Abstract
Due to an inability to ethically access developing human brain tissue as well as identify prospective cases, early-arising neurodevelopmental and cell-specific signatures of Schizophrenia (Scz) have remained unknown and thus undefined. To overcome these challenges, we utilized patient-derived induced pluripotent stem cells (iPSCs) to generate 3D cerebral organoids to model neuropathology of Scz during this critical period. We discovered that Scz organoids exhibited ventricular neuropathology resulting in altered progenitor survival and disrupted neurogenesis. This ultimately yielded fewer neurons within developing cortical fields of Scz organoids. Single-cell sequencing revealed that Scz progenitors were specifically depleted of neuronal programming factors leading to a remodeling of cell-lineages, altered differentiation trajectories, and distorted cortical cell-type diversity. While Scz organoids were similar in their macromolecular diversity to organoids generated from healthy controls (Ctrls), four GWAS factors (PTN, COMT, PLCL1, and PODXL) and peptide fragments belonging to the POU-domain transcription factor family (e.g., POU3F2/BRN2) were altered. This revealed that Scz organoids principally differed not in their proteomic diversity, but specifically in their total quantity of disease and neurodevelopmental factors at the molecular level. Single-cell sequencing subsequently identified cell-type specific alterations in neuronal programming factors as well as a developmental switch in neurotrophic growth factor expression, indicating that Scz neuropathology can be encoded on a cell-type-by-cell-type basis. Furthermore, single-cell sequencing also specifically replicated the depletion of BRN2 (POU3F2) and PTN in both Scz progenitors and neurons. Subsequently, in two mechanistic rescue experiments we identified that the transcription factor BRN2 and growth factor PTN operate as mechanistic substrates of neurogenesis and cellular survival, respectively, in Scz organoids. Collectively, our work suggests that multiple mechanisms of Scz exist in patient-derived organoids, and that these disparate mechanisms converge upon primordial brain developmental pathways such as neuronal differentiation, survival, and growth factor support, which may amalgamate to elevate intrinsic risk of Scz.
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Introduction
Schizophrenia (Scz) typically emerges in early adulthood and is a chronic brain disorder that affects ~1% of the population. Upon onset, Scz neuropathology is already sufficiently vast that mechanistic studies have failed to pinpoint definitive causes of disease, as well as whether pathology identified in postmortem studies are causes or consequences of disease progression. While adolescent brain development is established as a critical period for Scz onset [1], Scz appears to maintain earlier developmental origins [2]. Due to ethical and technical constraints that prevent the collection of biological specimens at early developmental time-points, pre-disease signatures of Scz prior to adolescence remain unknown. Thus, defining the timing of developmental neuropathology in Scz, as well as the temporally specific involvement of putative biological risk factors, could lead to the identification of common pathways regulating ontogenesis of disease.
Evidence that Scz risk may begin to accumulate in utero has been collected for decades now, and epidemiological evidence suggests that prenatal stress [3], prenatal famine [4], early vitamin D deficiency [5], as well as maternal immune challenges [6, 7] may elevate Scz risk. Indeed, risk may manifest as early as the first trimester of brain development [3]. However, little is known of the mechanisms involved in prenatal Scz risk, and almost all knowledge of Scz developmental phenotypes has emerged from maternal immune activation (MIA) models [8,9,10,11,12,13,14,15,16,17,18,19,20,21,22,23,24]. MIA Scz models have reported increased cell death [20] as well as delayed axon development [21], and have also unveiled alterations in tonic neurotrophic support in vivo (e.g., BDNF and TrkB expression) [22], perturbations in neuronal differentiation of progenitors in vitro [23], as well as effects on new-born neuron birth in vivo [24]. In addition, these phenotypes are of particular noteworthiness given that similar alterations have been observed in Scz postmortem studies. This includes alterations in growth factors (e.g., BDNF, NT-3, and NT-4) [25,26,27], neurotrophin receptors [28, 29], cell death markers [30], neural stem cell proliferation [31], and reduced new-born cell numbers [32]. Together, these animal and human studies implicate that factors and pathways related to brain development may regulate Scz risk.
Genetic studies have also converged upon brain development factors as loci of Scz risk. Analysis of tens of thousands of Scz patients has revealed at least 108 prominent loci of risk [33], including previously unknown regions that may encode or modify regulators of neurodevelopment, growth factors, as well as other proximal genes (e.g., Pleiotrophin, otherwise known as PTN [33]). However, many association studies have also produced inconsistent linkage (for e.g., the BDNF gene locus, see discussion in [34,35,36]). Therefore, mechanisms of Scz have remained not just elusive, but also speculative.
To overcome these gaps, here we generate patient-derived cerebral organoids to investigate early developmental pathology of Scz in 3D human-derived tissue. We found that Scz cerebral organoids exhibited abnormalities in ventricular zone progenitors, which died at increased rates and also exhibited disrupted neuronal differentiation. There was a corresponding depletion of neuron numbers in 3D cortical assemblies of Scz organoids. In a search for the molecular underpinnings of these neurodevelopmental features, we adapted unbiased mass-spectrometry and found that Scz organoids differed not in their molecular diversity, but rather in their expression of development factors (POU-domain transcription factors, e.g. POU3F2/BRN2) as well as potentially novel Scz risk factors and putative growth factors (e.g. PTN). Single-cell RNA-sequencing (scRNA-Seq) confirmed that Scz organoids were depleted of progenitors and neurons, principally due to remodeling of progenitor transcriptomes yielding altered differentiation trajectories. In addition, scRNA-Seq confirmed the depletion of BRN2 and PTN gene-expression in Scz progenitors and neurons. In separate experiments, we modulated BRN2 or PTN levels in Scz organoids and found that both factors rescued neuron numbers, albeit via seemingly different mechanisms. In sum, high-content analysis revealed cell-specific neuropathology and multiple mechanisms of Scz within 3D patient-derived organoids, which unveiled distinct developmental pathways and novel disease factor mechanisms that may contribute to Scz risk during early corticogenesis.
Results
Patient-derived Scz organoids exhibit ventricular entropy and neuropathology
To study neurodevelopmental aspects of Scz we generated self-assembling, self-maturating, and human-derived cerebral organoids [37]. Cerebral organoids recapitulate transcriptomic [38] and epigenomic [39] programs of fetal development that drive the assembly of ventricular progenitor zones that give rise to neuronal ensembles [7, 8]. This broadly mimics the first trimester of human brain development [37, 40], and these organoids have already been successfully used to understand mechanisms of cortical development and disease [41,42,43]. Recent organoid models often apply exogenous growth factors (e.g., BDNF [44,45,46], NT-3 [46], and EGF [46]) and/or pathway modulators (e.g., TGFβ and WNT pathway inhibitors [47, 48]) to forcibly direct the differentiation of progenitors towards a neuronal fate or promote their survival by reducing apoptosis. However, factors such as BDNF and related neurotrophins [25,26,27, 35], TGFβ [49,50,51,52,53,54], and WNT signaling [55,56,57,58,59,60] (as well as other morphogens) are longstanding contributors to Scz pathophysiology and may play a role in the ontogenesis of disease during early neurodevelopment. Indeed, these same factors and pathways have hypothesized roles in early disease development via their effects on stem cells and neuronal programming [61]. Another consideration was the degree to which cerebral organoids faithfully recapitulate cellular diversity of the developing cortex. Notably, cerebral organoid models [37,38,39,40] have reported concordant expression of all major developing neural cell-types found in the developing cortex [62,63,64,65,66,67,68] including late originating lineages also implicated in post-mortem schizophrenia studies (e.g., oligodendroglia and astrocytes) [69, 70]. Therefore, given our particular interest in disease modeling, we adapted a morphogen-free organoid protocol that recapitulates cell-types of interest whilst avoiding the potentially confounding effects of exogenous morphogen factor exposure [37].
We consequently generated 3D cerebral organoids from healthy controls (Ctrls; who had neither personal history nor known first-degree relatives with a Scz diagnosis) and idiopathic Scz cases (for clinical notes see Supplementary Table 1, and for sampling see Supplementary Table 2). Cerebral organoids generated from both Ctrl and Scz patients were subjected to rolling quality control assessments (see “Methods”) and all iPSC lines exhibited reproducible LC/MS intensities and minimal (<2%) batch variation (see Fig. S1). This quality control assessment ensured that all iPSC lines, and groups, produced 3D tissue that was approximately analogous in composition, making 3D tissue generated from Ctrls and Scz suitable for comparison between and within groups. Organoids also routinely exhibited the formation and presence of ventricles and ventricular zones that were comprised of neural progenitors (SOX2+, and NESTIN+ progenitor cells) that produced extensive neuronal fields (filled with β3+ and MAP2+ neuronal cells). Similar to Ctrl organoids, Scz organoids also exhibited extensive neural induction that was defined by the presence of NESTIN+ fibers and SOX2+ progenitor-enriched ventricular zones (see Fig. 1b). However, relative to Ctrls, Scz organoids exhibited ventricular zones that appeared smaller than Ctrls and cortical fields that were more sparsely filled with neurons. These phenotypes mutually suggest that Scz progenitors may be prematurely dying or unable to initiate neurogenesis. An analysis of progenitor cell death in a large number of iPSC donors (n = 20–21 human iPSCs; Ctrl = 4–5 donors and Scz = 15–17 patients) revealed that Scz progenitors exhibited both a significant increase in ventricular progenitor cell death (Fig. 1c) and a significant decrease in the number of neurons within Scz cortical fields (Fig. 1d). In an independent, pseudorandomly sampled cross-sectional cohort, increased apoptosis was replicated in Scz organoids via three independent markers of cell death induction (increased DNA fragmentation, pH2AX+ DNA damage, and PARP+ cells, see Fig. S2). This suggests that due to increased ventricular progenitor death, fewer Scz progenitors are able to successfully differentiate into neurons.
However, these data do not rule out the possibility that Scz progenitors that were not the subject of premature death may also exhibit a difference in their neurogenic potential. That is, while progenitor cell death is likely to be an important rate-limiting factor in the production of neurons within Scz organoids, it was also possible that other mechanisms may simultaneously restrain new-born neuron generation in Scz organoids. To resolve this, we adapted a BrdU pulse-chase paradigm that comprised 24 h BrdU pulse and a 7 d chase period (Fig. 1e) that would identify if an intrinsic difference in the proportion of new-born neurons being generated also co-existed within Scz organoids. Following our pulse-chase regime, we harvested organoids and examined the proportion of BrdU+ proliferating progenitors that underwent neuronal differentiation (BrdU+ CTIP2+) or progenitor self-renewal (BrdU+ PAX6+) within the same field. This allowed us to map neuronal cell fate decisions as well as determine whether Scz progenitors were preferentially self-renewing instead of generating neurons. In Ctrl organoids, progenitors predominantly differentiated into early-born neurons within our 7 d chase period. However, Scz organoids exhibited significantly disrupted neurogenesis relative to Ctrls (48.6% vs 16.1% in Scz organoids). In sum, these data revealed that neuronal loss in Scz organoids was found to arise from an amalgamation of both elevated apoptosis and decreased neurogenesis.
Proteome mapping reveals enrichment for disease factors in Scz organoids
Having identified two cellular phenotypes (progenitor death and disrupted neuron numbers) in our Scz organoids, our next goal was to identify and define the molecular candidates responsible for these effects. To do this, we employed high-throughput, unbiased, and computational tools to deconvolute the molecular architecture of Scz organoids. A major goal of this approach was to resolve novel Scz disease signatures at the posttranslational level. In addition, we also sought to determine whether known disease factors and pathways from the Scz GWAS literature were recapitulated in Scz patient-derived organoids.
To map the proteome of 3D human-derived organoids, we adapted Tandem Mass Tag (TMT) chemistry to globally barcode peptides isolated from Ctrl and Scz cerebral organoids. This allowed a pseudorandomly selected cross-section of organoid samples to be pooled into a single multiplexed suspension that could be simultaneously subjected to quantitative Liquid Chromatography-Mass Spectrometry (LC-MS; Fig. 2a). This approach identified 3772 proteins, of which ~97.4% were quantifiable. The most abundantly expressed proteins, evidence of neuronal enrichment, and differentially expressed candidates are presented in Supplementary Tables 3–8. Remarkably, the overlap in protein identities between Ctrl and Scz cerebral organoids was almost complete (99.95% similarity in protein diversity in this particular sample) with only two proteins being unique to Scz cerebral organoids (WASL & MPV17; Fig. 2b and Fig. S3 for further data and discussion). The reproducibility of samples was robust in this dataset (Fig. S3d), and even at the single-protein level coefficients of variation remained low for over 3000 identified peptides (Fig. 2c). Indeed, at baseline, only 3 of 3671 (or, ~0.08% of the entire organoid proteome) exhibited substantial variability. Therefore, while undirected cerebral organoids varied in their morphologies and appearance, their macromolecular composition was found to be relatively stable and consistent. In addition, both Ctrl and Scz cerebral organoids exhibited enrichment for neuronal and brain developmental pathways (e.g., axons, neurogenesis, postsynaptic density, neuron projection development and WNT signaling; see Supplementary Table 4). This once more provided independent confirmation that neural induction was universally achieved.
Although the diversity of proteins in Ctrl and Scz organoids were very similar, further computational analysis revealed notable differences in the quantity of peptides within Scz organoids. Analysis of global Log2 intensities revealed that 222 proteins, reflecting ~5.9% of the proteome, differed in expression between Ctrl and Scz organoids (Fig. 2d). Of these proteins, 151 were up-regulated and 71 were down-regulated. Interestingly, peptide fragments of POU-domain containing transcription factors were identified in Scz organoids. This is of note, as the upper-layer cortical neuron marker and forebrain-specific transcription factor, POU3F2 (BRN2), is prominently involved in embryonic corticogenesis (see identity markers in [38]). BRN2 is an established initiator of neuronal differentiation [71] and BRN2 is also dysregulated in organoids with DISC1 disruption [72]. When differentially expressed proteins were screened against large-scale Scz gene association studies [33, 73], at least ~70 putative Scz risk proteins were discovered to be commonly present in organoids. Only 4 of these specific risk factors, PLCL1, PTN, PODXL and COMT, displayed significant differential expression in Scz organoids. Notably, PLCL1 (phospholipase-like C1; involved in GABAergic neurotransmission [74]) and PTN (pleiotrophin; a possible neurodevelopmental growth factor [75]) were significantly down-regulated in Scz organoids. Contrary to this, PODXL (podocalyxin; a neural adhesion molecule involved in axonal fasciculation, neurite outgrowth, and synaptogenesis [76]) and COMT (catechol-O-methyltransferase; involved in dopamine and catecholamine elimination [77] and cognitive response to antipsychotics [78,79,]) were innately up-regulated in Scz organoids (Fig. 2e). This suggests that neuropathology of Scz converges upon the disruption of common molecular factors with established disease risk, perhaps as a consequence of a shared disruption of broader regulatory networks.
Single-cell sequencing reveals aberrant cell-type diversity in Scz organoids
Next, to study disease signatures of Scz with greater resolution, both with respect to cell-specificity and capture potential, we employed scRNA-Seq. To do this, we used chromium microfluidic devices to generate single-cell nanodroplet emulsions that could then be broken and amplified for library preparation and sequencing (Fig. 2f).
Our high-content scRNA-Seq pipeline yielded 26,335 single-cell transcriptomes, comprising 20,844 captured genes that could be harmonized into 8 cellular clusters (Fig. 2f) identified against human fetal brain samples [79]. Replicating data from Figs. 1–2, there was decreased abundance of both progenitors (SOX2 and PAX6) and neurons (MAP2, DCX, and STMN2) in Scz organoids (Fig. 2g). Instead, Scz organoids exhibited abnormal enrichment for brain-related cell-types including neuroendothelia, myeloid, mural, choroid plexus, and retinal markers (Fig. 2f). Ctrl samples also exhibited these same cell-types but in lower abundance (~7% of all Ctrl cell-types, vs ~25% of Scz cell-types; Fig. 2h). Scz organoids therefore recapitulated all appropriate cell-types also present in Ctrl organoids but, due to disrupted differentiation (Fig. 1e), Scz organoids were defined by an increase in neuroendothelial-related cells and a decrease in neuron numbers.
Altered pseudotime trajectories reveals remodeling of Scz organoid cell-lineages
We next sought to determine whether alterations in differentiation and diversity in Scz organoids arose from transcriptomic remodeling of cell lineages. We computationally modeled the differentiation trajectories of organoids by harmonizing single-cell transcriptomes into principal components that exist in pseudotime [80]. This yielded differentiation trajectories of Ctrl and Scz organoids that were similar but subtly distinct (Fig. 3a). Ctrl organoids reflected enrichment of known neuronal programming factors with established mechanistic roles in neuronal differentiation (Fig. 3a). Contrary to this, Scz organoids were defined by different markers that were instead associated with pluripotency, cytoskeletal filaments, and neuroendothelia. This included POU5F1 (OCT4), the proliferation and apoptosis balancing factor CRABP1, and pan enrichment for the inflammatory factor IFITM3 in Scz organoids (Fig. 3a). In Scz organoids, the enrichment of POU5F1+ cells coincided with cell-type clusters that were broadly consistent with progenitors and developing neurons, indicating that these markers were expressed within cell-type clusters that already exhibited some evidence of neural induction. This indicates that these aberrant markers were over-populated in progenitor and neuronal clusters at the expense of other prototypic neuronal development factors and related cell-types. This analysis was also consistent with other up- and down-regulated developmental factors in Scz progenitors and neurons identified during unbiased clustering and analysis (discussed further below). Therefore, this statistical pseudotime analysis provided unbiased confirmation that Scz cell-lineages exhibited remodeling that putatively diverts progenitor differentiation away from neuron production within organoids.
Cell-specific encoding of neuropathology in Scz progenitors and neurons
We next sought to define the specific transcriptional factors responsible for the disrupted neurogenic potential of SOX2+ Scz progenitors (Fig. 3b). Numerous transcriptional regulators of differentiation were down-regulated in Scz progenitors, including a depletion of axon development pathway factors (Fig. 3b). Intriguingly, delayed axon development is also a known sequelae of in utero animal models of Scz [81]. Many of the axon development factors identified here also regulate neuronal differentiation and development (e.g., HOXA2, AUTS2, MAP2, SLITRK6, WNT2B, NRN1). Prominently, this included the depletion of BRN2 in Scz progenitors. Down-regulation of Neurotrophin-3 mRNA (NT-3 or NTF3) was also detected in Scz progenitors. Consistent with pseudotime analyses, Scz progenitors exhibited abnormal enrichment for structural, filament, adhesion, and angiogenic pathways (see Fig. 3b). Therefore, we identified that Scz progenitors exhibited depletion of an ensemble of development factors that promote neuronal differentiation and potentiate early neuronal development.
We next sought to determine if developing neurons also exhibit cell-specific signatures of Scz. Similar to progenitors, several neuronal development factors remained down-regulated in Scz neurons including BRN2. Neuronal filament factors (e.g., NEFM) and guidance factors (e.g., ROBO3 and NTNG2) were also disrupted in Scz neurons. Curiously, we identified enrichment for Pl3K-Akt signaling (see Fig. S4) as well as a growth factor binding pathway in Scz neurons (Fig. 3c). This included down-regulation of the TrkA (NTRK1) receptor and the up-regulation of the neurotrophin cleavage factor, FURIN. In humans, FURIN localizes to one of 108 Scz loci with genome-wide significance [33]. In support of this, interactome modeling revealed potential interplay between growth factor binding factors that may be initiated by interactions related to FURIN and TrkA at the posttranslational level (Fig. 3d). The interleukin-6 signal transducer (IL6ST), which was up-regulated in Scz neurons, may be downstream of FURIN and TrkA based on interactome modeling (Fig. 3d). Notably, FURIN is responsible for cleaving immature neurotrophins into their mature isoforms, and the differential expression of these identified pathways (e.g., growth factor binding and Pl3K-Akt signaling factors) is broadly consistent with a compensatory response to diminished neurotrophin signaling. This suggests that growth factor binding factors, including FURIN, may be enriched in neurons to compensate for broadly diminished growth factor signaling via TrkA, which is a known regulator of neuronal differentiation, development, and survival.
Cell-specific neurotrophin alterations in Scz progenitors and neurons
The down-regulation of NT-3 in Scz progenitors and TrkA in Scz neurons in unbiased statistical modeling indicates that other discrete patterns of neurotrophin dysfunction may exist. Deeper hypothesis-driven analysis revealed that Scz progenitors also tended to exhibit down-regulated BDNF, but up-regulated NT-4, gene-expression. Correspondingly, we identified that TrkB (NTRK2) was the only down-regulated neurotrophin receptor in progenitors (Fig. 3e). Contrary to this, Scz neurons only exhibited a cell-specific down-regulation of TrkA (as described above; Fig. 3e). These data thus provide further evidence to support our hypothesis that divergent cell-specific neuropathology may converge upon common pathways in Scz organoids (e.g., growth factor support), resulting in related but non-overlapping cell-specific neuropathology of Scz between progenitors and neurons.
Identifying BRN2 and PTN as candidate disease factors in organoids
To identify potential mechanistic factors of Scz neuropathology in our patient-derived organoids, we examined whether proteome targets could be validated in our scRNA-seq transcriptomic datasets (see Fig. S5a, b). Global, as well as progenitor- and neuron-specific, analyses revealed that POU3F2 (BRN2) and PTN were depleted in Scz samples (Fig. 3f, g). Intriguingly, PTN holds disease relevance due to the proximity of an index SNP/novel locus with genome-wide significance in the largest Scz GWAS conducted to date (n = ~150,000 humans, see [33] and Fig. S6). On the other hand, BRN2 does not appear to be a genetic locus of Scz risk, but does exhibit some evidence of disease linkage in prior differential methylation studies (Fig. S6c). This suggests that BRN2 may be a commonly targeted downstream pathophysiological factor (see Scz database repository mining in Fig. S6). The neurobiology of these candidates only further amplified our interest, as BRN2 promotes the production of late-born neurons during embryonic development [71] and PTN is a putative growth factor that promotes cell survival [82, 83] as well as other neurodevelopmental processes. Importantly, informatic mining of the BrainCloudTM (dbGaP Accession: phs000417.v2.p1) database revealed that both BRN2 and PTN exhibit peak expression during prenatal human brain development (n = 269 time-points including n = 38 fetal samples, see Fig. S6a), making them bonafide embryonic targets that may be related to Scz risk during this period. In sum, these Supplementary Informatics analyses provided additional veracity for our core Scz phenotypes, providing confidence in the translational value of our 3D organoid cultures and their ability to recapitulate disruption of novel embryonic disease factors.
Modulating BRN2 levels in Scz progenitors rescues neurogenesis
Having established the reproducibility of our core phenotypes (progenitor death and neuronal loss) in Scz organoids, we next sought to mechanistically establish the functionality of the candidate rescue factor BRN2 within our Scz organoid system. BRN2 is a forebrain specific transcription factor expressed in neural progenitors as well as in migrating neurons in the mammalian brain (see Fig. 3 and [71]). When disrupted in vivo, stalled production of upper-layer neurons ensues, indicating a functional role for BRN2 in early cortical neurogenesis [71]. The endogenous disruption of BRN2 in Scz organoids (Figs. 2–3) implicated that BRN2 may be a downstream pathophysiological substrate of Scz neuropathology. We hypothesized that the robust down-regulation of BRN2 in Scz progenitors resulted in the disrupted neuronal differentiation observed in Scz organoids. To test this, we specifically supplemented BRN2 in Scz progenitors and assessed neuron numbers within the same Scz organoids. To do this, we used a sophisticated self-regulating viral construct (hPGK>BRN2:P2A:EGFP.MIRT1244, see Fig. S7a–c; hitherto BRN2-Virus) that maintained sustained production of exogenous BRN2-GFP expression within infected progenitor cells but not post-mitotic neurons (Fig. 4a, b, S7). This was achieved via a neuronal “off-switch” in viral transcripts, which was controlled by four recognition sites for the neuronal noncoding RNA miRNA-124 (MIRT-1244; for details see “Methods”). During the early stages of organoid development, tissue was infected with either a control-GFP (CTRL-Virus) or BRN2-GFP lentivirus (Fig. 4a), leading to viral expression within neural progenitors as expected (Fig. 4b). Whole-organoid images revealed that Scz phenotypes, such as neuronal loss, were independently recapitulated in Scz organoids (Fig. 4c, see also Fig. S8 for enlarged images of neuronal loss). Analysis revealed that BRN2-Virus+ Scz organoids exhibited a significant increase in BRN2+ late-born neuron numbers. Indeed, late-born neuron numbers were rescued to levels that were consistent with Ctrl organoids (Fig. 4d). In addition, due to a significant Group x Treatment interaction, MAP2+ neuron numbers were also increased in BRN2-Virus+ Scz organoids relative to CTRL-Virus+ Scz organoids (Fig. 4e). However, viral delivery of exogenous BRN2 to Scz progenitors failed to rescue increased rates of progenitor apoptosis within Scz organoids (Fig. 4f). While raw data are presented (Fig. 4) for transparency, further analysis of phenotypes by the average of individual iPSC lines reaffirmed that BRN2-Virus Scz organoids exhibited increased neuron numbers but no change in progenitor death (see Fig. S7). Together, these data establish that down-regulated BRN2 mechanistically contributes to neuronal differentiation, but not apoptosis, phenotypes in Scz organoids (Fig. 4). Therefore, due to our inability to rescue cell death phenotypes with BRN2-Virus, we considered the possibility that other disease mechanisms must be operating within Scz organoids.
PTN corrects neuron numbers in Scz organoids via neurotrophic-like effects
Recent work has established that PTN exhibits strong expression in neural progenitors (see [84] and Fig. S5a). We were also able to independently replicate the expression of PTN within progenitors here via scRNA-Seq (Fig. 3f, g). PTN has been suggested to play a role in early corticogenesis by promoting neuronal differentiation [85]. PTN can also protect neurons from apoptosis in vivo [82], possibly via endothelial-related cell-types which we also observed enrichment for here. Nevertheless, to determine whether PTN plays a role in early Scz pathology in our organoid system, we adapted recombinant human PTN as a morphogen to generate Vehicle- and PTN-Supplemented Ctrl and Scz cerebral organoids (Fig. 5a, see also enhanced Nestin expression profile in Fig. 5b). Similar to earlier experiments (Figs. 1, 2, 4), Scz phenotypes were recapitulated in Vehicle-treated Scz organoids and this included a significant increase in Scz progenitor apoptosis (Fig. 5c). However, PTN-treated Scz organoids exhibited a significant reduction in progenitor apoptosis (Fig. 5c, and S9a for enlarged whole-organoid images). PTN-treated Scz organoids exhibited increased new-born cell survival (Fig. S10) and thus significantly increased neuronal differentiation (Fig. 5d). This was reflected in the numbers of MAP2+ neurons, which were increased relative to Vehicle-treated Scz organoids (Fig. 5e; see also enlarged whole-organoid images in fig. S9b). Importantly, these phenotypes were replicated irrespective of whether data were analyzed as a pool or by the average of individual iPSC lines (see Fig. 5 and S11), and all successfully rescued phenotypes comprised significant Disease x Treatment interactions. In sum, these experiments collectively established that PTN mechanistically regulated new-born cell survival and thus neuron number in Scz cerebral organoids by simultaneously promoting neurogenesis and restraining apoptosis.
Discussion
The idea that Scz is defined by developmental pathology has been widely discussed in the literature, however, the timeline for when Scz-related pathology commonly commences has remained speculative. This is largely because of an inability to both access and ethically study developing human neural tissue in utero. Here we resolve, for the first time, that Scz is defined by cell-specific neuropathology and that multiple mechanisms operate within self-developing patient-derived neural tissue of human origin. While we discuss our results from patient-derived 3D cerebral organoids in the context of disease, it is important to emphasize that all organoid systems remain experimental models (i.e., they’re not a perfectly symmetric substitute for actual brain experimentation). Nevertheless, we believe the data from these systems are useful as they enable ethical access to, and control of, human cells in a 3D macroenvironment that is similar to early brain development. As such, we interpret our results with these caveats in mind. Notably, we report that a series of downstream alterations in Scz neuronal progenitors yielded a depletion of Scz neurons within Scz patient-derived organoids, which is indicative of neurogenesis defects similar to those reported in several animal models, 2D iPSC studies from schizophrenia donors, and postmortem analyses. However, the most important advances from this body of work remain our discovery of cell-specific neuropathology and multiple potential regulators of disease in a human-derived 3D tissue system, which fundamentally supports long-standing hypotheses on the developmental ontogeny of Scz.
In our organoid cultures, we first identified that the ventricular progenitor pool was defined by increased rates of cell death. In further experimentation (Figs. 1e and 3), we identified that Scz progenitors exhibited disrupted differentiation and did not produce neurons in expected quantities (Figs. 1e and 2f, g). In single-cell analyses, we determined that Scz organoids exhibited cell-specific reprogramming in both progenitors and neurons (Fig. 3b, c), that ultimately resulted in misdirected progenitor differentiation (Fig. 3a) and reduced growth factor support (Fig. 3c–e). This single-cell analysis identifies, for the first time, that neuropathology of Scz is vastly more complex than believed as disease signatures are likely to be encoded in a cell-specific manner within cellular lineages (e.g., progenitors vs neurons), leading to both similarities but also distinct differences between cell-types. Thus, different cellular identities may encode and exhibit unique and non-overlapping disease pathology of Scz (Fig. 3), leading to neuropathology that is encoded on a cell-by-cell basis.
Importantly, because cerebral organoids recapitulate in utero brain development, these experiments also establish that cell-specific mechanisms of disease are also likely to converge upon common mechanisms and/or pathways important for early brain development. Thus, while different cell-types may exhibit unique neuropathology of disease, our data also indicate that some similarities between cell-types are also likely to exist. Notably, we identified that both Scz progenitors and Scz neurons exhibited discrete growth factor alterations within the neurotrophin system family (Fig. 3e). In addition, we identified a gross depletion of BRN2 and PTN in Scz within progenitors and neurons (Fig. 3f, g). Importantly, in two separate rescue experiments, we exemplified that neuron numbers could be modulated when these mechanistic substrates are reconstituted back into Scz organoids. However, while BRN2 could modulate neurogenesis within Scz organoids, it could not rescue other Scz phenotypes (e.g., progenitor apoptosis; Fig. 4). Notably, PTN was putatively able to restrain apoptosis while simultaneously promoting neuronal development (Fig. 5). When amalgamated, these data also identify that ensembles of endogenously disrupted disease factors are capable of eliciting multiple potential mechanisms during early brain development.
Mechanisms of Scz have traditionally been studied within the adult nervous system. This is due to the protracted age of onset of Scz and relatively low incidence. However, there is also increasing debate whether disease phenotypes represent a ‘cause or consequence’ of disease in the adult brain. Meanwhile, for several decades, evidence has continued to accumulate that early brain development is a critical period for Scz risk. Yet, without a way to ethically acquire, study, and subsequently identify whether human fetal tissue would definitively become a future Scz case, little progress has been made in understanding early developmental mechanisms of Scz. In this respect, patient-derived cerebral organoids are technically and ethically a model system for studying self-developing human tissue in 3D. Notably, cerebral organoids recapitulate the earliest phases of brain development, including corticogenesis. Indeed, our scRNA-Seq revealed that Ctrl organoids predominantly comprised progenitors, proliferating cells, and developing cortical cell-types as expected (Fig. 2). TMT-LC/MS supported this by exemplifying widespread induction of neural ontology pathways required for brain development (see Supplementary Tables). Across a number of experiments, we identified critical differences between Ctrl and Scz organoids within the ventricular progenitor pool. Relative to Ctrls, we identified that ventricular progenitors in Scz organoids exhibited increased apoptosis and decreased neuronal differentiation. Critically, in a cell-fate pulse-chase experiment (Fig. 1e), we identified that Scz progenitors exhibited a dramatic decrease in neurogenesis alongside a concomitant increase in rates of differentiation into “other” neural-related cell-types. In a follow-up analysis of 26,335 single-cell transcriptomes, we identified the identity of these other cell-types. Namely, we found that an enrichment for neuroendothelial and neurovascular-related cell-types that, despite of their differences in lineage and ontogenesis, were seemingly produced at the expense of neurons (Figs. 2–3). In deeper analyses, we identified that Scz progenitors exhibited a reprogramming in their expression of neuronal differentiation markers (Fig. 3a, b), including transcription factors such as BRN2 that are almost completely diminished (Fig. 3f, g). Other altered factors in Scz progenitors comprised neuronal development factors, such as HOXA2, AUTS2, SLITRK6, WNT2B, NRN1, and NT-3, which also collectively orchestrate neuronal differentiation. Instead of exhibiting these expected cell-fate programming factors, Scz progenitors exhibited enrichment for extracellular matrix factors, actin filaments, cell-substrate adhesion, vascular-related metabolic processes, and angiogenic markers (Fig. 3a, b). In pseudotime trajectories, these factors predicted the altered differentiation trajectories of Scz progenitors away from neurogenesis and towards different cellular lineages (specifically, mural, myeloid, and endothelial cells; see Fig. 3a). While the numbers of these cell-types were abnormal in Scz organoids, it is nonetheless important to emphasize that these cells are necessary for brain development and are ordinarily found in Ctrl organoids too (Fig. 2f). Therefore, in sum, computational modeling subsequently identified the induction of altered cell-lineages in Scz organoids and the depletion of an ensemble of neuronal programming factors in Scz progenitors. This outlines a suite of novel neuropathology in developing human organoids that sheds light on possible early-arising alterations in the developing brain that may be related to intrinsic Scz risk.
As discussed above, a critical finding in our manuscript was the observation that Scz progenitors seemingly lacked the transcriptional machinery necessary to support neuron production and thus neocortical neurogenesis. To provide mechanistic support for this hypothesis, we sought to identify a neurogenic target that could be exogenously modulated in situ within organoids. This led us to focus on BRN2 (POU3F2), as Scz organoids exhibited robust down-regulation of this factor at the mRNA level as well as POU-domain fragments at the peptide level (Figs. 2e and 3f, g). Prior studies have implicated that BRN2 is important for the induction of progenitor differentiation into neurons within the developing cortex [71]. In addition, in a prior study it was reported that disruption of DISC1 resulted in elevated progenitor mitotic activity and altered BRN2+ neuron numbers [72], which mimicked the phenotypes reported here. This led us to target BRN2 in our first rescue experiment, whereby we utilized a self-regulating viral vector to deliver exogenous BRN2 selectively to Scz progenitor cells but not neurons. This led us to confirm that supplementation of BRN2 levels in Scz progenitors reinstated their neurogenic potential, yielding increased neuron numbers in Scz organoids (Fig. 4). Thus, with no major disease association at the genetic level (Fig. S6), these experiments established BRN2 as a forebrain-specific transcription factor that may contribute to Scz neuropathology as a downstream intermediary during early brain assembly. However, because BRN2 did not rescue Scz progenitor apoptosis, it was also apparent that yet further mechanisms were operating within our 3D Scz patient-derived organoids.
In addition to neuronal programming factors, Scz progenitors were further defined by cell-specific alterations in the expression of growth factors. This was of note, as growth factors regulate not only neurogenesis but also cellular survival. Growth factor alterations included the significant down-regulation of NT-3 (NTF3) and TrkB (NTRK2) gene-expression in Scz progenitors (Fig. 3e). Gene variants within NT-3 [86], and epistatic interactions between BDNF and TrkB gene variants [87], have previously been suggested to precipitate Scz risk. Intriguingly, functions linked to these neurotrophins were also hallmark neuropathology of Scz organoids. Indeed, neurotrophins and TrkB-mediated signaling are potent regulators of differentiation and survival [88] and likely elicit neuroprotective effects in Scz [89]. Neurotrophins also orchestrate transcriptional mechanisms of neuronal fate making [90,91,92] and protect neural stem cells from apoptosis via activation of Pl3K/MAPK signaling [93]. A disruption in growth factor homeostasis within Scz progenitors may therefore contribute to alterations in disrupted neurogenesis and increased progenitor cell death. Interestingly, NT-4 expression was selectively up-regulated in Scz progenitors, and Scz neurons exhibited none of these alterations but instead exhibited a substantial depletion of TrkA mRNA expression. These cell-specific differences are thus consistent with our suggestion of discrete cell-specific neuropathology, whereby cell-types belonging to the same overall cellular lineage may exhibit similar or convergent targeting of common pathways and/or targets via distinct effects. Thus, the convergence of both Scz progenitors and neurons upon neurotrophin dysregulation support this hypothesis. Additionally, the divergence in expression between these cell-types likely reflect differences in the temporal coordination and cell-specific actions [94] of individual neurotrophins [95, 96] during brain development. In this respect, it is possible that common pathways may be altered between cell-types via different mechanisms, similar to what we report in our rescue experiments (Figs. 4–5). Nonetheless, these data correspondingly evidence the cell-type specificity of growth factor neuropathology in Scz, and identify that a developmental switch in the expression of neurotrophin-related factors occurs as progenitors differentiate into neurons.
Disrupted neurotrophin homeostasis within the progenitor pool led us to target a putative growth factor for our second rescue experiment. Similar to our BRN2 rescue experiment, we assigned priority to factors that exhibited independent cross-validation at both the mRNA and peptide level within Scz organoids. This selection criterion led us to target PTN for our second rescue experiment. PTN was depleted in Scz progenitors and neurons (Fig. 3f, g) as well as in our proteomics assays (Fig. 2), and PTN also functions as a potential embryonic growth factor [97] in the developing cerebral cortex [98]. Evidence supporting a genetic association between PTN and Scz is defined by an index SNP in proximity to PTN that was identified in the largest-ever Scz GWAS (n = ~150,000) [33] (see also Fig. S6). However, because this comprised the discovery of a novel locus, the role of PTN in Scz has remained unclear and thus undefined. Here we discovered that PTN exerted neuroprotective effects in Scz organoids by restraining apoptosis whilst simultaneously promoting neurogenesis (Fig. 5). Therefore, we also mechanistically established that PTN positively regulated neuron numbers in Scz patient-derived organoids albeit via similar, yet independent, effects to BRN2 (see discussion below). While PTN is unlikely to be a good therapeutic target due to its diverse ‘yin-and-yang’ functionality in both the brain and periphery, this work identifies that novel Scz disease factors still remain to be discovered at the basic science level. Overall, these experiments establish that multiple Scz mechanisms are likely to be operational during corticogenesis within patient-derived organoids. However, we also cannot rule out that these mechanisms may differ depending on the composition of the patient subtypes being studied, which will be important for future organoid studies to both consider and address.
It is important to emphasize that our rescue experiments established that BRN2 and PTN rescue Scz neuron numbers via related, but distinctly different, effects. This principally included neuronal differentiation and survival. Our data exemplifies that both neuronal differentiation and survival factors are likely to be mutually important, and that disease-implicated factors likely amalgamate to alter neurodevelopment within Scz organoids. This is broadly supported by our Scz phenotypes described throughout the manuscript, including a depletion of normative neuronal development factors in progenitors (Fig. 3a, b) that potentially divert progenitor cellular lineages away from neurogenesis (Figs. 1e and 3a). Additional correlates included endogenously diminished growth factor support (e.g., Figs. 2e, 3e, f, g, 5), increased apoptosis (Figs. 1, S2, 4, and 5), and altered differentiation trajectories (Figs. 1e and 3a) in Scz organoids. Indeed, we were able to repetitively replicate progenitor death and neuronal depletion (Figs. 1, 2, 4, and 5). However, as shown in our two independent rescue experiments (Figs. 4–5), disrupted neuron production could only be reinstated if mechanistic substrates (e.g. BRN2 or PTN) were reconstituted in Scz organoids. Because BRN2 functions as a differentiation-inducing transcription factor and PTN as a growth factor, this suggests that alterations in neurogenesis and survival factors yielded an intrinsically ligated potential for cortical development within Scz organoids (Figs. 1e, 2f, g, 3a, 4, 5). Consistent with this, complete phenotypic rescue could only be achieved if progenitor apoptosis was normalized alongside neurogenesis; as was the case only in our PTN rescue experiments (Fig. 5) but not our BRN2 rescue experiments (Fig. 4). This disparity between our mechanistic rescue experiments exemplifies that numerous molecular agents are capable of regulating similar, yet also distinct, Scz neuropathology within patient-derived organoids, and that neurogenesis defects alone do not explain the breadth of Scz organoid phenotypes. Instead, these data support that mechanisms regulating cell death and neuronal differentiation are dysfunctional in self-developing Scz patient-derived organoids, resulting in a terminal upstream depletion of cortical neurons. This supports the idea that multiple mutual mechanisms operate within Scz organoids, and that Scz disease factors may target similar biological processes and pathways necessary for neurodevelopment.
While our work provides proof of principle that multiple factors regulate intrinsic neuropathology of Scz organoids, we believe that yet more mechanisms are likely to be operational in Scz organoids. Importantly, alterations in the availability of other Scz molecular factors may also produce differential or synergistic risk [99]. It will be particularly important to parse the functionality of Scz risk factors validated in both proteomics and scRNA-Seq. A prominent target may be another novel Scz risk factor with nascent genome-wide significance [33], namely PODXL (a neural adhesion molecule involved in axonal fasciculation, neurite outgrowth, and synaptogenesis [76]). Other targets included longstanding Scz risk factors such as PLCL1 (involved in GABAergic neurotransmission [74]) and COMT (involved in dopamine and catecholamine elimination [77] and cognitive response to antipsychotics [78]). These factors are therefore potential targets for unraveling yet further mechanisms of Scz risk.
Our unbiased datasets also identified several other potential disease factors that do not hold genetic association with Scz but exhibit face validity for future investigations. Namely, our data also revealed an intrinsic enrichment for the interferon-induced transmembrane factor IFITM3 in Scz organoids. IFITM3 enrichment was present across a multitude of cell-type clusters. In the postmortem Scz brain, enrichment of IFITM3 in the hippocampus [100], amygdala [101], and frontal cortex [102] has been reported and may reflect increased neuroinflammation. These phenotypes may be related to increased markers of oxidative stress in Scz neural progenitors [103, 104]. Interestingly, IFITM3 has also been suggested to mediate perinatal/neonatal immune activation effects on the brain [105] and, consistent with this, knockout mice are protected from neuronal pathology induced by perinatal Poly(I:C) treatment [106]. IFITM3 has also been implicated in another disorder defined by immune-related risk during neurodevelopment, namely autism [107]. Correspondingly, IFITM3 has even been proposed as a novel drug target for Scz [108]. These data only enhance the novelty of our discovery that IFITM3 is enriched in Scz patient-derived organoids and suggests that neuroinflammation may correspondingly be an intrinsic Scz phenotype during early brain development. In support of this, our data also identified cell-specific up-regulation of the interleukin-6 signal transducer IL6ST (or, GP130) specifically within Scz neurons. Given that IL6ST mediates the induction of downstream transcriptional effectors of IL-6, and was associated with growth factor binding factors in Scz neurons (Fig. 3c, d). This result was therefore also intriguing. Similar to IFITM3, there is preliminary evidence that IL6ST holds putative disease relevance to Scz. This includes elevated IL6ST expression in Scz postmortem midbrain samples [109] as well as altered expression in the dorsolateral prefrontal cortex of a mixed postmortem cohort with high neuroinflammation [110,111,112,113,114]. Interestingly, IL6ST in the prefrontal cortex may only be associated with shorter durations of illness [115]. This implicates that IL6ST may be involved in early disease induction and/or states, which is consistent with its emergence in our neurodevelopmental dataset. Cumulatively, these data provide fundamental support for the idea that inflammation may be an intrinsic component of early developmental neuropathology in Scz patient-derived organoids. Therefore, IFITM3 and IL6ST represent fruitful targets that are deserving of further study within the context of Scz and relevant neurodevelopmental hypotheses.
Lastly, an important avenue of further research will be to further map the functional qualities of various cell-types identified in cerebral organoids. For example, single-cell analysis of neuronal dynamics via calcium signaling or more elaborate single-unit electrophysiology may provide important functional data on Scz neuron activity within a 3D macroenvironment. In addition, it may be of value to further harness organoids to model the neurodevelopmental effects of PTN and BRN2 ablation—perhaps by applying gene-editing and/or interference strategies to Ctrl organoids—so to better understand the functionality of these factors specifically within healthy 3D tissue of human origin. It is also plausible that other organoid models, other cell-types, or specific patient groups may yet unveil disease effects that were not identified here. In this respect, just as we hypothesize that more mechanisms of Scz exist, we predict that more Scz phenotypes also remain to be discovered. It is therefore plausible that greater sampling may be required to identify subtle phenotypes, or that clinically stratified samples are required to identify how certain Scz cases segregate between clinical or genetic Scz subtypes. While these experiments are outside the scope of the current study, future studies should consider the utility of other single-cell technologies and develop pipelines that enable a broader range of patient samples to be functionally interrogated.
Concluding Remarks
In closing, our patient-derived organoid data conceptually validates principles behind numerous long-held hypotheses regarding the developmental basis of Scz. We experimentally establish that an ensemble of novel Scz risk factors likely amalgamate in various combinations to trigger the ontogenesis of Scz developmental neuropathology. We specifically exemplify via unbiased deep-phenotyping that organoids provide utility by enabling Scz mechanisms to be parsed in a human 3D environment that also captures the broader molecular-genetic background of disease. Our study also identifies the potential disease relevance of two novel factors, PTN and BRN2, in Scz organoids. Importantly, we establish that these factors positively regulate neuronal development in Scz patient-derived organoids via similar but putatively distinct mechanisms. While reconstitution of BRN2 was shown to only regulate neurogenesis deficits in Scz organoids (Fig. 4), PTN was determined to regulate death, differentiation, and neuron numbers within Scz patient-derived organoids (Fig. 5). This indicates that multiple mechanistic factors can contribute to both independent phenotypes and convergent (i.e., common) disease pathology. This work therefore defines novel early-arising signatures of Scz at the single-cell and posttranslational levels in 3D organoids.
When combined, our data identify that Scz neurodevelopmental alterations are putatively encoded on a cell-type-by-cell-type basis (yielding cell-specific encoding of Scz neuropathology) and that multiple mechanisms of Scz may exist within human-derived tissue. Thus, we suggest that neuropathology of Scz is likely to be substantially more complex than currently accepted, and that alterations across multiple primordial pathways may amalgamate within the early developing brain to elevate intrinsic risk of Scz.
Materials and Methods
Human induced pluripotent stem cells
Human iPSC lines were sourced from NIH deposits at the Rutgers University Cell and DNA Repository. All lines have undergone extensive characterization for identity, pluripotency, exogenous reprogramming factor expression, genetic stability and viability. A total of 25 different Induced Pluripotent Stem Cell (iPSC) lines (see Fig. S1) were utilized between organoid experiments. Importantly, each of these iPSC lines was biologically independent, with each representing a unique human donor. Specific Ctrl iPSC lines utilized for cellular experiments included MH0159019, MH0159020, MH0159021, MH0159022, MH0167170, MH0174677, and MH0174686. One Ctrl line, utilized only for computational reproducibility analysis (Fig. S1), was sourced from the Coriell Institute for Medical Research (GM23279). A comprehensive list and description of Scz patient iPSC donors and their clinical characteristics are provided in Supplementary Table 1. Sampling for cellular experiments is described in further detail within Supplementary Table 2 (Ctrl and Scz patients). All Scz samples were derived from idiopathic cases, which we define here as schizophrenia cases that maintained unknown disease origins and do not meet a genetic/syndrome-based diagnosis (as listed in NIMH notes) that would otherwise explain ontogeny of disease. Ctrl iPSC lines were screened for both personal, and family history, of major mental illnesses. All iPSC lines were maintained on Vitronectin-coated plates and fed with Essential 8 (E8) + E8 Supplement Media (ThermoFisher, CAT#: A1517001).
Three-dimensional cerebral organoid culturing system
We adapted the undirected-differentiation organoid system published by Lancaster et al. in Nature [37] and Nature Protocols [40]. While some discussion of this system was included in the manuscript, allowing the context of results to be framed by a broader audience, this culturing system can be minimized into four major stages. First, iPSCs are dissociated with Accutase (Laboratory Disposable Products, CAT#: 25-058-C1) and cultured into three-dimensional embryoid bodies for up to 7 days using previously described media (see [40]) in ultra-low attachment 96 well plates (Corning; CAT#: 3474). Rock inhibitor (1:1000; Stem Cell Tech, CAT#: 72304) and basic fibroblast growth factor (Pepro Tech, CAT#: 100-18B) are included in media for the first 2–4 days of embryoid body culturing to promote stem cell aggregation and survival. Following this, healthy embryoid bodies are isolated and transferred to Nunclon Sphera 24 well plates (Thermo Scientifiic, CAT#: 174930) for neural fate specification, using custom neural induction media (see [40]). Once neuroepithelium was apparent (see Supplementary Fig. 1), successful early “organoids” were embedded in a 30 µl Matrigel (Corning, CAT#: 354234) spheroid-droplet and polymerized at 37 °C for 20–30 min which provided a matrix for subsequent neural expansion. Organoids suspended in matrigel droplets were next cultured in terminal organoid media (see [40]) for 4–6 days without agitation, and then cultured with agitation at 60–70 RPM until harvested for experiments. All stages of culturing occurred at 37 °C with 5% atmospheric CO2 in a sterile incubator. Cerebral organoids from healthy control and schizophrenia iPSC lines were generated and maintained in parallel, ensuring that idiosyncratic differences in culturing conditions were accounted for between control and schizophrenia organoids. Last, all cultures underwent quality control assessments on a rolling basis, utilizing the published criterion and guidelines in [40] which describes numerous “Go/No Go” criteria at different stages of organoid generation. In addition, inclusion/exclusion criterion were adapted from other organoid protocols which comprised screening for evidence of neural induction including the presence of neural stem cells/progenitors (SOX2+, NESTIN+ cells), forebrain/cortical-specific progenitors (FOXG1+, PAX6+ cells), and early-developing neurons (DCX+, MAP2+ cells) including those with cortical-specific identities (CTIP2+, SATB2+, and BRN2+ cells). This ensured that all lab-generated tissue in the manuscript exhibited neural induction as well as cell-types specific for the developing cortex. Independent confirmation of neuronal induction was also achieved via unbiased analysis of our scRNA-seq and proteomics datasets.
Immunohistochemistry and laser-scanning confocal microscopy
Prior to immunohistochemistry, organoids were drop-fixed in 4% paraformaldehyde, dehydrated in 30% sucrose, embedded in Tissue-Tek OCT compound (CAT#: 4583) using biopsy molds and cryosectioned serially between-slides at 30 µm (~25 slides per organoid). Each slide therefore contained 3–4 unique sections/Fields of View (FOV) from each organoid studied. This allowed for robust assessment of both independent and focal cell populations in each biological and technical organoid replicate. All sections underwent heat-mediated antigen retrieval in citrate buffer, and incubated in primary overnight. Primary antibodies comprised SOX2 (1:1000; R&D Systems, CAT#: MAB2018-SP), PAX6 (1:1000; Biolegend, CAT#: 901301), β-tubulin III (1:1000; Abcam, CAT#: AB41489), MAP2 (1:1000, Abcam, CAT#: AB11267; 1:1000, Abcam, CAT#: AB32454), BrdU (1:1000, BD Pharminogen, CAT#: 555627), DCX (1:1000, Santa Cruz, sc-271390), Activated/Cleaved Caspase-3 (1:1000; Cell Signaling Biology, CAT#: 9661S and Thermo Fisher Scientific, CAT#: 66470-2-IG), Nestin (1:1000, Abcam, CAT#: AB176571), pH3 (1:1000; Millipore, CAT#: 06-570), Ki67 (1:1000; BD Biosciences, CAT#: 550609), TBR2 (1:300; Abcam, CAT#: AB23345 and EMD Millipore, CAT#: AB15894), GFP (1:1000, Thermofisher, CAT#: A10262), CTIP2 (1:300; Abcam, CAT#: AB18465), and BRN2 (1:750, Santa Cruz, CAT#: SC-393324). Secondary antibodies were incubated for 2 h at room temperature, and comprised antibodies for rabbit (Fluor 488 CAT#: A11008; Fluor 546 CAT#: A11035; & Fluor 633 CAT#: A21070), mouse (Fluor 488 CAT#: A11001; Fluor 546 CAT#: A11003; & Fluor 633 CAT#: A21052) and chicken (Fluor 546 CAT#: A11040) were used at a 1:2000 dilution, and sourced from Life Technologies. Microscopy was completed on an Olympus IX81 Laser-Scanning Confocal Microscope, controlled by proprietary Olympus FluoView software. Images were typically acquired at 1200 x 1200 resolution with optical Z slices (step sizes) ranging from 0.5 to 10 µm depending on the unit of analysis.
BrdU pulse-chase assay for mapping cell fate
Neuronal differentiation experiments comprised a 24 h pulse of BrdU and a 7 d chase period [116]. Organoids were pulsed with 10 µM BrdU in media that was aspirated 24 h later. Organoids were washed three-times with differentiation media and left to maturate. Approximately 7 d following BrdU pulse, organoids were drop-fixed, cryosectioned, and immunostained to examine progenitor self-renewal and neuronal differentiation (Fig. 1).
High-throughput flow cytometry of apoptosis & DNA damage in organoids
To derive an unbiased assessment of DNA damage, cell death, and DNA-damaged cells undergoing apoptosis following drug treatment, we adapted a well validated and widely utilized FACS kit (BD Pharmingen, CAT#: 562253). Briefly, pseudorandomly selected organoids were dissociated to a single-cell suspension via a 20 min exposure to accutase followed by tricheration and serial filtering through 70→30 μm pores. Cells were resuspended and incubated in in Cytofix/Cytoperm solution for fixation and initial permeabilization for 30 min at room temperature. Cells were subsequently washed, resuspended in BD “Plus” permeabilization buffer for 10 min on ice, and re-exposed to Cytofix/Cytoperm solution for 5 additional min to achieve refixation. Cells were washed and resuspended in 30 μg of DNAse for 60 min at 37 °C. Cells were washed and labeled with PE-Cleaved PARP (BD Pharmingen, CAT#: 51-9007684) to label cells committed to apoptosis and Alexa647-H2AX (pS139, BD Pharmingen, CAT#: 51-9007683) for cells exhibiting DNA damage. Double positive cells represented apoptotic cells exhibiting DNA damage. Per manufacturer instructions, antibodies were diluted at a 1:25 ratio and incubated for 20-minutes at room temperature. Cells were washed and resuspended in staining solution. Labeled suspensions were analyzed utilizing a BD Aria II (Becton Dickinson) cell sorter to acquire multiparameter data files. Data were presented as a % of H2AX+ DNA damaged cells, and % of PARP+ H2AX+ double-positive cells that exhibited both DNA damage and induction of cell death.
Single-cell DNA content analysis
Organoids were prepared to a single-cell suspension as described above, and washed successively with calcium/magnesium free PBS at 4 °C to remove residual peptides in solution. Samples were centrifuged, supernatant removed, and pelleted cells resuspended in PBS. Cells were EtOH fixed (100%, at 4 °C) while being gently vortexed. Cells were rehydrated, and incubated with Triton-X with DNAse added for 5 min. Cells were pelleted, Triton-X removed, and resuspended in 200 μl of calcium/magnesium free PBS at 4 °C. Immediately prior to flow cytometry, suspensions were incubated with 2 μl of Propidium Iodide (PI; Thermofisher, Material#: P3566), and analyzed for single-cell DNA content utilizing a BD Aria II (Becton Dickinson) cytometer. Analysis was subsequently modeled post hoc in the FloJo cytometry analysis package (Becton Dickinson).
Tandem mass tag (TMT) liquid chromatography-mass spectrometry (LC/MS)
TMT mass-spectrometry proteomics was completed as previously described [117]. Briefly, organoids were reduced with dithiotreitol and underwent alkylation with iodoacetamide before tryptic digestion at 37 °C overnight. Peptide suspensions were desalted using C18 stage-tips prior to Liquid Chromatography-Mass Spectometry (LC-MS) analysis. An EASY-nLC 1200, which was coupled to a Fusion Lumos mass spectrometer, (ThermoFisher Scientific) was utilized. Buffer A (0.1% FA in water) and buffer B (0.1% FA in 80% ACN) were used as mobile phases for gradient separation [117]. A 75 µm I.D. column (ReproSil-Pur C18-AQ, 3 µm, Dr. Maisch GmbH, German) was packed in-house for separating peptides. A separation gradient of 5–10% buffer B over 1 min, 10–35% buffer B over 229 min, and 35–100% B over 5 min at a flow rate of 300 nL/min was adapted. Data dependent mode was selected during operation of the Fusion Lumos mass spectrometer. An Orbitrap mass analyzer acquired Full MS scans over a range of 350–1500 m/z with resolution 120,000 at m/z 200. The top 20 most-abundant precursors were selected with an isolation window of 0.7 Thomsons and fragmented by higher-energy collisional dissociation with normalized collision energy of 40. The Orbitrap mass analyzer was also used to acquire MS/MS scans. The automatic gain control target value was 1e6 for full scans and 5e4 for MS/MS scans, respectively, and the maximum ion injection time was 54 ms for both.
Bioinformatics pipeline for TMT-LC/MS proteomics
Mass spectra were pre-processed as described [118] and processed using MaxQuant [119] (1.5.5.1). Spectra were searched against the full set of human protein sequences annotated in UniProt (sequence database Sep-2017) using Andromeda. Data was searched as described [120] with fixed modification, cysteine carbamidomethylation and variable modifications, N-acetylation and methionine oxidation. Peptides shorter than seven amino acids were not considered for further analysis because of lack of uniqueness, and a 1% False-Discovery Rate (FDR) was used to filter poor identifications at both the peptide and protein level. Protein identification required at least one unique or razor peptide per protein group. Contaminants, and reverse identification were excluded from further data analysis. Resulting p values were adjusted by the Benjamini-Hochberg multi-test adjustment method for a high number of comparisons [121] and statistics performed as previously described [122]. The proteome profiles from the analyses of two biological replicates and individual technical replicates were combined by calculating the average intensity. Proteins that were quantified in only one replicate were also included in the combined data set. For further data analysis, the normalized intensities were converted into log2 ratios of the intensities over the median intensity measured for each protein across each sample group.
For enrichment and pathway analyses, Kyoto Encyclopedia of Genes and Genomes (KEGG) and NIH Database for Annotation, Visualization and Integrated Discovery Bioinformatics Resources 6.7 (DAVID) platforms were utilized using recommended analytical parameters [123]. For gene ontology (GO) enrichment and network analyses UniProt (www.uniprot.org, [124]) database resource (biological process, molecular function), Ingenuity Pathway Analysis, and Reactome knowledgebase were utilized. Clustering of sample groups was performed by principal component analysis (PCA) and visualized using ggplot2 [125] and ggfortify (https://cran.r-project.org/web/packages/ggfortify/index.html; [126]). Protein abundance distribution for global and subset groups was performed using gplots (https://cran.r-project.org/web/packages/gplots/index.html; [127]). Based on hypergeometric distribution, the GO terms and pathways that differentially expressed proteins are significantly enriched-in were calculated. Benjamini-Hochberg method was used to correct obtained p values. A corrected p ≤ 0.05 was considered to represent significant enrichment. Protein–protein associations were evaluated for differentially expressed protein subsets using STRING database. Correlation pairs were ordered, and redundancies were removed before comparison to a non-redundant version of the STRING database to find STRING-annotated interactions. Only STRING interactions of high confidence (score ≥ 0.700) were considered for proteome-target analyses. Unbiased computational analysis of proteomics data utilized correction methods such as FDR rates and p value adjustment using the Benjamini-Hochberg method were adapted, as described above, and Statistical testing of was performed using a Poisson distribution with EdgeR software v3.2.
10x ChromiumTM microfluidic device single-cell RNA-sequencing
Single-cell sequencing was conducted as described in-text, figure legends, and depicted in our schematic pipeline (see Fig. 2f). Briefly Organoids were dissociated using Accutase, serially filtered to remove debris, and were subjected to high-throughput FACS (Aria II flow cytometer, Becton Dickson). This procedure allowed us to isolate only live cells in a defined concentration (2000 live cells/ µL) that could be standardized between lines for microfluidic-device loading. Cell viability was confirmed using Countess-II (Invitrogen, Thermofisher, CAT#: AMQAX1000). Next, cells were prepared for 10X Genomics Chromium library preparation according to manufacturer instructions (see ChromiumTM Single-Cell 3’ Library and Gel Beads and ChromiumTM CHIP kit, 10x Genomics). Post sample generation, barcoded-emulsions were broken, amplified, and libraries prepared. cDNA was examined on a Fragment Analyzer running PROSize v3.0 3.0.1.6 (Advanced Analytical Technologies). Libraries were subsequently subjected to next generation sequencing via Next-Seq High-Output 150-cycled 26-8-98.
Bioinformatics pipeline for single-cell RNA sequencing
Initial processing of raw reads involved alignment to GRCh38 with the CellRanger v3.0.2 pipeline (10x Genomics, USA). Subsequent analyses were performed in R and Bioconductor (https://osca.bioconductor.org/) per guidelines [128]. This comprised numerous functions in the scater and scran packages [129]. Cells with fewer than 317 genes and >8% mitochondrial reads were removed based on outlier calculations. Subsequent processing and integration of samples was completed using Seurat v3.1 following vignette recommendations. More specifically, read counts were first individually normalized using SCTransform for each sample [130]. The different samples were then integrated using the top 3000 most informative genes [131] before performing various dimensionality reduction steps including principal components analysis (PCA) and UMAPs [132]. Batch correction was also applied. A shared nearest neighbor graph was constructed with default settings (e.g., k = 20). This comprised the first 25 principal components. Subsequent clustering was performed with the resolution parameter set to 0.2. For visualizations and assessments of normalized expression values, SCTransform-normalized (log-transformed) expression values were principally adapted. Cell-type clusters were labeled based on marker enrichment, derived from both Seurat-identified clusters (using default parameters) as well as automated assignment with SingleR using reference datasets [133]. Seurat analysis comprised Find Markers and Find All Markers functions were used with default settings as well as scran::Find Markers(), comparing only cells of the control condition. For SingleR, we used its in-built reference data set of the human primary cell atlas, which contains RNA-seq from adult human tissues, including neurons and myeloid cells. In addition, we downloaded the single-cell RNA-seq data from numerous human fetal brain samples [79] and used it as the training data with the refactored bioconductor version of SingleR (http://www.bioconductor.org/packages/devel/bioc/html/SingleR.html).
After integration, we determined differential gene-expression using a pseudo-bulk approach [134] that summed the reads across all cells belonging to the same type of cells (where “type” would be determined by the sample and the membership within a given subpopulation of interest). To identify genes with significantly different expression (DEG) levels between two types of cells, we used methods implemented in the edgeR package including dispersion estimation and gene-wise negative binomial generalized linear models with quasi-likelihood tests [135]. Unless stated otherwise, DEG were based on adjusted p values lower than 0.01. To test for over-representation of specific gene sets of KEGG, Reactome, and Gene Ontology collections in our DEG lists, we used the enrichment functions implemented in clusterProfiler and reactomePA [136] with an adjusted p-value cut-off of 0.05. Note, for STRING protein–protein interactome modeling of scRNA-Seq pathway factors (specifically, Fig. 3d), specific analysis parameters were applied. Namely, kmeans clustering (n = 3) was applied, network edges were limited to molecular action, a minimum interaction confidence limit of 0.4 was adapted, and no more than 5 interactors in the first shell were allowed. Code used for scRNA-Seq analysis is available on github, and the dataset will be available via repository curation following publication of this manuscript.
Diffusion maps and pseudotime trajectories of single-cell transcriptomes
For ordering the cells along pseudotime trajectories, we first constructed diffusion maps [137] that are implemented in the destiny package [80]. Cell lineages and temporally expressed genes were inferred using slingshot [138] following recommendations in vignettes and technical materials. In brief, pseudotime values were extracted for each cell along each lineage identified by slingshot. Then, each gene’s normalized expression values were regressed on the pseudotime variable using a general additive model to identify those whose expression patterns most closely correlate with the pseudotime weights. This allowed profiles of cellular differentiation to be computationally constructed in an unbiased environment based on large-scale single-cell sequencing data.
Technical details of BRN2 and PTN rescue experiments
For BRN2 mechanistic rescue experiments, virus was administered during neural induction when 3D embryoid bodies remained at their lowest cellular densities. As described in-text, CTRL-Virus organoids were administered a GFP virus as a vehicle while BRN2-Virus organoids received a self-regulating BRN2-GFP viral vector (vector details, including complete viral schematic, are provided in Fig. S10). As described in-text, this hPGK>BRN2:P2A:EGFP.MIRT1244 lentiviral vector was a GFP-modified version of a previously validated neuronal conversion tool [112]. Expression of the neuronal mRNA, miRNA-124, to four recognition units in virus transcripts (MIRT.1244) leads to translational suppression in neurons but not other cell-types [112]. Specifically, Expression of miRNA-124 represses SOX9 to direct progenitors towards a post-mitotic neuronal fate [139] where miRNA-124 expression is preferentially maintained [140] and reaches its peak [141]. This high intracellular expression of miRNA-124 in neurons suppresses translation of BRN2-Virus, leading to complete loss of exogenous BRN2-GFP in mature post-mitotic neurons only. Organoids were infected under uniform conditions irrespective of line, preparation, or group allocation. Virus and polybyrene was supplemented into neural induction media for 24 h. Organoid generation then continued as described without further modification. For PTN mechanistic rescue experiments, organoids were also generated as described excepting the addition of 25 ng/mL recombinant human PTN (Peprotech, CAT#: 450-15) into differentiation media for 7 d. This concentration was derived as it is similar to concentrations of morphogens used in other organoid studies, and this yielded viable 3D tissue without evidence of deterioration. Organoids allocated to the vehicle-treatment group received culture-grade diluent without PTN. For pulse-chase experiments in PTN-supplemented organoids, BrdU administration coincided with first exposure to PTN. Organoids were pseudorandomly selected to treatment groups for both mechanistic rescue experiments.
Design and analysis
Statistical analysis and graphing was completed in Graphpad Prism v6.0. All data is presented as Mean ± Standard Error of the Mean (SEM). As most comparisons comprised only two groups, t tests were the predominant hypothesis-test utilized fpr cellular assays comprising only two groups. However, for rescue experiments, two-way ANOVAs were our primary analysis tool so that all four groups could be appropriately analyzed and compared (as well as Group x Treatment interactions). Cohen’s d was correspondingly adapted for effect size estimation where of interest, and assumptions screened. Significance was set at p < 0.05 per Fisher’s tables, tailed according to statistical-directionality guidelines and corrected for multiple-comparisons. To temper variability, a high-content approach was adapted. Specifically, per sampling theory, we generated, observed, and analyzed as many units of analysis as possible. Thus, all experiments comprised multiple field, organoid, and human biologic replicates. For multi-cohort replication, samples that were continuously generated for baseline analyses/core phenotype analysis were pooled from across multiple batches, cohorts, and experiments (where possible) to increase data-point capture and maximize power between experiments. To ensure appropriateness, we conducted multiple types of statistical screening to ensure phenotype compliance including a thorough analysis of baseline reproducibility and quality control measures/markers (as previously described in our “Methods”). Consistent with this, and to promote phenotype representativeness and reproducibility whilst controlling for idiosyncratic differences that may emerge from individual batches, organoids were typically sampled from between 2 and 6 independent preparations per line that were subsequently pooled. This ensured that organoid quantifications were subjected to high-content sampling to temper human sources of technical (e.g., batch effects) and protocol-derived (e.g., idiosyncrasies) statistical nuisance variance. Indeed, this approach yielded suitable statistical evidence of reproducibility as coefficients of variance between batches were shown to be highly consistent. In addition, all lines utilized in our rescue studies were pseudorandomly selected for cross-sectional sampling and were not selected based on severity of phenotype or any other qualifying factor. Across immunohistochemistry experiments, up to 12 unique fields from up to 10 cerebral organoid replicates per line were sampled. This included analysis in up to 21 iPSC lines (see Fig. 1) for our core cellular phenotyping experiments. Typically, sampling comprised 2–5 unique observations (VZs or cortical fields) per organoid, and 3–5 organoids were typically sampled per iPSC line. This yielded total sample sizes that often comprised hundreds of observations in sum. Individual group numbers used for sampling have been provided throughout the manuscript for clarity. Across all experiments no iPSC lines were explicitly/specifically excluded from an analysis. Rather, experiments were conducted in accordance with the production and survival of organoid batches, the relative availability of sections for experiments, as well as indicators of observed power. This cross-sectional sampling approach is consistent with effect sizes and power analyses as well as phenotype replication throughout the manuscript. Cellular quantifications were typically conducted in 5000 µm2 Regions of Interest (ROI). VZs themselves were defined as progenitor-enriched (SOX2+, PAX6+, NESTIN+) structures that exhibited morphological evidence of a ventricle as well as pseudostratification of neuroepithelium. All cellular analyses were normalized to total levels of the primary cell-type of interest within ROIs (e.g., progenitor death was normalized to quantified progenitor numbers within the same ROI field). Computational analyses were completed, and corrected for false discovery rates, as described above.
Data availability
Proteomics and transcriptomics data used to support the findings of this study have, or will be, deposited in repositories but will be embargoed pending further follow-up analysis/study. However, select –omics data may be accessible following paper publication per reasonable request. Code used for transcriptomics data analysis will also be made available by request, but is broadly accessible via Github (https://github.com/abcwcm/Notaras_MolPsy). See also GEO submission GSE184878. Other -omics data may be accessible following paper publication, contingent on the completion of follow-up studies that are also harnessing our multimodal datasets.
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Acknowledgements
MN was the recipient of a NHMRC CJ Martin Fellowship which supported stem cell training completed at Weill Cornell Medical College of Cornell University.
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MN and DC conceived the project and designed experiments. MN conducted all experiments, analyzed data, and wrote the paper. AL provided important logistical support by assisting with numerous experiments and processing tissue, and NS assisted with early experiments as part of a PhD rotation. PC assisted with wet-lab processing of single-cell sequencing experiments under supervision of HT, and FD completed single-cell analysis with biological-driven input from MN. Last, DG completed all LC/MS computational analysis presented in the paper.
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Notaras, M., Lodhi, A., Dündar, F. et al. Schizophrenia is defined by cell-specific neuropathology and multiple neurodevelopmental mechanisms in patient-derived cerebral organoids. Mol Psychiatry 27, 1416–1434 (2022). https://doi.org/10.1038/s41380-021-01316-6
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DOI: https://doi.org/10.1038/s41380-021-01316-6