Abstract
Externalizing disorders (ED) are a cause of concern for public health, and their high heritability makes genetic risk factors a priority for research. Adhesion G-Protein-Coupled Receptor L3 (ADGRL3) is strongly linked to several EDs, and loss-of-function models have shown the impacts of this gene on several core ED-related behaviors. For example, adgrl3.1−/− zebrafish show high levels of hyperactivity. However, our understanding of the mechanisms by which this gene influences behavior is incomplete. Here we characterized, for the first time, externalizing behavioral phenotypes of adgrl3.1−/− zebrafish and found them to be highly impulsive, show risk-taking in a novel environment, have attentional deficits, and show high levels of hyperactivity. All of these phenotypes were rescued by atomoxetine, demonstrating noradrenergic mediation of the externalizing effects of adgrl3.1. Transcriptomic analyses of the brains of adgrl3.1−/− vs. wild-type fish revealed several differentially expressed genes and enriched gene clusters that were independent of noradrenergic manipulation. This suggests new putative functional pathways underlying ED-related behaviors, and potential targets for the treatment of ED.
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Introduction
The global public health and economic burden associated with untreated or unaddressed externalizing behaviors (alcohol and substance misuse, violence, and aggression, oppositional or disruptive behavior) are significant. Externalizing disorders (ED), such as attention-deficit/hyperactivity disorder (ADHD), conduct disorder, oppositional defiant disorder, or substance use disorder, are common among young people: ADHD ~ 4% [1]; substance use disorders ~4%; conduct disorders ~3% [1]. ED is characterized by several transdiagnostic phenotypes, including inattention, hyperactivity, and poor impulse control [2,3,4]. As well as disrupting development and education, ED are associated with a range of debilitating comorbidities (bipolar disorder [5], depression [6, 7], anxiety [8,9,10], substance misuse [11, 12], and sleep disorders [13]).
The high degree of heritability of ED (~80% [14]) has motivated the search for candidate genes. Recent linkage studies have identified several variants in the adhesion G-protein-coupled receptor L3 (ADGRL3) gene that increase susceptibility to, and severity of, several EDs. For example, ADGRL3 is linked to an increased risk of ADHD diagnosis and its clinical manifestation and affects the efficacy of psychostimulant treatments [15]. ADGRL3 variants are also linked to substance use disorders [12]. Several ADGRL3 variants are associated with the clinical progression of ADHD and may have a similar impact on other externalizing behaviors. For example, ADGRL3 variants cause a 6-fold increase in risk for ADHD [16], increase the persistence of combined-type ADHD into adulthood [17], increase impulse-control problems in ADHD patients [18], and increase symptom severity in ADHD patients [19,20,21]. Despite being strongly associated with ADHD and several other impulse-control disorders (e.g., substance abuse) [12, 15] the underlying mechanisms by which ADGRL3 affects externalizing behavioral phenotypes are not well characterized. Our aim in this study was to perform a behavioral and molecular characterization of adgrl3.1 to understand its role in promoting or mediating externalizing behaviors.
ADGRL3 codes for a G-protein-coupled receptor involved in cell-adhesion, signal transduction, and synaptic signaling, and two main ligands are involved in its function: FLRT3 and teneurin [19, 22, 23]. It is widely expressed throughout the brain, including the prefrontal cortex (PFC), caudate nucleus, amygdala, and cerebellum, and across a diverse range of central nervous system (CNS) structures and nuclei including the cerebrum (frontal and temporal lobes, occipital pole), limbic system (hippocampus) and striatum (putamen) [22]. ADGRL3 is conserved across a range of taxa [24,25,26], and knocking out or knocking down this gene causes a range of ED-relevant symptoms. For example, Adgrl3−/− rats and mice, and both adgrl3.1 antisense morpholino oligonucleotide (MO) knock-down and adgrl3.1−/− knock-out zebrafish larvae, display persistent hyperactivity [24, 27], which is rescued by both stimulant and non-stimulant ADHD treatments (e.g., the dopamine (DAT) reuptake inhibitor methylphenidate [28] and the noradrenaline (NET) reuptake inhibitor atomoxetine [24, 28, 29]).
As well as hyperactivity, Adgrl3−/− mice display decreased inhibitory control [26]. Inhibitory control is a multifaceted process that includes the inhibition of prepotent responses, intolerance of delay, and preference for small-immediate vs. large-delayed rewards [3]. Despite being dissociated from one another both clinically and neurologically, and impulse-control-subtypes rarely inter-correlating at the interindividual level [30], deficits in all impulse-control subtypes are reversed by the selective noradrenergic reuptake inhibitor atomoxetine, suggesting a general mechanistic role for noradrenaline in this process [31]. In addition, extensive previous research has demonstrated that atomoxetine significantly reduces impulse-control deficits in rodents [31], humans [32], and zebrafish [33]. In terms of hyperactivity, we recently carried out a screen of adgrl3.1−/− zebrafish larvae and found several drugs that rescue hyperactivity, including aceclofenac, amlodipine, doxazosin, and moxonidine [29]. Although the molecular mechanisms of action by which this gene impacts externalizing behaviors is not clear, collectively, these data suggest that ADGRL3 is functionally involved with two core externalizing symptoms (hyperactivity and reduced impulse control) representing an ideal tool for identifying targets for the development of novel therapeutics.
In order to understand the contribution of adgrl3.1 to externalizing symptoms such as poor impulse control, risk-taking, inattention, and hyperactivity, we characterized these behavioral phenotypes in adgrl3.1−/− zebrafish, and examined the effects on these phenotypes of atomoxetine (a drug that is commonly used as a treatment for externalizing disorders). We found that adgrl3.1−/− shows marked deficits in impulse control and attention and increased risk-taking and hyperactivity, all of which are rescued by atomoxetine. We then carried out an in-depth examination of the brain transcriptome of adgrl3.1−/− compared to wild-type controls, to characterize alterations in gene networks and biological pathways. In addition, we examined immediate changes in gene expression that occur when adgrl3.1−/− is treated with atomoxetine. We identified several differentially expressed genes (DEGs) between WT and adgrl3.1−/−, and several enriched gene clusters, offering insights into the mechanism by which ADGRL3 may mediate externalizing behaviors and suggesting potential targets for treatment.
Materials and methods
Generation of adglr3.1 −/− fish
The fish used in this study were homozygous adgrl3.1 mutant zebrafish (adgrl3.1−/−) created by CRISPR-Cas9 genome engineering, as previously described [29], and age-matched adgrl3.1+/+ controls. Adult fish (~50:50% male: female) was housed in an aquarium facility at the University of Portsmouth (UK), and kept on a 14:10 light: dark cycle (~28 °C, pH ~8). adgrl3.1−/− and controls (wild-type AB strain) were simultaneously in-crossed (pair breeding) and grown on a recirculating rack (Aquaneering, USA) to 4 months post-fertilization before testing. All housing tanks contained enrichment substrates from 10-days post-fertilization and throughout (gravel pictures under the tanks). Offspring from adgrl3.1−/− and wild-type controls were randomly selected from ~5–10 groups of 20, with equal numbers of males and females in each experimental group (detailed below). All work was carried out following scrutiny from the University of Portsmouth Animal Welfare and Ethical Review Body (AWERB), and under license from the UK Home Office (PPL P9D87106F).
Drug treatment
adgrl3.1−/− fish were individually treated with 0.5 mg/L atomoxetine (TCI UK Ltd., Oxford, UK) for 30 min prior to behavioral recording. The concentration used was based on extensive previous research from our group and others [33]. The drug was dissolved in aquarium-treated water and animals were individually treated in 300 mL beakers. For the 5-CSRTT, atomoxetine treatment followed the establishment of steady-state responses in the final phase of the 5-CSRTT.
RNA sequencing analysis
Fish were euthanized by rapid cooling (immersion in 2 °C water) and the whole brain tissue was removed, snap-frozen in liquid nitrogen, and kept at −80 °C until further use. RNA extraction was performed using the GeneJET RNA Purification Kit (Thermo Scientific) as described in the manufacturer’s instructions. Next, RNA concentration was determined using the Bioanalyzer 2100 (Agilent Technologies) using an RNA 6000 Nano kit. RNA quality was evaluated using the NanoDrop ND-1000 spectrophotometer (Thermo Scientific) and the Bioanalyzer 2100 (Agilent Technologies). A260/A280 and A230/A260 ratios greater than 1.8 and an RIN greater than 8 were considered acceptable. RNA samples were stored at −80 °C. RNA sequencing (RNA-seq) was performed by BGI Tech Solutions (Copenhagen, Denmark) using non-stranded library preparation with mRNA enrichment (oligo(dT) magnetic beads), paired-end sequencing with 100 bp read length on the DNBSEQ platform.
Bioinformatics
The paired-end raw sequence data had a total number of 7.99 E + 08 reads (mean 6.66E + 07 stdev 1.30E + 07) and were quality-controlled using FastQC (Galaxy Version 0.11.9). On average 78.2% (stdev 0.66%) of the reads could be uniquely mapped to the zebrafish reference genome GRCz11 using the RNAStar aligner (Galaxy Version 2.7.8a) [34]. The final transcript count data was generated using the HTSeq framework (Galaxy Version 0.9.1) for high throughput sequencing data [35] based on Ensemble release 99 gene annotation using standard settings. All analysis was conducted on a private Galaxy instance running on the MedBioNode cluster at the Medical University of Graz. Further downstream analysis was conducted using R version 4.0.3 within the free RStudio Desktop version. Differential gene expression analysis was performed with DESeq2 package version 1.30.1 [36] on the count table as output from the HTSeq framework. DAVID Bioinformatics Resources 2021 [37] was used for pathway enrichment analysis by clustering DEGs and associated biological annotation terms into functional groups. The enrichment score cutoff in DAVID was set to 1.3, which corresponds to a corrected p-value of 0.05.
Behavioral screening
Impulsivity
The 5-CSRTT is a continuous performance test [38] that has been extensively validated to measure impulsivity in zebrafish [33, 39]. Briefly, the fish (n = 9–10) is trained to respond regularly to a light stimulus in one of five spatially distinct locations on the rear wall of the test tank in order to gain a food reward (delivered at the front wall of the tank) in a purpose-built testing arena (Zantiks AD, Cambridge, UK). Impulsivity is ascertained by examining the animal’s ability to withhold its response to the forthcoming light stimulus during a defined pre-stimulus interval (a variable-interval of 5-s). In zebrafish, the test has been pharmacologically validated using atomoxetine, which reliably reduces impulsivity while not affecting other test parameters [33, 39, 40]. The pre-training and test phases are described in detail in the Supplementary Material.
Risk-taking behavior
Novel object test
Increased risk-taking behavior is common in ADHD patients [41], and can be assessed in zebrafish using the novel object test [42, 43]. This test assesses boldness by measuring the fish’s approach, in a new environment, towards a new object in that could be perceived as a potential threat, reflecting their willingness to take risks. We measured the time that zebrafish (n = 12–14 per group) spent close (within 2 cm) to a novel object (15 cm long black tube) in a novel tank (dimensions: 36 cm length × 27 cm height × 10 cm water column depth). Fish were recorded for 6 min and behavioral response was analyzed using automated video-tracking software (EthoVision, Noldus Information Technology Inc., Leesburg, VA—USA).
Hyperactivity
The open-field test is commonly used for measuring locomotion and exploratory activity in adult zebrafish [44, 45]. Adult zebrafish (~4 months post-fertilization; n = 35 habituation and n = 17 testings) were placed individually in a tank (20 cm length × 15 cm width, 10 cm water column depth) and filmed during 30-min exposure to an open field environment each day for 3 days. After 3 days of habituation, both adgrl3.1−/− and wild-type fish were placed individually in a beaker (300 mL) in home tank water or in a solution containing atomoxetine (adgrl3.1−/− only; 0.5 mg/L) for 30 min before being transferred to the open field test. All behaviors were analyzed using automated video-tracking software (ANY-maze ©—Stoelting Co., USA). The tank was separated into two virtual areas (central and peripheral area, 2 cm close to the wall) to provide a detailed evaluation of the exploratory activity. The following endpoints were measured: distance traveled (m), and immobility (s). Water was changed between each individual to minimize data variability [46].
Results
adgrl3.1 −/− increases externalizing behaviors by altering noradrenergic signaling
Genetic variation in Adgrl3 is associated with deficits in impulse control in rodents [26] and ADGRL3 polymorphisms (GWAS) have been linked to externalizing, impulsivity-related disorders in humans [12, 15]. We first investigated whether loss of adgrl3.1 similarly reduced impulse control in adult zebrafish by using the 5-CSRTT (Fig. 1A) [33, 39]. There was no difference in acquisition rates, nor any overall difference between WT and adgrl3.1−/− in the number of correct responses (Fig. 1B) during the pre-training stages of the 5-CSRTT. However, in the 5-CSRTT itself, compared to WT siblings, adgrl3.1−/− zebrafish displayed a significantly lower proportion of correct responses (Fig. 1C) reflecting inattention, and a greater number of anticipatory responses (Fig. 1D) reflecting impulsivity. There were a similar number of omissions in WT and adgrl3.1−/− (Fig. 1E) meaning that both genotypes completed the test the same number of times. The decreased attention and heightened impulsivity were more prominent in male adgrl3.1−/− zebrafish compared to females (Supplementary Fig. 1A). Treatment with atomoxetine partially reversed the attentional deficits and fully reversed the impulsivity in adgrl3.1−/− (Fig. 1C, D) suggesting that this gene modulates inattention (to a small degree) and impulsivity, predominantly via noradrenergic signaling.
Children with ADHD and externalizing personality dimensions also display heightened levels of boldness in novel situations. This is strongly related to disruptive behaviors and conduct-related problems [47]. This behavior could be characterized as ‘high approach’ to unfamiliar situations and represents a further facet of the ‘uncontrolled’ or impulsive phenotype [48]. For this reason, we next examined fish boldness in terms of their approach to a novel object [42, 43]. adgrl3.1−/− zebrafish spent more time close to the object (Fig. 1F), suggesting an increase in boldness. This increase was fully rescued by atomoxetine (Fig. 1F). There was no influence of sex effect on boldness in the novel object test (Supplementary Fig. 1B).
In summary, mutation of adgrl3.1 made adult zebrafish significantly inattentive, impulsive, and bolder, with a stronger effect in male animals for impulsivity (5-CSRTT) but not for boldness.
adgrl3.1 −/− zebrafish show noradrenaline-mediated hyperactivity after habituation to a novel environment
Previous studies with adgrl3.1−/− have focussed on single measures of hyperactivity as the endpoint [27, 28]. Here, we investigated the effect of loss of adgrl3.1 function on motor activity over several test phases. Hyperactivity develops over time in children with ADHD (e.g., ref. [49]). Similar patterns have been observed in Adgrl3 knock-out rats [50] as well as in spontaneously hyperactive rats [SHR] [51], suggesting a strongly conserved mechanism. Therefore, prior to assessing hyperactivity, we first habituated the fish to their recording environment and analyzed changes in their behavior. As predicted, we did not observe any differences in hyperactivity between WT and adgrl3.1−/− on the first three days of recording (Fig. 2A). However, adgrl3.1−/− showed a complex response pattern, spending significantly more time immobile than WT on day 1, an effect that reduced considerably on days 2 and 3 (Fig. 2A). This was consistent with the hypothesis that adgrl3.1−/− were experiencing higher anxiety on the first day [52]. On recording day 4, we found that adgrl3.1−/− was hyperactive compared to WT, swimming significantly further during the 5 min recording period. This phenotype was rescued by atomoxetine treatment, again suggesting a noradrenergic basis (Fig. 2B, C). There was no difference in immobility between the genotypes at this time point (Fig. 2C). A sex effect was also observed for the distance traveled: male adgrl3.1−/− showed the highest distance traveled and appeared to be driving the significant group differences (Supplementary Fig. 1C).
Genome-wide effects of adgrl3.1 knockout identify novel functional pathways for the treatment of ED
Transcriptomic differences between the brains of adgrl3.1−/− and wild-type zebrafish
We next investigated transcriptomic differences between wild-type, adgrl3.1−/− and adgrl3.1−/− + ATO fish immersed acutely (20 min) in atomoxetine (adgrl3.1−/− + ATO; Fig. 3). Because atomoxetine rescued all the observed phenotypes, we used acute treatment with atomoxetine to identify the rapid effects of pharmacological alteration of noradrenergic signaling upon gene expression in adgrl3.1−/−. Principal component analysis (PCA) showed a clear separation between wild-type and adgrl3.1−/− (with and without ATO treatment) along PC1 of the plot explaining 54% of the total variance (Fig. 3A). In contrast, acute immersion in ATO did not lead to a large change in the transcriptome, with adgrl3.1−/− and adgrl3.1−/− + ATO clustering close together in the PCA plot. Differential expression analysis found a total of 869 differentially expressed genes between WT and adgrl3.1−/− and 896 differentially expressed genes between WT and adgrl3.1−/− + ATO (Fig. 3B). Only 34 genes were differentially expressed between adgrl3.1−/− and adgrl3.1−/− + ATO (Fig. 3B). Hierarchical clustering of the samples based on these differentially expressed genes showed consistent up- or downregulation of genes in all samples of a given group between WT and adgrl3.1−/− (Fig. 3C) and WT and adgrl3.1−/− + ATO (Fig. 3E). However, the few genes differing between adgrl3.1−/− and adgrl3.1−/− + ATO (Fig. 3G) showed considerable variation within the groups. We used volcano plots to highlight the most significant differentially expressed genes in each group. When comparing WT to adgrl3.1−/− we found heightened expression of genes including atp6v1b2 (ATPase H+ transporting V1 subunit B2), birc6 (baculoviral IAP repeat containing 6), and moesin a (membrane-organizing extension spike protein a); and decreased expression of dusp6 (dual-specificity phosphatase 6), irs2a (insulin receptor substrate 2a), shisha4 (shisa family member 4), bean1 (brain expressed, associated with NEDD4, 1) and shisha7a (shisa family member 7a) (Fig. 3D). A comparison of WT and adgrl3.1−/− + ATO revealed increased expression of the same genes as WT vs. adgrl3.1−/−, as well as nono (non-POU domain containing, octamer-binding). The same genes showed decreased expression when comparing WT vs. adgrl3.1−/− + ATO and WT vs. adgrl3.1−/− (Fig. 3F). Finally, when directly comparing adgrl3.1−/− to adgrl3.1−/− + ATO we saw a significant increase in fosa (v-fos FBJ murine osteosarcoma viral oncogene homolog a), fosb (v-fos FBJ murine osteosarcoma viral oncogene homolog b), socs3a (suppressor of cytokine signaling 3a), carmil2 (capping protein regulator and myosin 1 linker 2) and ripor2 (RHO family interacting cell polarization regulator 2), and a downregulation of birc2 (baculoviral IAP repeat containing 2), rgs7b (regulator of G-protein signaling 7 binding protein b) and pcf11 (PCF11 cleavage and polyadenylation factor subunit) (Fig. 3H).
Pathway analysis reveals an enrichment of SPRY domain proteins and transcription factor activity
We used DAVID pathway [37] analysis to investigate biological pathways underlying the observed gene expression changes and classify DEGS into functional clusters. We identified six significantly enriched clusters (enrichment > 2.43) in WT compared to adgrl3.1−/− (Table 1). The most enriched annotation cluster contained the GO term SPRY domain, followed by zinc-finger DNA-binding domains and RNA polymerase II transcription factor activity in cluster 2. Other clusters included metabolism of drugs, xenobiotics and retinal (cluster 4), and immunoglobulins (cluster 5), suggesting that immune system activity may differ between WT and adgrl3.1−/−. Comparison of WT vs. adgrl3.1−/− + ATO identified similar GO terms, including SPRY domain proteins in cluster 1, DNA binding and transcription factor activity in cluster 2, and lectins, interleukins and immunoglobulins in clusters 4, 5, 8, and 9 suggesting an important difference in immune system function between WT and adgrl3.1−/− (Table 1). In contrast, a comparison between adgrl3.1−/− and adgrl3.1−/− + ATO did not reveal any enriched pathways.
Discussion
In this study, we show that adult zebrafish lacking adgrl3.1 displayed high levels of externalizing behaviors (impaired impulse control and increased boldness in a novel situation), attentional deficits, and high levels of hyperactivity, all of which were rescued by atomoxetine. Our findings are thus consistent with the hypothesis that ADGRL3 is associated with core aspects of externalizing disorder phenotypes. We also found evidence of an increased stress response in a novel environment associated with adgrl3.1−/−, with high levels of immobility displayed during habituation to the recording setup prior to hyperactivity being expressed. Finally, differential gene expression (DEG) analysis comparing WT vs. adgrl3.1−/− revealed several DEGs including dusp6 (MKP3), which has been previously identified in a GWAS of ADHD patients [4], and is known to modulate noradrenaline transporter (NET) activity. The DEG analysis also identified several putative functional pathways for externalizing behaviors including enrichment of the SPRY domain, lending support to theories about the role of the immune system in ADHD and other EDs [53, 54].
Disruption of ADGRL3 function has been repeatedly linked to externalizing symptoms in rodents [24,25,26] and zebrafish [27, 28]. Here, we characterized several core externalizing phenotypes in adgrl3.1−/− zebrafish, and the effect of atomoxetine on reducing these behaviors. Although during the training phase adgrl3.1−/− did not show any differences compared to WT, adgrl3.1−/− performed a higher number of incorrect responses than WT in the 5-CSRTT test day. Considering the increased cognitive demands of the test phase [31], these data suggest attentional deficits in adgrl3.1−/− individuals [55]. In the same task, adgrl3.1−/− showed a high level of impulsivity (higher anticipatory responses). Finally, adgrl3.1−/− displayed high rates of boldness in a novel environment, another core feature of externalizing phenotypes [56]. Externalizing behaviors such as impulsivity are debilitating and affect patients’ lives and outcomes. For example, an estimated 26.2% (95% CI: 22.7–29.6 [57]) of prison inmates have ADHD. Increased externalizing behaviors have been cited as key risk factors for criminality [58] and predict the likelihood of delinquency [59]. Furthermore, other behaviors linked to higher rates of impulsivity (e.g., substance abuse) are more common in ADHD patients [12, 60]. adgrl3.1−/− has been linked to several ED, including substance abuse, and this has been shown to be independent of an ADHD diagnosis [12]. Furthermore, ADGRL3 variants are associated with more extreme ADHD phenotypes (ADHD-combined; ADHD-C), worse outcomes in terms of disruptive behavior, persistence into adulthood, and differential response to stimulant medication [61]. Rodents’ models knockout for the Adgrl3 gene also shows altered externalizing behaviors, such as decreased impulse control [62]. The fact that these behavioral phenotypes are so well conserved across vertebrate species, and even invertebrates [63], strongly suggests that ADGRL3 is functionally related to shared externalizing phenotypes such as impulsivity and hyperactivity. This has significant implications for psychiatry, as dysfunctional ADRGL3 may be implicated across a range of ED.
Mechanisms of adgrl3.1-induced impulsivity and hyperactivity
Very little is known about the molecular function of ADGRL3, outside of its role in neuronal migration during development [64]. Here, for the first time, we found that the selective noradrenaline transporter inhibitor atomoxetine fully rescues several externalizing phenotypes in adgrl3.1−/−, suggesting an important role for noradrenaline in ED. Previous work has linked ADGRL3 variants to the dopamine system. Several markers of differential DA and NE activity have been identified in the striatum of Adgrl3 knockout mice, including upregulation of presynaptic Tyrosine Hydroxylase and Slc6a3 (which codes for the dopamine transporter), downregulation of Dopamine receptor d1 in the striatum [24], and upregulation of DAT in the prefrontal cortex [26]. These findings are conserved across vertebrates, with adgrl3.1 morphant zebrafish displaying changes in the topography and the number of dopaminergic neurons in the diencephalon [27, 28]. Collectively, these findings have led to the theory that ADGRL3 exerts its behavioral effects via either direct or indirect effects on striatal dopamine [65]. Dysfunction of the DA system is an attractive hypothesis, given (for example) the therapeutic benefits of psychostimulant and non-psychostimulant medications in externalizing disorders such as ADHD (e.g., atomoxetine blocks the presynaptic noradrenaline transporter, and thus can enhance both noradrenergic and dopaminergic signaling in the synapse). However, this is not necessarily useful from a clinical perspective, given the side effects of current ADHD medications, and the individual variability in therapeutic efficacy [2, 66]. Previous work has shown that transient knockdown of adgrl3.1 in zebrafish larvae renders them more sensitive to stimulation of dopamine signaling [28]. This suggests that adgrl3.1−/− larvae have dysregulated NE levels, perhaps leading to saturation, as NE receptors regulate the response to dopamine agonists [67].
To identify novel therapeutic targets for externalizing symptoms, we carried out a transcriptomic analysis of the whole brain of adult adgrl3.1−/− zebrafish and identified several DEGs. One notable DEG was dusp6 (MKP3), which has been previously identified in an ADHD GWAS [4] and was downregulated in adgrl3.1−/−. Protein kinase c (PKC) regulates the internalization of both DAT and NET, and recently dusp6 (MKP3), a phosphatase that inactivates MAP kinases, has been shown to mediate PKC regulation of transporters [68, 69]. Therefore, it is possible that dusp6 functions as a regulator of neuronal and synaptic plasticity [69]. Together with our data showing that atomoxetine rescues the behavioral phenotypes, this strongly implicates dysfunction of the NE system in more severe forms of ED. adgrl3.1 is a receptor for several ligands, including the Fibronectin leucine-rich transmembrane protein 3 (flrt3) [70]. adgrl3.1 is expressed presynaptically, and flrt3 in the postsynaptic membrane, with interaction occurring via their extracellular tails. Deletion of the chromosome segment which includes FLRT3 increases ADHD risk in humans, suggesting that loss of FLRT3 function may cause the disease [71]. flrt3 mediates cell-adhesion and sorting [72] to control cell migration, axon guidance, and axon outgrowth following injury, as well as activating Fibroblast growth factor (fgf) signaling [73]. FGF receptors are required for the transcription of dusp6. Therefore, it is possible that the fgf pathway, which can activate target genes via MAPK/ERK [73] (a pathway that is known to modulate hyperactivity [74]) underpins externalizing symptoms. Adgrl3 and Flrt3 have also been linked to synaptogenesis during development; antisense knock-down of Adgrl3 or Flrt3 in mouse reduces the number of glutamate synapses in the hippocampus [13, 70]. However, the link between the dopaminergic phenotype of adgrl3.1−/− synaptogenesis is not clear, and it is possible that the function of adgrl3.1−/− differs across different developmental stages. A subset of dopaminergic neurons co-release both dopamine and glutamate and activation of dopamine D2 receptors inhibits both synapse formation and dopamine release [72]. Furthermore, ED-linked neural circuits may be fine-tuned by controlling the number of dopaminergic and glutamatergic synapses [71]. Therefore, it is possible that the noradrenergic phenotype of adrgl3.1−/− leads to a reduction of both dopamine and glutamate synapses, thus altering network activity and triggering ED symptoms. This may be an interesting target for future drug development.
The DAVID analysis revealed several pathways that were enriched in adgrl3.1−/−. Of particular interest was the SPRY domain, which was the most enriched cluster. The SPRY domain is involved with protein interactions in a diverse range of signaling pathways, ranging from innate immunity to RNA processing. Perhaps most interestingly, we found several enriched clusters relating to immune system function in adgrl3.1−/−. The links between externalizing disorders and immune function are well established [75]. Children with ADHD have high levels of neuroinflammatory biomarkers such as Tumor Necrosis Factor-alpha (TNF-α) [75]. In addition, childhood atopic diseases (eczema, asthma) are associated with an increased risk of ADHD [76]. Children with externalizing behavioral problems have elevated levels of C-reactive protein (CRP) and interleukin 6 (IL-6) [77]. Despite this evidence for a link, cause and effect are hard to ascertain as studies are generally correlative in nature [78]. An example is studies into substance use disorders and neuroimmune function: these are confounded by the inflammatory response to the administration of substances of abuse [79, 80]. Here, we identified several pathways linked to innate neuroimmunity, suggesting potential shared genetic mechanisms. Previous transcriptomic analysis of discrete brain regions using mice null for the Adgrl3 gene observed genotype‐dependent DEG and diverse patterns of DEGs according to the age of the animals, particularly relating to cell-adhesion molecules and calcium signaling proteins [81]. With the adult fish here, we found DEGs in similar cell signaling pathways, suggesting some level of conservation. However, there were also several differences in the mouse adgrl3−/− vs. wild-type transcriptome reflecting species-level differences, but also potentially relating to the analysis algorithms employed (i.e., DAVID vs. GAGE analyses).
Finally, although externalizing behaviors and EDs are consistently found to be more common in males than females, the biological basis of this difference is not clear [82,83]. For example, gender differences are observed bidirectionally in impulsivity subtypes [81] and it is hard to disentangle social and environmental factors that may impact on ED (e.g., normative gender roles and teacher/parental influences). Here, we found sex differences in attention, impulsivity, and hyperactivity (both more prominent in male adgrl3.1−/− zebrafish compared to females), but not in the novel object approach. This suggests some potential heritability of sex differences associated with these core ED phenotypes, and merits further investigation.
Conclusion
In this study, we show that adgrl3.1−/− displays strong, innate decreases in inhibitory control, increased risk-taking behavior, decreased attention and increased hyperactivity, suggesting an important genetic basis for externalizing behaviors. All these behaviors were rescued by atomoxetine suggesting a critical role of noradrenergic signaling in these phenotypes. Transcriptomic analyses of adgrl3.1−/− revealed several genes and pathways that may be useful for future study into the genetic basis of ED, and inform targets for future treatment.
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Acknowledgements
This study was financed in part by the Coordenação de Aperfeiçoamento de Pessoal de Nível Superior—Brazil (CAPES)—Finance Code 001 at the University of Portsmouth, UK. MOP currently receives funding from the NC3Rs (UK), and Dstl (UK). FR received funding from the Austrian Science Fund (grant numbers: J4090-B29 and P35774). The funders had no role in study design, data collection, and analysis, decision to publish, or preparation of the manuscript. We are grateful to Slave Trajanoski of the Center for Medical Research at the Medical University of Graz for biostatistical advice.
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Conceptualization: BDF, KÆK, WHJN, MP; Formal analysis: BDF, MP, FR, WHJN; Funding acquisition: BDF, WHJN, MP; Investigation: BDF, NA, CH; Methodology: BDF, FR, CAT, PL, AS, WHJN, MP; Project administration: MP; Resources: FR, PL, AS, MP; Supervision: WHJN, MP; Visualization: BDF, FR, WHJN, MP; Writing—original draft preparation: BDF, WHJN, MP; Writing—review & editing: BDF, FR, CAT, PL, AS, NA, CH, KÆK, WHJN, MP.
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Fontana, B.D., Reichmann, F., Tilley, C.A. et al. adgrl3.1-deficient zebrafish show noradrenaline-mediated externalizing behaviors, and altered expression of externalizing disorder-candidate genes, suggesting functional targets for treatment. Transl Psychiatry 13, 304 (2023). https://doi.org/10.1038/s41398-023-02601-4
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DOI: https://doi.org/10.1038/s41398-023-02601-4
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