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Villa, C. IPSCs and organoids in ASD. Encyclopedia. Available online: https://encyclopedia.pub/entry/10826 (accessed on 29 March 2024).
Villa C. IPSCs and organoids in ASD. Encyclopedia. Available at: https://encyclopedia.pub/entry/10826. Accessed March 29, 2024.
Villa, Chiara. "IPSCs and organoids in ASD" Encyclopedia, https://encyclopedia.pub/entry/10826 (accessed March 29, 2024).
Villa, C. (2021, June 14). IPSCs and organoids in ASD. In Encyclopedia. https://encyclopedia.pub/entry/10826
Villa, Chiara. "IPSCs and organoids in ASD." Encyclopedia. Web. 14 June, 2021.
IPSCs and organoids in ASD
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Autism spectrum disorder (ASD) encompasses a broad range of complex polygenic and multifactorial neurodevelopmental diseases affecting social interaction, communication, interests, and behavior. The major limit to ASD research remains a lack of relevant models which can faithfully re-capitulate key features of the pathology. Recent advances in induced pluripotent stem cells (iPSCs), reprogrammed from somatic cells of patients, have provided a promising cellular tool for disease modelling and development of novel drug treatments. Moreover, iPSCs can be differentiated and organized into 3D organoids, providing a model which mimics the complexity of the brain’s architecture. 

autism spectrum disorders induced pluripotent stem cells brain organoids

1. Introduction

Over the past decade, the development of induced pluripotent stem cell (iPSC) technology has provided a novel means to generate disease-relevant cells for in vitro investigation of the molecular and cellular mechanisms underpinning human complex disorders [1][2]. Diseases affecting the central nervous system (CNS) have been the most frequent targets, given the limited access to vital human brain cells and to the lack of or adequacy of existing animal models [3]. iPSCs are undifferentiated cells with self-renewal capability and can be directly generated from somatic cells (isolated from the skin, blood, or urine of an individual) by expressing the reprogramming factors Oct4, Sox2, Klf4, and c-Myc [4]. In principle, the resulting patient-specific iPSCs can subsequently differentiate into disease-relevant cell types, including multiple subclasses of neurons, astrocytes, and microglia, thus providing an unlimited source of cells that harbor the patient’s precise genome associated with the pathogenesis in the appropriate microenvironment. Therefore, the use of iPSCs offers opportunity to study CNS disorders overcoming the ethical limits of human embryonic stem cells (hESCs) or limited durability of primary cultures [5]. Recapitulating disease features, these cells can serve as large-scale drug screening platforms for novel therapeutic targets and have the great potential to be used in cell therapy and personalized medicine as compared to different sources of stem cell, such as hESCs or mesenchymal stem cells (MSCs). Main advantages and disadvantages of these stem cell types are briefly summarized in Table 1.

Table 1. Main advantages and disadvantages of different types of stem cells: ESCs, MSCs, and iPSCs.

Cell Types Advantages Disadvantages
ESCs Low cost
Established protocols for maintenance in culture
Any cell type differentiation (pluripotency)
Efficient differentiation
Mutation rate
Embryo destruction
Ethical/political concerns
Difficulty to obtain
Lack of genetic/immunohistocompatibility match
MSCs Availability
Ease to isolate and expand
No ethical concerns
Trans-differentiation capacities
Success in various clinical applications
Limited number of cell type differentiation (multipotency)
Loss of proliferative and differentiation capacities over
continuous passages
Standardization difficulty
Genetic heterogeneity
iPSCs No ethical concerns
Ease to obtain
Use of abundant somatic cells of donor
Any cell type differentiation (pluripotency)
Genetic/immunohistocompatibility match
Utility for drug development and developmental
studies
Cost of production
Difficulty of standardization, reproducibility and
maintenance
Tumorigenesis
Genomic instability
ESCs, embryonic stem cells; MSCs, mesenchymal stem cells; iPSCs: induced pluripotent stem cells.

Although iPSCs-based two-dimensional (2D) brain cultures have increased the understanding of different diseases, human pathologies originate in the context of complex interactions at the cellular, tissue and organ levels. To overcome the inherent constraints associated to iPSCs-derived 2D cultures, three-dimensional (3D) models have been recently implemented, leading to the generation of cerebral organoids, a complex self-organizing 3D aggregate of different cell types derived from iPSCs [6]. Brain organoids possess cerebral-like structures, thus mimicking more closely the in vivo human pathophysiology [7].

Autism spectrum disorder (ASD) encompasses a broad range of complex polygenic and multifactorial neurodevelopmental diseases diagnosed in early childhood, affecting social interaction, communication, interests, and behavior [8]. The worldwide prevalence of ASD is just under 1% in children with higher estimates in high-income countries and has markedly increased in the last decade probably due to rising awareness of the condition and improved criteria for diagnosis [9]. The core symptoms of ASD vary in degree of severity and are often accompanied by other concomitant diseases and conditions, including epilepsy, anxiety, obsessive compulsive disorder, intellectual disability, schizophrenia (SZ), and attention-deficit hyperactivity disorder (ADHD) [10][11]. Because of the heterogeneity of symptoms and severity of ASD, the disorder may be diagnosed in children at different ages [12]. Most children who are diagnosed with ASD at less than 3 years have retained their diagnosis, while approximately 9% of children who are diagnosed with ASD in early childhood may not meet criteria for ASD by young adulthood [12]. While its exact etiology remains unclear, ASD is known to have a strong genetic background, with family and twins studies suggesting a sizable heritability ranging from 50 to 90% [13][14][15]. The clinical heterogeneity of ASD is due to several factors: the complexity of its genetic profile (the involvement of multiple genes and the existence of different inheritance patterns); the existence of gene-environment interactions; the diverse nature genetic variants involved (ranging from common, rare, de novo and inherited in both coding and non-coding regions of the genome) [16][17]. ASD has been typically classified into non-syndromic (idiopathic, unknown genetic etiology) and syndromic (caused by a known genetic defect), based on a lack of or association to clinical manifestations outside of the autistic features, respectively [18][19]. In the “omics” era, the terms “syndromic” versus “non-syndromic” ASD fare slightly better under careful scrutiny and could be used with appropriate caveats. The use of this classification based on clinical observation demonstrated that it could led to erroneous conclusions that might be corrected retrospectively by means of “omic” studies. For example, rare syndromic mutations were reported in individuals with ASD who were thought not to have syndromic features based on a clinical exam, and, conversely, syndromic features became apparent only by a re-categorization of non-syndromic cohorts after genetic evaluation. Recently, it has become clear that a considerable overlap exists between molecular pathways and biological mechanisms detected in syndromic versus non-syndromic ASD. The term syndromic would be better substituted with “associated with known medical or genetic condition”. Nonetheless, in the description of studies on iPSCs and organoids, we will use the classical classification in syndromic and non-syndromic considering that the cited literature is based on these two groups.

Several autism-susceptibility or genetic risk factors identified in syndromic forms of ASDs involved genes with a role in different processes: the regulation of synaptic plasticity, cell adhesion, neural connectivity, dendritic trafficking, transcription, gene imprinting, chromatin remodeling, and neurotransmission [20][21][22][23][24]. Moreover, modifying risk factors contribute in delineating the observed phenotype. These factors include several pre- and postnatal environmental factors, including maternal smoking, parental age of birth, infection, alcohol consumption, pollution, pesticide exposure, and gestational complications, such as bleeding or diabetes [25][26][27][28][29].

As the multigenic origin of idiopathic ASD makes it difficult to model, iPSCs-based technologies from individuals with genetically complex etiologies have enabled the investigation of pathological mechanisms in disease-relevant human brain cell types and therefore offer a promising platform to test drugs in a safe environment with human genetic background and relevance [30]. Herein, we report advances in modeling ASD with iPSCs-derived technologies and their use in the drug discovery and the development of potential new treatments, as well as their relevance in clinical applications and precision medicine approaches (Figure 1).

Figure 1. Schematic representation of disease modeling and drug discovery with iPSCs in Autism spectrum disorder (ASD). Specific iPSCs can be derived from somatic cells of ASD individuals and can be further differentiated into different cells types of the central nervous system (CNS) or organized in brain organoids for drug discovery in vitro, development of new drugs, and clinical trials, leading to a personalized medicine for ASD. This figure was created with BioRender.com (accessed on 11 February 2021).

2. iPSC Models of ASDs

The iPSC technology has led to insight into relevant cell types involved in disease mechanisms of ASD, offering a ground-breaking platform to study abnormalities in neurodevelopmental processes that can functionally alter neural circuitry [31]. The majority of iPSCs disease modeling studies use the conventional 2D monolayer culture models to recreate disease-relevant cell types. Two different main strategies are used for producing neural cell starting form iPSCs: the direct differentiation or the reprogramming. In the first case, iPSCs are firstly induced to neural progenitor cells (NPCs) and then differentiated by exposition to trophic factors (e.g., cAMP, BDNF, NT3, and GDNF) [32]. In the reprogramming strategy, iPSCs are transduced with lentiviruses carrying specific transcription factors and an antibiotic selection cassette for efficient conversion and selection [33]. Different iPSCs-derived phenotypes in NPCs, neurons and glial cells (mainly astrocytes and oligodendrocytes) have been already described for both non-syndromic and syndromic forms of ASD.

2.1. iPSCs-Derived Neural Progenitor Cells

NPCs are a population of cells with self-renewal and multipotent differentiation ability that can differentiate into both mature neurons and glial cells. NPCs play an important role in neurogenesis [34], and their dysfunction has been related with both non-syndromic [35][36][37][38] and syndromic ASD, including RETT syndrome (RTT) [39][40][41][42], Fragile X syndrome (FXS) [43][44], tuberous sclerosis complex (TSC) [45][46], Phelan-McDermid syndrome (PMDS) [47], and Timothy syndrome (TS) [48][49].

In regard to idiopathic ASD, NPCs from individuals with macrocephaly displayed an increased cellular proliferation resulted from alterations in a canonical Wnt-β-catenin/BRN transcriptional cascade [35]. These abnormalities in proliferation lead to aberrant neurogenesis and reduced synaptogenesis, thus contributing to functional defects in neuronal networks [35]. Consistently, a recent study demonstrated that the hyperproliferation observed in NPCs derived from iPSCs of ASD subjects with macrocephaly affects genome instability by inducing replication stress-associated genes [36]. Other authors reported that iPSCs-derived NPCs show an impaired crosstalk between the pathways of mTORC1 and Reelin-DAB1, which is known to play a crucial role in regulating neuronal migration and synapse function [37]. This altered interplay was already shown to affect neuronal migration and positioning in a TSC mouse model and in cortical tubers from TSC patients [50]. Moreover, abnormalities in neuronal development, morphology and function were observed in NPCs from a non-syndromic ASD child with a de novo balanced translocation disrupting TRPC6, encoding for the human transient receptor potential 6 channel, involved in excitatory synapse and dendritic spine formation [38].

NPCs were also obtained from patients affected by RTT (OMIM #312750), an early-onset neurodevelopmental disorder caused by mutations in the X-linked gene methyl-CpG-binding protein 2 (MECP2; Xp28), a ubiquitously expressed transcriptional regulator essential for the maturation and normal function of neurons [51][52]. This syndrome is the second most common cause of severe intellectual disability in females and, a considerable fraction of affected individuals meets diagnostic criteria for ASD [53]. Atypical RTT variants have been identified, associated with mutations in cyclin-dependent kinase-like 5 (CDKL5; Xp22.13) and forkhead box protein G1 (FOXG1; 14q12) [51]. NPCs derived from iPSCs of patients carrying different MECP2 mutations underwent X-inactivation when differentiating into functional neurons [39]. Another study found an increase in neural long-interspersed nuclear element-1 (LINE-1) retrotransposon, suggesting that MECP2 is involved in its mobility within the CNS [40]. In three children with MECP2 duplication, an altered expression of neuronal progenitor genes in NPCs was found [41]. Interestingly, a recent report demonstrated that NPCs and also cortical neurons show a global repressed translation and a decreased ribosome engagement of NEDD4-family ubiquitin ligases, leading to accumulation of target proteins that escape proteasome degradation. These evidences provide insight into novel therapeutic strategies based on the regulation of ubiquination process [42].

FXS (OMIM #300624) is responsible for the most common monogenic cause of ASD that is typically due to a triplet repeat expansion (>200 CGG repeats in the 5′ untranslated region) and subsequent methylation of the FMR1 gene on the X chromosome (Xq27.3) [54]. As a result, the amount of FMRP (protein product of FMR1) decreases, leading to an abnormal translation of different proteins. In fact, FMRP is an mRNA binding protein that regulates the mRNA transport and translational regulation in dendrites [54]. In the case of FXS, Telias et al. performed directed differentiation of cells from three patients and observed in FXS neural progenitors an abnormal expression of key NPC genes (SOX1, NOTCH1, PAX6) [43]. The iPSCs-derived FXS NPCs were then used to investigate functional maturation of the excitatory transmission system in response to the glutamate analog (AMPA) [44]. The authors demonstrated an impairment in calcium (Ca2+) signaling via AMPA receptors (AMPARs), suggesting that their functional alterations affect neuronal differentiation and contribute to aberrant neuronal circuit formation and function in FXS [44].

Another ASD-associated syndrome where iPSCs were obtained and studied is TSC (OMIM #191100 and #613254), an autosomal dominant genetic disorder, characterized by benign tumors in the brain and other organs, epilepsy, cognitive impairment, and high penetrance of ASD [55]. The prevalence of ASD in TSC varies among studies, but it is estimated to range from 36% to 50% [55]. TSC is caused by mutations in two genes: TSC1 (hamartin gene, 9q34) and TSC2 (tuberin gene, 16p13.3) that act as tumor suppressors inhibiting the mammalian target of rapamycin (mTOR) [56]. These events lead to constitutive activation of mTOR complex 1 cascade and the uncontrolled proliferation of cells. In neurons, dysfunction of this pathway results in abnormal development of fundamental processes that have been proposed to contribute to the behavioral deficits seen in ASD [55]. Human iPSCs-derived from TSC patients exhibited a delay in their ability to differentiate into neurons that is probably related to a dysregulated PI3K/AKT signaling [45]. Recently, isogenic NPCs derived from a patient carrying a nonsense TSC1 mutation revealed altered early neurodevelopmental phenotypes displaying enhanced proliferation, aberrant neurite outgrowth and enlarged cell size, consistent with mTORC1 activation [46]. However, rapamycin treatment was effective only in reverting enlarged cell size, whereas it was ineffective in increasing proliferation and neurite outgrowth in iPSCs-derived NPCs. Thus, it could be speculated that early neurodevelopmental phenotypes due to TSC1 loss are not solely related to mTORC1 activation. Moreover, transcriptome analysis showed differentially expressed genes (DEGs) related to ASD phenotype with a genotype-dependent linear response: upregulated/downregulated genes were further increased/decreased in homozygous NPCs, generated by CRISPR/Cas9 (clustered regularly interspaced short palindromic repeats/CRISPR-associated protein 9 nuclease) genome editing technology, compared to the heterozygous state [46].

Similarly, genome-wide RNA sequencing was applied to explore DEGs in iPSCs-NPCs and forebrain neurons derived from PMDS probands and unaffected siblings [47]. PMDS (OMIM #606232), also called 22q13 deletion syndrome, is a rare disease with different clinical features, such as severe intellectual impairments and ASD. A critical region involved three genes, but SHANK3 is the strongest candidate for the neurobehavioral symptoms [57]. In fact, SHANK3 encodes a scaffolding protein enriched in the postsynaptic density of glutamatergic synapses and plays a critical role in synaptic function and dendrite formation [58]. In PMDS-iPSCs, the authors found an underexpression of genes involved in Wnt signaling, embryonic development, and protein translation, whereas an overexpression was observed in genes related to pre- and post-synaptic signaling, synaptic plasticity regulation and G-protein-gated potassium channels. Interestingly, these data partially overlapped with iPSC transcriptome findings in other ASDs, converging on altered Wnt signaling and extracellular matrix [47].

In 2011, patient-specific iPSCs-derived NPCs and cortical neurons offered new insights into the pathogenesis of TC (OMIM #601005), a rare and lethal multi-organ disorder connected with gain-of-function missense mutation in the CACNA1C gene (12p13.33) [59], linking its phenotype to defects in Ca2+ signaling and gene expression-dependent activity [48]. In the same study, the authors reported an abnormal expression of tyrosine hydroxylase (TH) and an increased production of norepinephrine and dopamine in neurons, consistent with the key role of catecholamines in sensory gating and social behavior [48]. A genome-wide weighted co-expression network analysis (WGCNA) on NPCs from TS-iPSCs further confirmed dysregulation of Ca2+ signaling in neural development and function [49].

2.2. iPSCs-Derived Neurons

Neurons, generated from NSCs during brain development, are electrically excitable cells that transmit information via specialized connections called synapses [60]. Post-mortem human brain analysis, as well as functional and structural imaging studies in ASD, showed an impairment in the formation of neuronal networks and synaptogenesis [61][62]. In addition, cerebral tissues displayed altered neuronal phenotype, consisting of reduced soma size, abnormal neuronal morphology, reduced dendritic arborization, fewer dendritic spines and synapses [63][64]. Similar morphological alterations were also found in iPSCs-derived neurons from non-syndromic ASD patient carrying a TRPC6 mutation [38]. The same authors demonstrated that the treatment with insulin-like growth factor 1 (IGF-1) or hyperforin, a TRPC6-specific agonist, is able to rescue the neuronal abnormalities, suggesting a possible target for therapeutic strategies in individuals with alterations in this pathway. Interestingly, it has been also shown that MECP2 levels affect TRPC6 expression, hypothesizing common pathways among ASD [38]. Additional iPSCs-based studies in idiopathic ASD reported an imbalance between excitatory and inhibitory synapses, leading to deficits in social interaction and behaviors as widely described in autistic individuals [65][66][67][68]. An overproduction of GABAergic inhibitory neurons has been observed in iPSCs-derived neurons from patients carrying FOXG1 mutations [69]. In ASD individuals with macrocephaly, other authors reported a reduced synaptogenesis, abnormal neurogenesis and a significant decrease in both inhibitory and excitatory neurotransmitters, leading to functional defects in neuronal networks which were rescued by IGF-1 treatment [45]. A reduced activity of neurons was further observed in a cohort of non-syndromic ASD patients, showing a significant decrease in excitatory neurotransmitter release, synaptic events and, consequently, spontaneous spike rate [31]. In iPSCs-derived neurons from non-syndromic individuals carrying SHANK2 mutations, other authors recently showed a hyperconnectivity as demonstrated by an increase in dendrite length and complexity, synapse number and frequency of spontaneous excitatory post-synaptic currents [70].

Human iPSCs-derived neurons have been largely used to study a wide range of syndromic ASD forms. Concerning RTT, several groups generated iPSC lines from patients and successfully differentiated them into NPCs and functional neurons. Similarly to results reported for NPCs, iPSCs-derived neurons exhibited increased susceptibility for LINE-1 retrotransposition, probably caused by MECP2 mutations [40]. Marchetto and collaborators [39] showed smaller soma size, reduced dendritic spine densities and fewer synapses in RTT iPSCs-derived neurons in comparison with the isogenic wild-type ones. Moreover, they observed alterations in Ca2+ influx, thus causing electrophysiological defects in the RTT neurons [39]. Conversely, other authors reported that cortical neurons, derived from iPSC lines with MECP2 duplicated gene, display increased synaptogenesis and dendritic complexity with altered neuronal network synchronization recorded by multi-electrode array (MEA) electrophysiology technique [41]. The functional phenotype was further rescued by the treatment with one histone deacetylase inhibitor, named NCH-51 [51]. RNA-seq profiling on differentiated iPSCs-neurons from RTT patients harboring different MECP2 mutations revealed a prominent enrichment in GABA pathway genes, including GABA receptors and other GABA circuits [71]. Intriguingly, MECP2-mutated neurons showed an impairment of the microtubule network along with a significant decrease of acetylated α-tubulin which was reverted by treatment with selective inhibitors of histone deacetylase 6 (HDAC6), the main cytoplasmic deacetylase in which the main substrate is acetylated α-tubulin [71]. In regard to CDKL5 deficiency disorder (CDD), an atypical form of RTT, a study successfully generated clones of CDKL5-mutated iPSCs to model disease pathogenesis in vitro [72]. CDD is an X-linked neurological disease caused by pathogenic mutations in the gene for cyclin-dependent kinase-like 5 (CDKL5), a serine-threonine kinase highly expressed in the brain [73]. This rare disease was considered as an atypical variant of RTT; however, it has since been recognized as a distinct disorder with common clinical features, such as early-life seizures, autistic behaviors, and intellectual disability [74]. Interestingly, CDKL5-mutated iPSCs from females maintained X-chromosome inactivation, allowing the use of clones expressing the wild-type allele as ideal experimental controls, genetically identical to those derived from the same patient [72]. In iPSC-derived neurons from patients carrying CDKL5 mutations, a following study detected a loss of synaptic contacts, as well as an increased number of aberrant dendritic spines, demonstrating an interesting role for CDKL5 in spine development and synapse morphogenesis [75].

The majority of studies performed in iPSCs-derived neurons from FXS patients revealed an impairment of neuronal differentiation and maturation as a result of epigenetic differences on FMR1 gene expression [76][77][78][79][80]. Moreover, neurons exhibited a number of additional phenotypic abnormalities, including an altered electrophysiological network activity, neurite outgrowth and branching defects [80][81]. Perturbations in synaptic transmission, cell proliferation and ion transmembrane transporter activity pathways were also reported [80]. Importantly, other authors demonstrated dysregulated Ca2+ signals in iPSCs-derived neurons, strengthening the key role of intracellular Ca2+ in neurite growth and synaptic connections [82].

In TSC, iPSCs-derived neurons presented with an enlarged soma, decreased neurite length, complex neurite branching and abnormal connections among cells, as compared to those from unaffected individuals [83]. These abnormalities may be related to hyperactivity of mTOR. Similarly, Zucco et al. generated iPSC-derived NPCs and neurons from two TSC patients reporting a dysregulation of PI3K/AKT/mTORC1 pathway [45]. In mono-cultures of iPSCs-derived cortical neurons, MEA analysis showed an increase in basal dendritic branching and spontaneous Ca2+ event frequency [84], consistent with the network hyperactivity previously observed in the TSC mouse model [85]. It should be noted that these aforementioned studies were performed in iPSCs-derived neurons from TSC patients with heterozygous mutations. In a recent study examining iPSCs-derived neurons carrying either single or biallelic mutations in TSC2, the authors reported that the loss of one or both alleles of TSC2 results in mTORC1 hyperactivation and specific neuronal abnormalities which were partially rescued by pharmacological treatment with mTOR regulator rapamycin [86]. However, only neurons harboring biallelic mutations displayed hyperactivity and upregulation of cell adhesion genes observed in cortical tubers. Collectively, these data suggest that the loss of one allele of TSC2 is sufficient to induce morphological and physiological changes in human neurons, but only with TSC2 biallelic mutations, a gene expression dysregulation could be detected [86].

In PMDS, neurons derived from iPSCs displayed an impairment in excitatory synaptic transmission, depending on both a failure to generate the correct number of excitatory synapses and a decrease in the expression of glutamate receptors [87]. Interestingly, these defects were rescued by restoring SHANK3 expression or treating neurons with IGF-1, thus suggesting a key role of SHANK3 in synapse formation [87]. Moreover, PMDS iPSCs-derived neurons from fibroblasts of 2 children with ASD harboring independent de novo SHANK3 mutations also provided a novel platform for screening active compounds able to reverse SHANK3 haploinsufficiency by increasing SHANK3 protein levels and its recruitment to the glutamatergic synapses [88]. The presence of synaptic abnormalities in ASD patients carrying SHANK3 mutations was further confirmed by a recent study in which iPSCs-derived pyramidal neurons exhibited a significant decrease in dendritic spine densities, as well as in whole spine and spine head volumes [89]. Yi and colleagues studied engineered iPSCs harboring heterozygous and homozygous SHANK3 deletions reporting significant decreases neurite outgrowth, hyperexcitability, increased input resistance and disrupt excitatory synaptic transmission and demonstrated that these excitability deficits were at least in part due to altered surface expression of hyperpolarization-activated cyclic nucleotide–gated (HCN) channels [90].

As already observed in iPSCs-derived NPCs, also neurons from TS patients showed defects in Ca2+ signaling, neuronal differentiation and aberrant expression of TH that was be reversed by treatment with roscovitine, a cyclin dependent kinase inhibitor [48]. Some authors suggested that a neuronal impairment of Ca2+ signaling may be caused by the increased intracellular Ca2+ influx in rodents and human iPSCs-derived neurons after membrane depolarization. Moreover, they showed that these cells exhibit the activity-dependent dendritic retraction [91]. A recent report suggested how aberrant CaV1.2 splicing affects differentiation of the developing cortex during TS pathogenesis [92].

In the first study using iPSCs-based technology for modeling Angelman syndrome (AS, OMIM #105830) and Prader-Willy Syndrome (PWS, OMIM #176270), no phenotypic differences were observed in neurons [93]. One of the major genes implicated in ASD is UBE3A (ubiquitin protein ligase E3A), gene involved in the AS. This disorder is typically caused by a maternal deletion within chromosome 15q11-q13, containing the gene (70 to 75% of cases). Other cases can be ascribed to paternal uniparental disomy (2% to 3%), imprinting center defect (3% to 5%), or single point mutation in the maternal UBE3A allele (5 to 10%) [94]. Proper gene dosage of UBE3A is crucial to normal brain development, as evidenced by the neurodevelopmental disorders associated with this syndrome [95]. Importantly, the authors found that UBE3A imprinting is established during neuronal differentiation of AS iPSCs through an up-regulated expression of paternal UBE3A antisense transcript (UBE3A-ATS) concomitant with a repression of paternal UBE3A [93]. A subsequent study revealed that the silencing of paternal UBE3A expression by SNHG14 (also named as UBE3A-ATS) induction is a late event during neuronal differentiation [96]. Moreover, it has been shown that iPSCs-derived neurons from AS individuals harboring a large deletion of 15q11–q13 display impaired maturation of resting membrane potential and action potential firing, a reduction in excitatory synaptic activity and a deficit in activity-dependent synaptic plasticity [97].

2.3. iPSCs-Derived Astrocytes

Astrocytes, a sub-type of glia, are the most abundant cells in the mammalian CNS and are involved in homeostasis and defense mechanisms. They also play an active role in neurogenesis, synaptogenesis, neuronal support, neurotransmitter recycling, and neuronal network formation [98]. Although the majority of current applications of iPSCs-based technologies in ASD patients have been focused on neurons, glial cells have been shown to play important role in the disorder. Indeed, post-mortem human brain from children with ASD exhibited abnormal glial cell numbers and function [99], as well as an altered density of excitatory synapses, probably caused by impaired synaptic pruning, the natural process by which extra neurons and synaptic connections are removed in order to increase the neuronal network efficiency [100].

In the case of non-syndromic ASD, only one study has been reported so far focused on the interplay between neurons and astrocytes [31]. Co-culture experiments revealed that astrocytes derived from ASD-iPSCs interfere with proper neuronal development. On the contrary, an improvement in the morphology and synaptogenesis of ASD neurons has been demonstrated by combining them with from control iPSCs-derived astrocytes. The same authors reported a high secretion of the pro-inflammatory cytokine interleukin-6 (IL-6) from astrocytes in ASD individuals probably linked to neural defects and showed an increased synaptogenesis by inhibiting IL-6 [31]. Interestingly, reactive astrocytes have been identified to be the main source of cytokines in post-mortem brain tissue of ASD patients [101] and IL-6 was already reported to be increased in plasma [102][103], cerebrospinal fluid [101] and peripheral blood cells of autistic individuals [104].

Astrocytes derived from iPSCs have been also used to study syndromic ASD, such as RTT. Williams and collaborators specifically focused on the glial effects in RTT neurons by differentiating iPSCs in astroglial progenitors and astrocytes [105]. In co-cultures systems, RTT astrocytes affected the phenotype of hippocampal neurons, causing reduced size of soma and number of terminal ends, as well as shorter neurite length, suggesting that the secretion factors from the astrocytes lead to the aberrant neuronal phenotypes. These morphologic abnormalities were partially rescued when neurons were treated with IGF-1 and GPE (a peptide containing the first 3 amino acids of IGF-1), indicating IGF-1 as a potential cellular target for RTT treatment and highlighting potential avenues for drug development [105]. The critical glial contribution to RTT pathology was further confirmed by another study showing a perturbed astrocyte differentiation in iPSC lines that in turn contributed to the functional immaturity of neurons [106].

2.4. iPSCs-Derived Oligodendrocytes

Oligodendrocytes are the myelinating glia of the CNS and originate from oligodendrocyte progenitor cells (OPCs), that hold the capacity to proliferate and migrate. They produce myelin sheath, a greatly extended and modified plasma membrane wrapped around the axons, enabling fast saltatory nerve conduction, axon integrity, and thus contributing to the optimal information processing in complex neural networks [107]. As the demyelination is a hallmark of several diseases, oligodendrocytes have become a great cell source for modeling demyelinating disorders [108]. However, increasing studies suggested a possible role of oligodendrocytes also in the ASD pathogenesis [109]. In the left frontal cortex of autistic patients, a decreased concentration of N-acetyl aspartate (NAA), an amino acid involved in the myelination support, was found [110][111]. Moreover, it has been shown that OPCs isolated from the cortex of TS mice exhibit a more complex morphology and higher protein levels of myelin [112].

Regarding iPSCs-derived oligodendrocytes, only one study has been performed in autistic patients. In the attempt to investigate neuro-glia interactions in TSC phenotypes, the authors found a neuronal hypertrophy and increased axonal density in co-cultures with oligodendrocytes. Moreover, decreased maturation but not cellular proliferation was shown in TSC-oligodendrocytes. Interestingly, pharmacological treatment with rapamycin, mTOR regulator, repressed these defects [84]. Hence, developing models for TSC disease and drug discovery based on the complex interaction between neuronal and glial cells may present a promising tool.

2.5. Current Challenges for the Applicability of iPSCs in ASD Modeling

Despite the potential benefits of iPSCs in ASD modeling, there are many challenges that need to be addressed for their applications in clinical setting and pharmacology. The selection of donor cell type (dermal fibroblasts, blood cells or renal tubular cells collected from urine) for the reprogramming process represent the first critical step for the iPSCs generation [4]. It has been shown that skin biopsy-derived dermal fibroblasts and blood cells might carry genetic mutations and chromosomal abnormalities due to exposure to high cell turnover rates and ultra-violet radiation [113]. Depending on the donor cell types, iPSCs can retain some degree of residual epigenetic memory due to an incomplete resetting of the non-CpG methylation patterns during reprogramming processes, thus affecting the differentiation potential [114]. The second step in the generation of iPSCs is the choice of the suitable method for cellular delivery of the reprogramming factors and strategy. The use of retroviruses and lentiviruses can produce an insertional activation of oncogenes and/or inactivation of tumor suppressor genes, leading to a constitutive expression of the reprogramming factors and altering the characteristics and the differentiation potential of iPSCs.

One of the major limitations to the use of iPSCs is the restricted amount of patient-derived cell lines that limits the possibility of quantitative analyses [115]. Another issue arising from iPSCs-based modeling in ASD is represented by the selection of a proper control. Indeed, in the majority of studies, unaffected subjects or family members are used as controls, but this can be questionable since each individual has a unique genetic background that could potentially affect the identification of disease-relevant phenotypes.

Like all cultured cells, iPSCs show natural genetic heterogeneity even in cell lines derived from the same individual. Therefore, such diversity can create difficulties at any step of reprogramming somatic cells to iPSCs and may also impair their differentiation ability into desired cell populations [116].

3. Brain Organoid Models of ASDs

Three-dimensional self-organized neural cultures rely on the ability of iPSCs or, more in general, stem cell to self-organize in 3D structures, frequently named mini-brain, providing also required self-patterning factors for morphogenesis and differentiation [117]. These organoids are able to sum up sequential neurogenesis, migration, gliogenesis, and synaptogenesis of cortical development that cannot be studied in 2D cell cultures [118]. Being able to be maintained in vitro for up to two years [119], they could reach later stages of neurodevelopment compared to those that can be studied with 2D cultures and, thus, produce later-born neural cells, including astrocytes and oligodendrocytes [119][120].

One of the first study on brain organoid deriving from cells of patients affected by idiopathic ASD and characterized by macrocephaly [69] reported abnormalities in cell-cycle and synaptic growth. In particular, they noted an increment in the expression of the transcription factor FOXG1 that correlated with an increased production of inhibitory neurons. The study highlights the role of this gene and suggests it as a potential therapeutic target [69]. More recently, Schafer and colleagues [121] performed a large study, based on a selected cohort of macrocephalic ASD patients, in which they combined direct iPSCs-to neuron conversion, transcriptomic analysis and cerebral organoids generation. This strategy made it possible to clarify that ASD-related neurodevelopmental abnormalities are triggered by a specific temporal sequence of gene networks dysregulation. The study showed different results in forebrain organoids than in iPSC-derived neurons. In particular, ASD alterations were well recapitulated in organoids, while the direct conversion of iPSCs to mature neurons abolished ASD-associated phenotypes [121]. Owing to the fact that CHD8, a gene encoding for a chromatin-remodeling factor, is mutated in a subgroup of patients with ASD and schizophrenia (SZ), some authors performed an RNA-seq analysis of cerebral organoids derived from iPSCs that are heterozygous for a CHD8 knockout allele, and from isogenic controls [122]. The study showed that CHD8 regulates the expression of other genes implicated in ASD and SZ, in particular TCF4 and AUTS2, and a large overlap was observed for DEGs found by Mariani et al. [69], especially for genes involved in GABAergic interneuron development. Pathway analysis of DEGs revealed an enrichment of genes involved in regulating Wnt/β-catenin signaling, a druggable pathway [122].

Organoids were used also to study RTT pathogenesis. In particular, Mellios and colleagues [123] analyzed alterations in different neuronal processes, such as neurogenesis, differentiation, and migration, in MECP2-deficient and patient-derived cerebral organoids, while, more recently, Xiang et al. [124] performed a transcriptome analyses revealing a cell-type-specific impairment in specific regions of brain organoids carrying MECP2 mutations.

In a recent study performed by combining CRISPR/Cas9 genome editing and brain organoids, Blair et al. [125], investigating the “two hit hypothesis” model of cortical tuber formation, demonstrated that homozygous, but not heterozygous, loss of either TSC1 or TSC2 impairs the developmental suppression of mTORC1 signaling. Moreover, they demonstrated that the development of TSC phenotype in organoid could be prevented by treating them with rapamycin [125][126].

Brain organoids were also successfully obtained from patient affected by TS in a study that represents the first example of fused organoid approach for the in vitro study neuronal circuits involving different brain regions [127]. In particular, authors studied the migration pattern of inhibitory neurons during brain development using live imaging of TS-forebrain assembloids (fused cerebral organoids resembling the dorsal and ventral forebrain regions). They demonstrated that TS interneurons display a cell-autonomous defect consisting in overall delayed migration from the ventral to the dorsal forebrain [127]. The functional phenotype was rescued by treatment with nimodipine, a drug inhibiting the activity of L-type calcium channel.

Very recently, brain organoids were studied to go deep inside into the pathological mechanisms underlying AS [128]. The study demonstrated that UBE3A suppresses neuronal hyperexcitability via ubiquitin-mediated degradation of calcium and voltage-dependent big potassium (BK) channels. Thus, the use of a BK channels antagonist could normalize neuronal excitability ameliorating also seizure susceptibility [128].

Current Challenges for the Applicability of Brain Organoids in ASD Modeling

Considering all the above reported studies (summarized in Table 2), besides the high cost of culturing organoids, there are still some challenges facing their use for studying ASD. As compared to 2D monolayer, 3D cultures can be more heterogeneous, displaying high variability in both the structure and the composition of organoids between cell lines, between individual experiments using the same cell lines and even between single organoids derived from the same cell line in the same experiment [129]. The high variability across batches is often the result of the stochastic nature of spontaneous neural in brain organoids, thus making quantitative studies challenging.

Table 2. Summary of main iPSCs-based studies as a model of ASD.

Disease Genetic Mutations
in Samples (n)
iPSCs-Based Models Relevant Findings Effective Drugs Reference
Non-syndromic ASD different
no ASD-related
variants (3)
neurons and
astrocytes
decreased synapses and
release of excitatory
neurotransmitters, glial
dysfunction, and high
levels of IL-6
anti-IL-6 [31]
  different
no ASD-related
variants (8)
NPCs and
neurons
increased proliferation in NPCs, abnormal
neurogenesis, reduced
synaptogenesis, and
decreased release of
inhibitory/excitatory
neurotransmitters
IGF-1 [35]
  different
no ASD-related
variants (3)
NPCs hyperproliferation
of NPCs
  [36]
  rare compound
heterozygous
missense variants in
RELN (1)
NPCs impaired crosstalk
between mTORC1 and Reelin-DAB1 pathways
rapamycin [37]
  de novo balanced
translocation in
TRPC6 (1)
NPCs and
neurons
abnormal neuronal
development and
morphology, fewer dendritic spines and synapses
IGF-1 and
hyperforin
[38]
  loss-of-function
mutations in FOXG1 (4)
neurons
and brain
organoids
overproduction of
GABAergic neurons and GABA
neurotransmitter
  [69]
  heterozygous
loss-of-function
mutations in SHANK2 (2)
neurons increased dendrite length and complexity, synapse number, and frequency of
spontaneous excitatory
post-synaptic currents
agonist of mGluRs DHPG [70]
  different
no ASD-related
variants (8)
brain
organoids
neurodevelopmental
abnormalities triggered
by temporal
dysregulation of
specific gene networks
  [121]
  heterozygous
knockout of
CHD8 (1)
brain
organoids
enrichment of genes
involved in GABAergic
interneuron
development and
Wnt/β-catenin
signaling
  [122]
RTT missense, frameshift and nonsense
mutations in MECP2 (4)
NPCs and
neurons
reduced soma size,
dendritic spine
densities and synapses,
altered Ca2+
signaling, and
electrophysiological
defects
IGF-1 and
gentamicin
[39]
  frameshift mutation in
MECP2 (1)
NPCs and
neurons
increased frequency
of de novo
LINE-1
retrotransposition
  [40]
  different
duplications in
MECP2 (3)
NPCs and
neurons
altered expression of
neuronal progenitor genes, increased
synaptogenesis and dendritic complexity with altered
network synchronization
histone deacetylase
inhibitor
NCH-51
[41]
  large
deletion in
MECP2 (1)
NPCs and
cortical neurons
repressed translation and
decreased
ribosome engagement of NEDD4-family
ubiquitin ligases
  [42]
  missense mutations in MECP2 (2) neurons impaired microtubule
network and decreased
acetylated α-tubulin
selective
inhibitors of HDAC6
[71]
  missense and
nonsense mutations in MECP2 (3)
neurons and
astrocytes
neuronal
morphological
abnormalities mediated
by mutant astrocytes
IGF-1 and GPE [105]
  missense and
nonsense mutations in MECP2 (2)
astrocytes perturbed astrocyte
differentiation
  [106]
  missense and frameshift mutations in MECP2 (2) brain
organoids
impaired neurogenesis,
neuronal differentiation
and migration
  [123]
  missense and
nonsense mutations in MECP2 (3)
brain
organoids
cell-type-specific
impairments
BET
inhibitor JQ1
[124]
CDKL5 disorder missense and
nonsense mutations in CDKL5 (2)
neurons decreased density of
dendritic spines and
reduced number of
excitatory synapse
  [72]
  translocation t(7;X)
inactivating
CDKL5 (1)
neurons decreased density of
dendritic spines and loss of
synaptic contacts
  [75]
FXS >200 CGG repeats in 5′UTR FMR1 (3) NPCs abnormal expression of key NPC genes (SOX1,
NOTCH1, PAX6)
  [43]
  >200 CGG repeats in 5′UTR FMR1 (4) NPCs impaired Ca2+ signaling
affecting neuronal
differentiation
  [44]
  >700 CGG repeats in 5′UTR FMR1 (3) neurons impaired neuronal
differentiation and
maturation
  [76]
  FMR1 knockout (2) neurons abnormal synaptic
transmission, neuronal
differentiation, and cell
proliferation
  [80]
  >700 CGG repeats in 5′UTR FMR1 (3) neurons altered neurite
outgrowth and
branching defects
  [81]
  94 CGG repeats in 5′UTR FMR1 (1) neurons dysregulated Ca2+
signals, reduced
synaptic protein
expression, and
shorter neurites
  [82]
TSC de novo mutations in
TSC2 (2)
NPCs and
neurons
delayed neuronal
differentiation
  [45]
  nonsense mutation
in TSC1 (1)
NPCs enhanced proliferation,
aberrant neurite
outgrowth, and
enlarged cell size
rapamycin [46]
  splicing mutation in TSC1 (1) neurons enlarged soma,
decreased neurite length, and abnormal connections
  [83]
  de novo mutation
in TSC1 and frameshift mutation in TSC2 (2)
co-cultures of
cortical
neurons and
oligodendrocytes
cellular hypertrophy and
increased
axonal density
rapamycin [84]
  single or biallelic
mutations in
TSC2 (2)
neurons morphological changes rapamycin [86]
  loss-of-function
mutations in TSC1 and TSC2 (2)
brain organoids impaired
developmental
suppression of mTORC1
signaling
by loss of either
TSC1 or TSC2
rapamycin [125]
PMDS small/large 22q13.3 deletions and frameshift mutation in SHANK3 (7) NPCs disrupted neurogenesis
leading to altered
excitatory/inhibitory balance
  [47]
  22q13
deletion (2)
neurons impaired excitatory synaptic transmission IGF-1 [87]
  de novo truncating and frameshift
mutations in SHANK3 (2)
neurons impaired excitatory synaptic transmission lithium
and valproic acid
[88]
  de novo truncating mutations in SHANK3 (4) pyramidal
neurons
decreased dendritic spines and altered spinogenesis   [89]
  heterozygous and
homozygous SHANK3
deletions (2)
neurons decreased neurite
outgrowth,
hyperexcitability,
increased input
resistance, and
disrupted excitatory synaptic transmission
  [90]
TS G406R missense
mutation in CACNA1C (5)
NPCs and
neurons
dysregulated Ca2+
signaling, impaired neuronal
differentiation,
increased TH and
catecholamine
expression
roscovitine [48]
  G406R missense
mutation in CACNA1C (3)
NPCs dysregulated Ca2+
signaling affecting
neuronal development and function
  [49]
  G406R missense
mutation in CACNA1C (2)
neurons Ca2+-dependent
dendritic retraction and
altered cellular
structure
C3
transferase
[91]
  G406R missense
mutation in CACNA1C (3)
neurons altered differentiation in the developing
cortex
  [92]
  G406R missense
mutation in CACNA1C (3)
brain organoids delayed migration of
inhibitory neurons
nimodipine [127]
AS maternal 15q11-q13 deletion including UBE3A (2) neurons no phenotypic
alterations
  [93]
  3bp deletion in the
maternally inherited
UBE3A (1)
neurons late paternal UBE3A
silencing during
neuronal
differentiation
  [96]
  large 15q11–q13
deletion (3)
neurons reduced synaptic
activity and plasticity
  [97]
  15q11.2-q13
microdeletion
including UBE3A (1)
brain organoids neuronal
hyperexcitability
BK
channels
antagonist
[128]
PWS paternal 15q11-13
deletion (1)
neurons no phenotypic
alterations
  [93]

BET, bromodomain and extra-terminal; BK, voltage-dependent big potassium channels; DHPG, 3,5 dihydroxyphenylglycine; GPE, peptide containing the first 3 amino acids of IGF-1; HDAC6, histone deacetylase 6; IGF-1, insulin-like growth factor 1; NPCs, neural progenitor cells; TH, tyrosine hydroxylase.

A limitation to the use of brain organoids for ASD modeling includes the lack of transport of nutrients and oxygen to cells through the vascularization which can ultimately induce hypoxia and inner necrosis. This also represent an obstacle to the study of blood-brain-barrier (BBB) interactions that is relevant for drug delivery to the brain. Moreover, the lack of vascularization in the neural tissue affects long-term maturation of cerebral organoids, which is extremely relevant to achieve a high degree of cellular complexity and neuronal maturity, including formation of dendritic spines and spontaneously active neuronal networks.

Although brain organoids contain most of the cerebral cell types, microglia are absent from iPSCs-derived brain organoids because of its embryonic origin distinct from that of neural progenitors [130]. As microglia regulate the synaptic pruning, thus contributing to the formation and maintenance of neural circuits [131], it is, therefore, difficult to model these cellular aspects of ASD.

4. Use of ASD Models for Drug Discovery and Development

The use of iPSCs as a tool has helped to unveil not only the etiology of ASD, but also aided the progress of the therapeutic areas. Mouse models have routinely been used to test drug candidates, but those identified to date have shown low efficacy in humans, thus limiting their translational potential [132][133]. Moreover, the development of drugs for ASD treatment is still challenging due to the high heterogeneity of the phenotypes, the limited understanding of its pathophysiology, and difficulties in modeling ASD both in vitro and in vivo.

Besides their value for the uncovering of cellular and molecular phenotypes underlying ASD, human iPSCs-based technologies have offered novel possibilities for personalized medicine and for screening drug candidates that can rescue normal phenotype and function. Among them, different iPSCs studies provided evidence that IGF-1 ameliorates some physiological deficits associated with ASD, both in non-syndromic [35][36] and syndromic forms [39][87][105]. In particular, this growth factor was able to restore impaired neuronal network [35], synaptic deficits [38][39][87], or neuronal morphological abnormalities [105] in iPSCs-derived neurons. The evidences coming from iPSCs-based studies in RTT and PMDS modeling have led to a stage II clinical trial on IGF-1 for the treatment of idiopathic and syndromic ASD with results expected in 2022 (https://ClinicalTrials.gov; protocols numbers: NCT01970345; NCT01894958; NCT01777542; NCT01525901; NCT01253317) [134][135]. Furthermore, gentamicin treatment on RTT iPSCs-derived neurons enhanced MECP2 protein levels and increased glutamatergic synapse, further confirming that patient-specific iPSCs can correct neuronal phenotypes [39]. Given MECP2 function at the epigenetic level, some authors planned to screen a library of 43 compounds with defined activity on epigenetic pathways in order to test the reversibility of the alterations observed in iPSCs-derived neurons harboring MECP2 duplicated gene. Among them, the histone deacetylase inhibitor NCH-51 was validated as a potential clinical candidate [41]. Intriguingly, in another study performed on iPSCs from MECP2-mutated neurons, phenotypic abnormalities were reverted by the treatment with selective inhibitors of HDAC6, the main α-tubulin deacetylase [71]. As mentioned above, other promising results were achieved by roscovitine that can reverse altered expression of TH and increased production of norepinephrine and dopamine displayed in iPSCs-derived neurons from TS individuals carrying a mutation in CACNA1C gene [48]. Additionally, the pharmacological intervention with rapamycin, mTOR regulator, successfully recapitulated the increased neuronal activity and morphological changes in TSC iPSCs-derived neurons, suggesting that these cells can also respond to existing drugs in vitro [84][86][125]. In this regard, it should be noted that clinical studies already showed encouraging improvements in TSC patients after treatment with rapamycin [136].

The aforementioned findings are very promising and suggest that disease-specific models based on iPSCs may represent an emerging and scalable platform for developing novel therapeutic agents targeting molecular mechanisms for ASD treatment (Figure 2). Since iPSCs are renewable, they can provide unlimited cellular resources for large-scale high-throughput screening (HTS). In this regard, one HTS was performed in iPSCs-derived cortical neurons from ASD individuals harboring SHANK3 mutations to search for compounds that rescue SHANK3-associated phenotypes by increasing its mRNA levels. Among 202 tested compounds, lithium and valproic acid were identified as agents with the best efficacy to correct SHANK3 haploinsufficiency, demonstrating that iPSCs can offer a novel cellular platform for developing specific disease-modifying treatments [88]. However, HTS platforms for drug discovery are still under development and require further standardization, including a homogeneity of cell types and a speeding up of the neuronal maturation by improving the differentiation protocols. Although the current advances in iPSC-based systems hold great promises for drug discovery, these technologies cannot completely replace animal models for preclinical evaluation of drugs.

Figure 2. Schematic representation of iPSCs-based models for drug discovery and development in ASD. Specific iPSCs can be isolated from patients with genetic ASD and can be further differentiated into patients-specific iPSCs or 3D self-organized in brain organoids. Potential drug screening can be performed in both 2D cultures of iPSCs-derived cells types of the CNS and in brain organoids. Selected drug candidates can be then firstly tested in in vivo models for safety, pharmacology, and toxicity and then used for clinical trials in humans. This figure was created with BioRender.com (accessed on 11 February 2021).

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