-cre mutants, ectopia develop without LPS administration (Fig. 1). We suspect that this may be due to concurrent ric8a deficiency in neural cell types, which may result in deficits that mimic immune stimulation. In the embryonic cortex, for example, studies have shown that large numbers of cells die starting as early as E12 (Blaschke et al., 1996; Blaschke et al., 1998). Radial glia and neuronal progenitors play critical roles in the clearance of apoptotic cells and cellular debris in the brain (Amaya et al., 2015; Ginisty et al., 2015; Lu et al., 2011) and Ric8a-dependent heterotrimeric G proteins promotes this function in both professional and non-professional phagocytic cells (Billings et al., 2016; Flak et al., 2020; Pan et al., 2016; Preissler et al., 2015; Zhang et al., 2023). Thus, ric8a deficiency in radial glia may potentially result in accumulation of apoptotic cell debris in the embryonic brain that stimulate microglia. To test this, we next additionally deleted ric8a from radial glia in the ric8a-cx3cr1-cre microglial mutant background by introducing nestin-cre. We have shown that ric8a deletion by nestin-cre alone does not result in ectopia (Fig. 1g-g’). However, we found that, like deletion by emx1-cre, ric8a deletion by the dual cre combination of cx3cr1-cre and nestin-cre also resulted in severe ectopia in all double cre mutants (6 of 6 examined) (Fig. 2f). Thus, these results indicate that elevated immune activation of ric8a deficient microglia during cortical development is responsible for ectopia formation.
Microglial app deficiency also results in ectopia formation
In the large numbers of cobblestone lissencephaly and related cortical ectopia mutants, besides the lateral cortex, severe ectopia are typically also observed at the cortical midline (Beggs et al., 2003; Belvindrah et al., 2006; Graus-Porta et al., 2001; Huang et al., 2006; Moore et al., 2002; Niewmierzycka et al., 2005; Satz et al., 2010). There are only a few mutants including the ric8a-emx1cre mutant that are exception, in that the ectopia are not observed at the cortical midline but are instead exclusively located to the lateral cortex (Fig. 1). The other mutants in this unique group include the app/aplp1/2 triple (Herms et al., 2004) and apbb1/2 double knockouts (Guenette et al., 2006). This suggests that similar mechanisms involving microglia may underlie ectopia formation in ric8a-emx1cre, app/aplp1/2, and apbb1/2 mutants. Independent studies also point to a role of non-neuronal cells in ectopia formation in app family gene mutants. For example, unlike the triple knockout, which causes neuronal over-migration, specific app knockdown in cortical neurons during development results in under-instead of over-migration of targeted neurons (Young-Pearse et al., 2007). Furthermore, Ric8a-regulated Gα proteins play a conserved role in mediating key branches of APP signaling in cells across species (Fogel et al., 2014; Milosch et al., 2014; Nishimoto et al., 1993; Ramaker et al., 2013) and we confirmed that Gαi proteins are severely depleted in ric8a-emx1-cre mutant cortices (Supplemental Fig. 9). Thus, like in ric8a-emx1cre mutants, microglia may play a key role in ecotopia formation in APP pathway mutants. To test this, we first analyzed app mutant microglia. To this end, we employed cx3cr1-cre to delete a conditional allele of app from microglia and found that microglia cultured from app-cx3cr1-cre mutants showed reduced TNFα and IL-6 secretion as well as muted IL-6 transcription upon stimulation (Fig. 3a, Supplemental Fig. 10a-b). This indicates that app plays a previously unrecognized, cell-autonomous role in microglia in regulating microglial activity. Microglia exhibit attenuated immune response following chronic stimulation, especially when carrying strong loss-of-function mutations in anti-inflammatory pathways (Chamberlain et al., 2015; Sayed et al., 2018). We suspect that the attenuated response by app mutant microglia may result from similar effects following in vitro culture. To test effects of app mutation under conditions that more closely resemble in vivo physiological conditions, we next isolated fresh, unelicited peritoneal macrophages and acutely analyzed their response to immune stimulation. We found that app mutant macrophages showed significantly elevated secretion of all cytokines tested (Fig. 3b). At the transcriptional level, mRNA induction was also increased for all cytokines (Fig. 3c). Thus, like that of ric8a, the normal function of app also appears to be to suppress the inflammatory activation of microglia.
To determine if microglial app deficiency is also responsible for ectopia formation in app triple knockout mutants, we next asked if activating microglia in microglia-specific app mutants similarly results in pial ectopia during cortical development. To this end, we administered LPS in utero at E11.5-12.5 to app-cx3cr1-cre mutant animals as we did to ric8a-cx3cr1-cre mutants above. We found that, while none of the 81 littermate controls administered LPS showed ectopia, a significant number of mutant neonates showed ectopia (6 of 31 neonates examined, ∼19%) and associated breaches in the basement membrane (Fig. 3e, Supplemental Fig. 10c-f”). Thus, app deficient microglia, when activated, also results in cortical ectopia during development. The reduced severity of the ectopia observed, as compared to that in ric8a/cx3cr1-cre mutants, likely in part results from the reduced LPS dosage (by ∼3 folds) we had to use in these animas due to the enhanced immune sensitivity of their strain genetic background. Other app gene family members are also expressed in microglia (Zhang et al., 2014) and ectopia are only observed in app/aplp1/2 triple but not in any double or single mutants (Herms et al., 2004). Aplp1/2 may therefore also compensate for the loss of APP in microglia. Thus, these results indicate that app normally plays a cell-autonomous role in microglia that negatively regulate microglial activation, and its loss of function underlies cortical ectopia formation. The similarities between app and ric8a mutant phenotypes suggest that they form a previously unknown anti-inflammatory pathway in microglia.
Monomeric Aβ suppresses microglial inflammatory activation via an APP-Ric8a pathway
The possibility that app and ric8a may form a novel anti-inflammatory pathway in microglia raises questions on the identity of the ligands for the pathway. Several molecules have been reported to bind to APP and/or activate APP-dependent pathways (Fogel et al., 2014; Milosch et al., 2014; Rice et al., 2012), among which Aβ is note-worthy for its nanomolar direct binding affinity (Fogel et al., 2014; Shaked et al., 2006). Aβ oligomers and fibrils have been shown by numerous studies to be pro-inflammatory, while non-fibrillar Aβ lack such activity (Halle et al., 2008; Huang, 2023, 2024; Lorton et al., 1996; Muehlhauser et al., 2001; Tan et al., 1999). In contrast, when employed under conditions that favor the monomer conformation, Aβ inhibits T cell activation (Grant et al., 2012). This suggests that, unlike pro-inflammatory Aβ oligomers (Supplemental Fig. 11j), Aβ monomers may be anti-inflammatory. To test this possibility, we dissolved Aβ40 peptides in DMSO, a standard approach in Alzheimer’s disease research that has been shown to preserve the monomeric conformation (LeVine, 2004; Stine et al., 2011). We found that Aβ monomers as prepared potently suppressed the secretion of large numbers of cytokines (Fig. 4a, Supplemental Fig. 10) and showed similar effects on microglia no matter if they were activated by LPS or poly I:C (Fig. 4b). We also found that the Aβ monomers similarly strongly inhibited the induction of cytokines at the transcriptional level (Fig. 4c, Supplemental Fig. 11). In addition, we observed these effects with Aβ40 peptides from different commercial sources. Thus, these results indicate that monomeric Aβ possesses a previously unreported anti-inflammatory activity against microglia that strongly inhibits microglial inflammatory activation.
To determine whether monomeric Aβ signals through APP, we employed app-cx3cr1-cre mutant microglia. We found that, unlike that of control microglia, Aβ monomers failed to suppress the secretion of all tested cytokines by app mutant microglia (Fig. 4d, Supplemental Fig. 11). Interestingly, this blockade appeared to be specific to app since Aβ monomers still significantly suppressed cytokine secretion by aplp2 mutant microglia. At the transcriptional level, Aβ monomers also failed to suppress cytokine induction in app mutant microglia (Fig. 4e, Supplemental Fig. 11). Together, these results indicate that APP is functionally required in microglia for Aβ monomer inhibition of cytokine expression at both transcriptional and post-transcriptional levels. Cultured microglia from app-cx3cr1-cre mutants showed attenuated immune activation (Fig. 3). To assess whether this may affect the efficacy of Aβ monomer inhibition, we next tested the response of fresh, unelicited macrophages. We found that, like that of control microglia, cytokine secretion by control macrophages was also strongly suppressed by Aβ monomers (Fig. 4f, Supplemental Fig. 11). However, even though app mutant macrophages showed elevated response to immune stimulation in comparison to control macrophages, they still failed to respond to Aβ monomers and displayed levels of cytokine secretion that were indistinguishable from those of DMSO-treated cells (Fig. 4f, Supplemental Fig. 11). Thus, these results further indicate that APP function is required in microglia for mediating the anti-inflammatory effects of Aβ monomers.
The similarity of ric8a ectopia to app ectopia phenotype (Figs. 2 & 3) also suggests that Ric8a functions in the same pathway as APP in mediating Aβ monomer anti-inflammatory signaling in microglia. This is consistent with previous studies showing that heterotrimeric G proteins are coupled to APP and mediate APP intracellular signaling in vitro and vivo (Fogel et al., 2014; Milosch et al., 2014; Nishimoto et al., 1993; Ramaker et al., 2013) and that Ric8a is a molecular chaperone essential for the post-translational stability of heterotrimeric G proteins (Gabay et al., 2011; Tall et al., 2003). To directly test if Ric8a is part of this pathway, we next employed ric8a-cx3cr1-cre mutant microglia. We found that, indeed, like that of app mutant microglia, Aβ monomers also failed to suppress the secretion of TNFα and IL-6 by ric8a mutant microglia (Fig. 4g). This indicates that heterotrimeric G proteins function is likely required in the same pathway of APP in microglia for the suppression of TNFα and IL-6 secretion. However, unlike APP, we found that Ric8a appears to be dispensable for Aβ monomer regulation of other cytokines. For example, unlike that of TNFα and IL-6, Aβ monomers still suppressed IL-1β secretion by ric8a mutant microglia (Supplemental Fig. 11). It also appears to be dispensable for the regulation of cytokine transcription since Aβ monomers similarly suppressed IL-6 transcriptional induction in both control and ric8a mutant microglia. These results suggest that heterotrimeric G proteins function may only mediate some of the anti-inflammatory signaling of monomeric Aβ. Thus, APP and Ric8a-regulated heterotrimeric G proteins form part of a novel anti-inflammatory pathway activated by monomeric Aβ in microglia.
Elevated matrix metalloproteinases (MMPs) cause basement membrane degradation
We have shown that heightened microglial activation due to mutation in the Aβ monomer-activated APP/Ric8a pathway results in basement membrane degradation and ectopia during cortical development. To further test this interpretation, we sought to test the prediction that inhibition of microglial activation in these mutants suppressed the formation ectopia. To this end, we employed dorsomorphin and S3I-201, inhibitors targeting Akt, Stat3, and other mediators in pro-inflammatory signaling (Lee et al., 2016; Qin et al., 2012). Consistent with their anti-inflammatory activity, we found that dorsomorphin and S3I-201 both suppressed astrogliosis associated with neuroinflammation in the cortex of ric8a-emx1-cre mutants (Supplemental Fig. 12). Furthermore, they also suppressed the formation of ectopia in ric8a-emx1-cre mutants, reducing both the number and the size of the ectopia observed (Fig. 5a-f). Most strikingly, the combined administration of dorsomorphin and S3I-201 nearly eliminated all ectopia in ric8a-emx1-cre mutants (Fig. 5d, 5e). Thus, these results indicate that excessive inflammatory activation of microglia is responsible for ectopia formation in ric8a mutants.
Under neuroinflammatory conditions, brain cytokines frequently induce MMPs, which lead to breakdown of the extracellular matrix and contribute to disease pathology (Pagenstecher et al., 1998; Wang et al., 2000). Since ric8a mutant microglia are hyperactive in inflammatory cytokine production, we wonder if induction of MMPs may underlie the laminin degradation and cortical basement membrane break observed in ric8a mutants. To test this, we examined MMP9 expression in the embryonic cortex by in situ hybridization. We found that at E13.5, MMP9 mRNA is strongly expressed in a sparse cell population resembling microglia populating the cortex at this stage (Squarzoni et al., 2014) (Supplemental Fig. 13). Next, we examined the activities of MMP2 and MMP9 in the developing control and mutant cortex using gelatin gel zymography. We found that the activity of MMP9 in the mutant cortex was significantly increased (Fig. 5i, Supplemental Fig. 13). In contrast, that activity of MMP2 remained unaffected. Similarly, at the protein level, we found that the immunoreactivity for MMP9 was increased in ric8a-emx1-cre mutants (Fig. 5g-h). To test if the increased MMP activity is responsible for the ectopia observed, we next employed BB94, a broad-spectrum inhibitor of MMPs. We found that BB94 administration significantly suppress both the number and the size of the ectopia in ric8a mutants (Fig. 5j-m). To narrow down the identity of MMPs responsible, we further employed an inhibitor specific for MMP9 and 13 (MMP-9/MMP-13 inhibitor I, CAS 204140-01-2) and found that it similarly suppressed both the number and the size of the ectopia (Fig. 5l-m). Furthermore, consistent with its near complete suppression of cortical ectopia (Fig. 5a-f), we found that the co-administration of dorsomorphin and S3I-201 also reduced MMP9 activity in the mutant cortex to the control level (Supplemental Fig. 14). Thus, these results indicate this Aβ monomer-regulated anti-inflammatory pathway normally promotes cortical development through suppressing microglial activation and MMP induction.
Discussion
The spatiotemporal expression of immune cytokines by glial cells in the brain plays critical roles in the normal development, function, and plasticity of the brain circuitry (Barres, 2008; Schafer and Stevens, 2015; Zipp et al., 2023). In this article, we have identified a novel microglial anti-inflammatory pathway activated by monomeric Aβ that inhibits microglial cytokine expression and plays essential roles in the normal development of the cerebral cortex. We have found that this pathway is mediated by APP and the heterotrimeric G protein GEF and molecular chaperone Ric8a in microglia and its activation leads to the inhibition of microglial cytokine induction at transcriptional and post-transcriptional levels (Figs. 1-4). We further show that a key function of this pathway is to suppress the activity of MMP9 during corticogenesis and disruption of this regulation results in cortical basement membrane degradation and neuronal ectopia development (Figs. 1-3, 5). Furthermore, we find that this pathway is activated specifically by the monomeric form of Aβ in vitro (Fig. 4), identifying, for the first time, an isoform specific activity of Aβ against microglia. These results provide novel insights into the neuron-glia communication mechanisms that coordinate the regulation of immune cytokines, key regulators of Hebbian and non-Hebbian synaptic plasticity, by glial cells in the brain. The discovery of the novel activity of monomeric Aβ as a negative regulator of microglia may also facilitate the further elucidation of Alzheimer’s disease pathogenesis.
Microglial activity regulation during cortical development
Among the glial cell populations in the brain, astrocytes and oligodendrocyte are both born within the nervous system at the end of cortical neurogenesis. As such, they play limited roles in the early steps of cortical development. In contrast, microglia are not only of a distinct non-neural lineage that originates from outside the nervous system but also begin to populate the brain at the onset of corticogenesis (Ginhoux et al., 2010; Hattori et al., 2023). As such, they play unique roles throughout cortical development. Indeed, microglial activity has been found to regulate the size of the cortical neural precursor pool (Cunningham et al., 2013). Microglia-secreted cytokines have also been found to promote both neurogenesis and oligodendrogenesis (Shigemoto-Mogami et al., 2014). As such, the precise regulation of microglial activity is critical to the normal development of the neocortex from an early stage. In this study, we have shown that immune over-activation of microglia deficient in a monomeric Aβ-regulated pathway results in excessive cortical matrix proteinase activation, leading basement membrane degradation and neuronal ectopia. Previous studies have shown that reductions in the expression of microglial immune and chemotaxis genes instead lead to the failure of microglia to populate the brain (Iyer et al., 2022). These results together highlight the importance of precisely regulating the level of microglial activity during brain development. The dramatic destructive effects of microglial hyperactivity observed during corticogenesis also foreshadow the critical roles it plays in brain dysfunction and disease at later stages of life.
In this study, we have also shown that the anti-inflammatory regulation of microglia in corticogenesis depends on a pathway composed of APP and the heterotrimeric G protein regulator Ric8a. This has revealed new insight into the intercellular signaling mechanisms regulating microglial activity in the brain. Heterotrimeric G proteins are well-known mediators of G protein-coupled receptor (GPCR) signaling. In this study, we have found that they likely also function in the same pathway as APP. To our knowledge, ours is the first study to report an in vivo anti-inflammatory function of this pathway in microglia and has significantly advanced knowledge in microglial biology. This is also consistent with previous studies showing that heterotrimeric G proteins directly interact with the APP cytoplasmic domain and mediate key branches of APP signaling from invertebrates to mammals (Fogel et al., 2014; Milosch et al., 2014; Nishimoto et al., 1993; Ramaker et al., 2013). In this study, we have in addition shown that this pathway is specifically activated in vitro by the monomeric form of Aβ, a peptide produced by neurons in the brain (Cirrito et al., 2005), providing further insight into the biological function of this pathway. In the early cortex, neurogenesis is just beginning, and most neurons born are in an immature state. It is unclear if this pathway is activated by Aβ at this stage in vivo. However, studies have shown that other APP ligands such as pancortin, a member of the olfactomedin family proteins known to inhibit innate immunity (Liu et al., 2010), are expressed in the cortex at this stage (Rice et al., 2012). It will be interesting to determine if these innate immune regulators play a role in regulating this pathway.
In this and previous studies, we have found that deletion of ric8a gene from radial glial progenitors using nestin-cre does not result in obvious cortical ectopia (Fig. 2) (Ma et al., 2017). However, when ric8a is in addition deleted from microglia, this results in severe cortical ectopia (Fig. 2), implicating a novel role of microglia in cortical ectopia development. Previous studies have reported that ric8a deletion by nestin-cre alone results in cortical ectopia (Kask et al., 2015; Kask et al., 2018). The cause for this discrepancy is at present unclear. The expression of nestin-cre, however, is known to be influenced by several factors including transgene insertion site and genetic background and the same nestin-cre has been reported to be active and induce gene inactivation in microglia (Karasinska et al., 2013; Takamori et al., 2009). These factors may play a role in this discrepancy. In our studies, we show that microglia specific ric8a deletion using cx3cr1-cre during development results in severe cortical ectopia upon and only upon immune stimulation (Fig. 2). We further show that microglia specific app deletion results in similar ectopia also only upon immune stimulation (Fig. 3). These results are important findings as they implicate, for the first time, a causative role played by microglial dysfunction in the formation of cortical ectopia in neurodevelopmental disorders.
Neuronal activity, glial cytokine expression, and brain circuit plasticity
Activity-dependent competitive and homeostatic plasticity is a foundational rule that regulates the development, maturation, and function of neural circuits across brain regions. Studies have shown that glial cells, through regulating the spatiotemporal expression of immune cytokines, play a pivotal role in this process. In the developing thalamus, by activating interleukin-33 expression in an activity-dependent manner, astrocytes have been found to promote the segregation of eye-specific axonal projection and the maturation of the visual circuitry (He et al., 2022; Vainchtein et al., 2018). In the visual cortex, astrocytic expression of TNFα similarly mediates activity-dependent homeostatic upscaling of cortical synapses following peripheral monocular deprivation (Barnes et al., 2017; Heir et al., 2024; Kaneko et al., 2008). In this study, we have shown that Aβ monomers inhibit expression of cytokines by brain microglia via a novel APP/heterotrimeric G protein-mediated pathway. Aβ is primarily produced by neurons in the brain in a neural activity-dependent manner and form oligomers when large quantities are produced (Cirrito et al., 2005). Aβ oligomers, in contrary to monomers, are proinflammatory and increase glial cytokine expression (Halle et al., 2008; Huang, 2023; Lorton et al., 1996; Muehlhauser et al., 2001; Tan et al., 1999). These findings thus suggest that different levels of neural circuit activity in the brain may differentially regulate glial cytokine expression through inducing different levels of Aβ. High levels of neural activity may lead to high levels of Aβ and the formation of Aβ oligomers that activate glial cytokine production, while low levels of neural activity may produce low levels of Aβ, maintain Aβ as monomers, and inhibit glial cytokine production. Thus, Aβ in the brain may not only be a reporter of the levels of neural circuit activity but may also serve as an agent that directly mediate activity level-dependent plasticity. Following sensory deprivation, for example, Aβ levels may be lowered due to loss of sensory stimulation. This may lead to the relief of monomeric Aβ inhibition of cytokines such as TNFα and as a result trigger homeostatic upscaling of cortical synapses in the visual cortex (Barnes et al., 2017; Heir et al., 2024; Kaneko et al., 2008). In contrary, when neural activity levels are high, large quantities of Aβ may be produced, leading to formation of Aβ oligomers that may in turn induce expression of cytokines such as IL-33 that promote synaptic pruning. A large body of evidence strongly indicates that Aβ and related pathways indeed mediate homeostatic and competitive plasticity in the visual and other systems of the brain (Galanis et al., 2021; Huang, 2023, 2024; Kamenetz et al., 2003; Kim et al., 2013). Our discovery of the Aβ monomer-activated pathway has therefore provided novel insights into a universal mechanism that senses neural circuit activity pattern and translates it into homeostatic and competitive synaptic changes in the brain, a mechanism with fundamental roles in cognitive function.
In this study, we have also found that the matrix proteinase MMP9 is a key downstream effector of microglial activity in the developing cortex. We find that microglial hyperactivity results in increased levels of MMP9, leading to cortical basement membrane degradation and neuronal ectopia and inhibiting MMP9 directly or indirectly suppresses the phenotype. This suggests that the regulation of MMP9 may be a key mechanism by which glial cells regulate brain development and plasticity. Indeed, independent studies have shown that, in the visual cortex, MMP9 is also a pivotal mediator of TNFα-dependent homeostatic upscaling of central synapses following monocular deprivation (Akol et al., 2022; Kaneko et al., 2008; Kelly et al., 2015; Spolidoro et al., 2012). In the Xenopus tectum, MMP9 has similarly been found to be induced by neural activity and promote visual activity-induced dendritic growth (Gore et al., 2021). Importantly, in both wildtype and amblyopic animals, light reintroduction after dark exposure has been found to reactivate plasticity in the adult visual cortex via MMP9, uncovering a potential treatment for common visual conditions (Murase et al., 2017; Murase et al., 2019). These results therefore highlight a conserved glia/cytokine/MMP9-mediated mechanism that regulates brain development and plasticity from embryogenesis to adulthood. In ocular dominance plasticity, MMP9 is activated at perisynaptic regions (Murase et al., 2017; Murase et al., 2019). MMP9 mRNA translation has been also observed in dendrites (Dziembowska et al., 2012). In the ric8a mutant cortex, we find that MMP9 activity is increased. Further studies are required to precisely determine the cellular sources of MMP9 and how its activity is regulated.
Aβ monomer anti-inflammatory activity and Alzheimer’s disease
Aβ is well known as a component of the amyloid plaques in the Alzheimer’s disease brain. It is a unique amphipathic peptide that can, dependent on concentration and other conditions, remain as monomers or form oligomers. Studies on Aβ have historically focused on the neurotoxic effects of Aβ oligomers and their proinflammatory effects on glia (Gulisano et al., 2018; Halle et al., 2008; He et al., 2019; Huang, 2023; Kim et al., 2013; Lauren et al., 2009; Lazarevic et al., 2017; Lorton et al., 1996; Muehlhauser et al., 2001; Parodi et al., 2010; Puzzo et al., 2008; Shankar et al., 2008; Tan et al., 1999; Walsh et al., 2002; Yang et al., 2015; Zott et al., 2019). In this study, we have found that, in contrary to Aβ oligomers, Aβ monomers instead possess a previously unknown anti-inflammatory activity that acts through a unique microglial pathway. We have further found that genetic disruption of this pathway in corticogenesis results microglial hyperactivity, leading to neuronal ectopia and large disruption of cortical structural organization. To our knowledge, ours is the first study to uncover this overlooked anti-inflammatory activity of Aβ monomers. It is in alignment with recent studies showing that Aβ monomers are also directly protective to neurons and positively regulate synapse development and function (Galanis et al., 2021; Giuffrida et al., 2009; Plant et al., 2003; Ramsden et al., 2002; Zhou et al., 2022). Assuming a set amount of Aβ peptides, the formation of Aβ oligomers and aggregates in the brain would, by chemical law, be predicted to result in the depletion of Aβ monomers (Dear et al., 2020; Michaels et al., 2020). Thus, in the Alzheimer’s disease brain, besides the obvious formation of Aβ aggregates, there may also be a less visible depletion of Aβ monomers taking place at the same time, which may, like Aβ oligomers, also contribute to the development of neuroinflammation and neuronal damage (Huang, 2023). In support of this interpretation, high soluble brain Aβ42, which likely also means high levels of Aβ monomers in the brain, have been found in clinical studies to preserve cognition in patients of both familial and sporadic Alzheimer’s disease, in spite of increasing amyloidosis detected in their brains (Espay et al., 2021; Sturchio et al., 2022; Sturchio et al., 2021). In our study, we have also found that the effects of microglial disinhibition are mediated by MMP9. Importantly, in neurodegenerative diseases, MMP9 has been similarly found to be a key determinant regulatings the selective degeneration of neuronal cell types (Kaplan et al., 2014; Tran et al., 2019). MMP9 levels are also upregulated in the plasma in both mild cognitive impairment and Alzheimer’s disease patients (Bruno et al., 2009; Lorenzl et al., 2008; Tsiknia et al., 2022). In addition, in several motor neuron disease models, reducing MMP9 has been found to protect neurons and delay the loss of motor function (Kaplan et al., 2014; Spiller et al., 2019). Thus, our study has not only uncovered a potentially overlooked role of Aβ monomer depletion in the development of Alzheimer’s disease but also identified downstream effectors. Elucidating the roles these factors play may reveal new insight into the pathogenesis of Alzheimer’s disease.
Methods
Generation of ric8a conditional allele
Standard molecular biology techniques were employed for generating the conditional ric-8a allele. Briefly, genomic fragments, of 4.5 and 2.5 kilobases and flanking exons 2-4 of the ric-8a locus at the 5’ and 3’ side, respectively, were isolated by PCR using high fidelity polymerases. Targeting plasmid was constructed by flanking the genomic fragment containing exons 2-4 with two loxP sites together with a neomycin positive selection cassette, followed by 5’ and 3’ genomic fragments as homologous recombination arms and a pgk-DTA gene as a negative selection cassette. ES cell clones were screened by Southern blot analysis using external probes at 5’ and 3’ sides. For derivation of conditional allele, the neomycin cassette was removed by crossing to an actin-flpe transgenic line after blastocyst injection and germ line transmission. The primer set for genotyping ric-8a conditional allele, which produces a wildtype band of ∼110bp and a mutant band of ∼200bp, is: 5’-cctagttgtgaatcagaagcacttg-3’ and 5’-gccatacctgagttacctaggc-3’. Animals homozygous for the conditional ric-8a allele are viable and fertile, without obvious phenotypes.
Mouse breeding and pharmacology
emx1-cre, nestin-cre, foxg1-cre, cx3cr1-cre, floxed app as well as the BAT-lacZ reporter mouse lines were purchased from the Jackson Lab. nex-cre and wnt3a-cre were as published (Goebbels et al., 2006; Yoshida et al., 2006). cre transgenes were introduced individually into the ric8a or app conditional mutant background for phenotypic analyses and ric8a or app homozygotes without cre as well as heterozygotes with cre (littermates) were both analyzed as controls. For BB94 and MMP9/13 inhibitor injection, pregnant females were treated daily from E12.5 to E14.5 at 30 μg (BB94) or 37.5 μg (MMP9/13 inhibitor) per g of body weight. For dorsomorphin and S3I-201 injection, pregnant females were treated on E12.5 at 7.5 and 25 μg per g of body weight, respectively. For sham treatment, pregnant females were treated on E12.5 with 100 μls of DMSO. BrdU was injected at 100 μg per g of body weight, and embryos were collected 4 hours later for cell proliferation analysis, or alternatively, pups were sacrificed at P5 for neuronal migration analysis and at P17 for other analysis. For LPS treatment, pregnant females were injected intraperitoneally with 400ng (ric8a genetic background) or 150ng (app genetic background) LPS per g of body weight on both E11.5 and E12.5. Animal use was in accordance with institutional guidelines.
Immunohistochemistry
Vibratome sections from brains fixed in 4% paraformaldehyde were used. The following primary antibodies were used at respective dilutions/concentrations: mouse anti-BrdU supernatant (clone G3G4, Developmental Studies Hybridoma Bank (DSHB), University of Iowa, IA; 1:40), mouse anti-RC2 supernatant (DSHB; 1:10), mouse anti-Nestin supernatant (DSHB; 1:20), mouse anti-Vimentin supernatant (DSHB; 1:10), mouse anti-Pax6 supernatant (DSHB; 1:20), moue anti-Reelin (Millipore, 1:500), mouse anti-chondroitin sulfate (CS-56, Sigma, 1:100), rat anti-Ctip2 (Abcam, 1:500), rabbit anti-phospho Histone H3 (Ser10) (Millipore; 1:400), rabbit anti-Cux1 (CDP) (Santa Cruz; 1:100), rabbit anti-laminin (Sigma; 1:2000), rabbit anti-GFAP (Dako;1:1000), rabbit anti-ALDH1L1 (Abcam, 1:500), rabbit anti-MMP9 (Abcam, 1:1000), goat anti-MMP2 (R&D Systems; 5 μg/ml), rabbit anti-Calretinin (Chemicon, 1:2000), mouse anti-S100β (Thermo Scientific; 1:100), rabbit anti-S100β (Thermo Scientific; 1:200), and rabbit anti-phospho-Smad1/5 (Ser463/465) (41D10; Cell Signaling, 1:200). FITC and Cy3 conjugated secondary antibodies were purchased from Jackson ImmunoResearch Laboratories (West Grove, PA). Peroxidase conjugated secondary antibodies were purchased from Santa Cruz Biotech. Staining procedures were performed as described previously (Huang et al., 2006), except for anti-Ric-8a, MMP9, and phospho-Smad1/5 staining, in which a tyramide signal amplification (TSA) plus Cy3 kit (PerkinElmer, Waltham, MA) was used per manufacturer’s instruction. Sections were mounted with Fluoromount G medium (Southern Biotech, Birmingham, AB) and analyzed under a Nikon eclipse Ti microscope or an Olympus confocal microscope.
Microglia culture and assay
Cerebral hemispheres were dissected from individual neonates, mechanically dissociated, split into 3-4 wells each and cultured in DMEM-F12 (Lonza) containing 10% fetal bovine serum (FBS) (Invitrogen). Microglial cells were harvested by light trypsinization that removes astroglial sheet on day 13-15. For experiments other than assaying IL-1β secretion, microglia were treated with LPS at 20ng/ml for 3 hours or at 5ng/ml overnight and, if applicable, DMSO or Aβ40 (ApexBio and Genscript) was applied at the same time as LPS. For assaying IL-1β secretion, microglia were primed with LPS at 200ng/ml for 5-6 hours before treatment with 3mM ATP for 15 minutes. In these experiments, DMSO or Aβ40 was applied at the same time as ATP if applicable. Supernatants were collected and used for cytokine ELISA assays per manufacturer’s instructions (Biolegend). Total RNAs were prepared from collected cells using Trizol (Invitrogen) and cDNAs were synthesized using a High-capacity cDNA reverse transcription kit (Applied Biosystems). Quantitative PCR was performed using a GoTaq qPCR master mix per manufacturer’s instructions (Promega). All gene expression levels were normalized against that of GAPDH.
Quantitative and statistical analysis
The sample size was estimated to be 3-9 animals each genotype (every 4th of 50 μm coronal sections, 7-10 sections each animal) for ectopia analysis, 3-5 animals each genotype (3-4 sections each animal) for immunohistochemical analysis, and 4-6 animals each genotype for gel zymography and Western blot analysis, as has been demonstrated by previous publications to be adequate for similar animal studies. Matching sections were used between controls and mutants. NIS-Elements BR 3.0 software (Nikon) was used for quantifying the numbers and sizes of neuronal ectopia, the numbers of laminin positive debris, as well as the numbers of astrocytes. ImageJ software (NIH) was used for quantifying the intensity of immunostainings. In analysis of radial glial cell division, the cleavage plane angle was calculated by determining the angle between the equatorial plate and the ventricular surface. Statistics was performed using Student’s t test when comparing two conditions, or one-way ANOVA followed by Tukey’s post hoc test when comparing three or more conditions. All data are represented as means ± s.e.m.
Acknowledgements
1. Z. H. thanks Dr. L. F. Reichardt for supporting the initial generation of ric8a mutant ES cells, Dr. E. A. Grove (Chicago) for providing the wnt3a-cre strain, the late Dr. B. A. Barres (Stanford) for critiques and input, and Drs. W. L. Murphy and E. Bresnick (UW-Madison) for access to a plate reader and a qPCR machine. We also thank the late Dr. D. Oertel (UW-Madison) for critical reading and editing and Dr. L Puglielli (UW-Madison) for critical reading of a previous version of the manuscript. This work was supported by funds from the Departments of Neurology and Neuroscience, UW-Madison, and a Basil O’Connor award from the March of Dimes foundation to Z.H.
Supplemental figures
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