Dopaminergic Co-Regulation of Locomotor Development and Motor Neuron Synaptogenesis is Uncoupled by Hypoxia in Zebrafish

Abstract Hypoxic injury to the developing human brain is a complication of premature birth and is associated with long-term impairments of motor function. Disruptions of axon and synaptic connectivity have been linked to developmental hypoxia, but the fundamental mechanisms impacting motor function from altered connectivity are poorly understood. We investigated the effects of hypoxia on locomotor development in zebrafish. We found that developmental hypoxia resulted in decreased spontaneous swimming behavior in larva, and that this motor impairment persisted into adulthood. In evaluation of the diencephalic dopaminergic neurons, which regulate early development of locomotion and constitute an evolutionarily conserved component of the vertebrate dopaminergic system, hypoxia caused a decrease in the number of synapses from the descending dopaminergic diencephalospinal tract (DDT) to spinal cord motor neurons. Moreover, dopamine signaling from the DDT was coupled jointly to motor neuron synaptogenesis and to locomotor development. Together, these results demonstrate the developmental processes regulating early locomotor development and a requirement for dopaminergic projections and motor neuron synaptogenesis. Our findings suggest new insights for understanding the mechanisms leading to motor disability from hypoxic injury of prematurity.


Introduction
Development of the CNS depends on precise regulation of oxygen levels. Absence of oxygen (anoxia) or low oxygen levels (hypoxia) can cause devastating effects on development, and a concomitant range of molecular, cellular, and neuronal changes (Bonkowsky and Son, 2018). Hypoxia is a major complication associated with premature birth, and can lead to permanent neurologic impairments including attention-deficit hyperactivity disorder, autism, cerebral palsy, motor impairment, epilepsy, or intellectual disability (Bass et al., 2004;Barrett et al., 2007;Saigal and Doyle, 2008;Back, 2014;Salmaso et al., 2014). Each year worldwide an estimated 15 million infants are born prematurely (,37 weeks' gestation; Di Fiore et al., 2016). While survival rates for premature infants have drastically improved and the total number of ex-premature infants has increased over the past decade , therapies to treat neurodevelopmental diseases resulting from prematurity have been lacking (Fanaroff et al., 2007;Hintz et al., 2011).
Accumulating evidence has shown that hypoxia causes altered neuronal connectivity in the brains of children born prematurely (Gozzo et al., 2009;Mullen et al., 2011). However, the mechanisms linking altered neuronal connectivity, defined as axon pathfinding and synaptic connectivity, to changes in motor function or behavior in vertebrates are still poorly understand. Previous work has shown that developmental hypoxia causes axon pathfinding errors in commissural telencephalic neurons, due to activation of the hypoxia-inducible factor (hif1) pathway in the developing zebrafish brain (Stevenson et al., 2012;Xing et al., 2015). In vivo as well as in vitro studies have demonstrated that hypoxia affects synapse development as well (Curristin et al., 2002;Valdez et al., 2007;Milash et al., 2016;Segura et al., 2016;Son et al., 2016). What has been lacking, however, is an understanding of how changes in connectivity in vertebrates alter behavior. In contrast, experiments in the nematode Caenorhabditis elegans have shown that altered connectivity after hypoxia causes behavioral changes including altered responses to sensory stimuli (Chang and Bargmann, 2008;Pocock and Hobert, 2010). The vertebrate motor system offers a well-characterized model for understanding functional effects of hypoxia-associated connectivity changes. Development of motor function is a tightly regulated process, involving genetically encoded programs and specification of neuronal types and connections (Garcia-Campmany et al., 2010), but also feedback from environmental pathways, such as central pattern generators (CPGs; Berg et al., 2018;D'Elia and Dasen, 2018). The neurotransmitter dopamine has been identified as a critical mediator in several distinct aspects of motor development: dopamine is a brain-derived signaling factor affecting neurogenesis in the spine (Popolo et al., 2004;Reimer et al., 2013); descending projections from the dopaminergic diencephalospinal tract (DDT) are required for vertebrate locomotor maturation; and it is required for regulation of locomotion (Jay et al., 2015;Sharples et al., 2015). Further, tyrosine hydroxylase (TH) immunoreactivity, a marker for synthesis of dopamine, has been shown juxtaposed to motor neurons (McLean and Fetcho, 2004a).
To explore hypoxia's roles on the interrelationship of motor function and circuitry, we investigated changes in the DDT and motor neuron connectivity, and accompanying effects on locomotor development. We developed transgenic animals expressing fluorescently tagged markers in the DDT and motor neurons to probe for colocalization and proximity at synapses. We found that DDT synaptic proteins immediately juxtapose motor neuron synapses. Since previous studies had shown that hypoxia affected DDT synapses , we characterized the effects of developmental hypoxia on the neurons and circuitry of the DDT and motor neurons. We found no change between hypoxic and normoxic conditions in the number of motor and dopaminergic neurons, or in the axon projections of the DDT to the spinal cord. However, in hypoxic conditions there was a decrease in the number of synapses observed between the DDT and motor neurons. The loss of motor neuron synapses corresponded to a decrease in swimming behaviors compared with normoxic conditions. The impairment in swimming behavior persisted into adulthood, suggesting that developmental hypoxic injury leads to permanent changes in circuitry controlling locomotion.

Ethics statement
All zebrafish experiments were performed in accordance with guidelines from our institute's. Animal Care and Use Committee, regulated under federal law (the Animal Welfare Act and Public Health Services Regulation Act) by the United States Department of Agriculture (USDA) and the Office of Laboratory Animal Welfare at the National Institutes of Health, and accredited by the Association for Assessment and Accreditation of Laboratory Animal Care (AAALAC) International.

Fish stocks, animal husbandry, transgenic line generation
Adult fish were bred according to standard methods. Embryos were raised at 28.5°C in E3 embryo medium with methylene blue, and embryos beyond 24 h postfertilization (hpf) were treated with phenylthiourea (PTU) to prevent pigment formation. For in situ staining and immunohistochemistry, embryos were fixed in 4% paraformaldehyde (PFA) in PBS overnight (O/N) at 4°C, washed briefly in PBS with 0.1% Tween 20, dehydrated stepwise in methanol (MeOH; 25%, 50%, 75%, 100%), and stored in 100% MeOH at À20°C until use.

Hypoxia reagents
For hypoxia experiments, we followed settings and conditions established in previously published protocols (Stevenson et al., 2012;Xing et al., 2015;Gao et al., 2018). In brief, embryonic zebrafish were placed in a sealed Plexiglas chamber connected via a controller that monitored and adjusted nitrogen gas flow to a desired pO 2 set point (Biospherix Ltd.). We observed that equilibration of oxygen partial pressures in water could take several hours measured with a dissolved oxygen water meter (Control Company). Therefore, we pre-equilibrated all solutions to either normoxia or hypoxia for at least 4 h before use, and transferred embryos into and out of preequilibrated solutions. At the desired time, embryos were placed into media that had been equilibrated to the hypoxic conditions. To terminate hypoxia, embryos were returned to media kept in normoxic conditions. Morphologic staging was used to help determine age at fixation for analyses.

Spontaneous swimming behavior analysis
Larval behavior analysis was performed on 5 d postfertilization (dpf) larvae in 96-well square bottom plates (Krackeler Scientific) using a video analysis software program (Noldus EthoVision). All experiments were performed in temperature-controlled room dedicated for behavior analysis. For spontaneous behavior observation, animals were transferred at 5 dpf to the 96-well plate for 30-min acclimations prior to recording of behavior. The spontaneous behavior was measured for a total of 70 min, including under alternating dark (4 Â 10 min) and light (3 Â 10 min) conditions and a one-way ANOVA was conducted.
Terminal deoxynucleotidyl transferase dUTP nick-end labeling (TUNEL) staining TUNEL was performed on whole-mount larvae (ApopTag Fluorescein In Situ Apoptosis Detection kit; Millipore Bioscience Research Reagents). After standard fixation and dehydration of larvae in 100% MeOH, larvae were rehydrated stepwise into PBS with 0.1% Tween 20 (PBST), permeabilized with 10 mg/ml Proteinase K in PBST at 28°C, washed twice with PBST, refixed for 20 min with 4% PFA, and washed with PBST. Subsequently, 75 ml of equilibration buffer was added to the larvae for 1 h and then removed and replaced with 55 ml of "working-strength" (per Apoptosis Detection kit instructions) terminal deoxynucleotidyl transferase enzyme overnight at 37°C. To avoid drying out the larvae, Eppendorf tubes were sealed with Parafilm. Before use, the anti-digoxigenin conjugate was warmed to RT. The end-labeling reaction was stopped by washing the embryos three times for 15 min each with 2 ml of the stop/ wash buffer, followed by three 1-min washes with PBS. Then 65 ml of working-strength sheep anti-digoxigenin rhodamine was added to the embryos overnight at 4°C. Double immunohistochemistry for GFP and TUNEL was performed by TUNEL staining; after washes with PBST, larvae were fixed for 20 min in 4% PFA at RT and washed again with PBST.

Western blot analysis
Thirty larvae (5 dpf) per group were deyolked by triturating and incubating in deyolking buffer (65 mM NaCl, 1.7 mM KCl, and 1.5 mM NaHCO 3 ) for 10 min at RT. Protein was extracted by grinding larval fish with pestle in a 100 ml of lysis buffer (150 mM NaCl, 20 mM Tris-HCl, pH 7.5, 1 mM EDTA, 1% NP-40, and 1% Triton X-100, 1Â Halt Protease and Phosphatase Inhibitor Cocktail; Life Technologies) on ice. The extract was centrifuged for 20 min (16,000 Â g RCF) at 4°C and the supernatant was transferred to a new tube. Total protein concentration was determined by BCA assay (Thermo Scientific Pierce BCA Protein Assay kit, Fisher Scientific). The protein extract was mixed with an equal amount of 2Â Laemmli buffer [20% glycerol, 4% SDS, 0.1% bromophenol blue, 0.125 M Tris (pH 6.8), and 2.5% b -mercaptoethanol] and boiled for 3 min. Samples were stored at À20°C until use. A total of 20 mg of total protein was loaded on to each lane of a 4-20% polyacrylamide gel (Mini-Protean TGX Gel Bio-Rad). After electrophoresis proteins were transferred to PVDF membranes and blocked in 3% non-fat dry milk in TBS (50 mM Tris, 0.138 M NaCl, and 2.7 mM KCl; pH 8.0) for 30 min at RT with agitation. Membranes were split, and then incubated in rabbit anti-TH (1:1000) or rabbit anti-b -actin (1:1000) for 2 h at RT, washed in TBS, and then incubated in HRP-antirabbit (1:5000 dilution) for 1 h at RT. Following incubation with secondary antibody, membranes were washed extensively in TBS containing 0.05% Tween 20, and then subjected to chemiluminescent detection (Clarity Western ECL Substrate; Bio-Rad). The Western blot analysis, imaging, and quantification were performed with a digital imager (Gel Do XR1System and Image Lab Software, Bio-Rad) in three separate experimental replicates.

Microscopy, image analysis, and movie analysis
Confocal imaging was performed, and quantification was performed in ImageJ by compiling a sum projection of 75 slices (step size 2.0 mm) into a single z-stack image. For counts at 72 hpf a 340 Â 170-pixel box was drawn in the telencephalon at with the ventral edge placed on the dorsal edge of the eye and the rostral edge at the nose; at 30 and 48 hpf, a 450 Â 300-pixel box was drawn around the entire brain. Thresholding was applied from a minimum of 125 to a maximum of 255; and the "Analyze Particles" function was used for quantification.

Statistical analysis
All data are presented as means 6 SEM. Analyses comparing dependent measures across hypoxia and normoxia were completed with Student's t test and one-way ANOVA followed by post hoc Tukey test. Overall, statistical significance was set at p 0.05.

Descending dopaminergic axons form synapses adjoining spinal cord motor neurons
We examined the projections of DDT axons, and the proximity of their synapses to spinal cord motor neurons in wild-type zebrafish at 5 dpf. We observed TH-positive (TH 1 ) immunostaining juxtaposed with anti-Hb9-positive (Hb 1 ) staining of motor neurons in the spinal cord (Fig.  1A). To test the source of the TH 1 immunoreactivity, we co-labeled axons in the Tg(otpb.A:EGFP-caax) line, which expresses GFP in the descending DDT (Fujimoto et al., 2011). We found co-expression of TH 1 and GFP in the DDT (Fig. 1B). Next, to evaluate for potential synapse formation between the DDT and motor neurons, we used double transgenic larvae in which a GFP-tagged intrabody (FingR; Gross et al., 2013;Son et al., 2016) labeled the endogenous postsynaptic density 95 (PSD-95) protein at the postsynaptic motor neuron, and RFP-caax labeled the DDT. We found co-localized punctate labeling in the spinal cord of Tg(otpb.A:TRFP-caax); Tg(Hb9:FingR (PSD95)-GFP) larvae, suggesting the presence of synapses between the DDT and motor neurons (Fig. 1C, arrowheads). Interestingly, we identified co-localization of the dopamine receptor 4 (D4R) with the punctate labeling of FingR (PSD95) on motor neurons (Fig. 1D). The D4R has been shown to mediate the developmental requirement for dopamine in locomotor maturation and in neurogenesis of motor neurons (Lambert et al., 2012;Reimer et al., 2013). Together, these data suggest the presence of synapses between the DDT and motor neurons in the developing zebrafish spinal cord.

Hypoxia reduces swimming activity
The DDT is required for locomotor development, and because of our observation of potential synapses between the DDT and motor neurons, we were interested in whether disruption of DDT connectivity would affect motor development. In particular, since hypoxia in developing zebrafish results in pathfinding errors (Stevenson et al., 2012;Xing et al., 2015), and hypoxia has been associated with long-term motor impairment in human infants born prematurely (Martin et al., 2011b;Salmaso et al., 2014), we were interested in whether hypoxia would affect DDT connectivity and lead to resultant swimming deficits. We exposed developing zebrafish larvae to different sublethal hypoxic conditions including 1% pO 2 from 1 to 2 dpf, 3% pO 2 from 2 to 3 dpf, and 5% pO 2 from 3 to 4 dpf. The timing and percentage hypoxia was based on previous work, in which these conditions were shown to be non-lethal, and to be non-disruptive to overall development including aspects of CNS development such as cell fate specification and progenitor specification (Stevenson et al., 2012;Xing et al., 2015). Following hypoxia, animals were returned to normoxia, and behavior was then examined at 5 dpf (as the developmental switch in the episodic locomotor (swimming) pattern occurs around 5 dpf; Fig.  2A; Buss and Drapeau, 2001;Lambert et al., 2012). Spontaneous swimming behavior was measured for 70 min, including under alternating dark (4 Â 10 min) and light (3 Â 10 min) conditions (Fig. 2B). A one-way ANOVA showed effects of hypoxia on motor behavior, including swimming distance in dark (F (3,111) = 11.930, p , 0.01) and in light (F (3,111) = 14.069, p , 0.01); rotation frequency in dark (F (3,111) = 2.860, p , 0.05) and in light (F (3,111) = 6.989, p , 0.01); and velocity in dark (F (3,111) = 12.175, p , 0.01) and in light (F (3,111) = 13.793, p , 0.01). Post hoc comparison using the Tukey HSD test indicated that spontaneous swimming behavior of larval zebrafish exposed to hypoxia was significantly decreased compared with that of larval zebrafish exposed to normoxia (21% pO 2 ; Fig. 2C; Table  1). Taken together, these results suggest that hypoxia decreases the spontaneous swimming behavior of larval zebrafish and impacts motor development.
Importantly, we also found that the motor impairments caused by hypoxia persisted into adulthood. In adult fish that had been exposed to hypoxia as 3-to 4-dpf larvae, we also found significant decreases in distance swam (t (16) = 2.9, p , 0.05) and velocity (t (16) = 2.5, p , 0.05; but not in total time spent swimming (t (16) = 1.1, p = 0.27; Fig.  2D; Table 2). Together, these results are consistent with hypoxia causing deficits in motor behavior that are sustained through development into adulthood. Further, this suggests that specific changes in motor circuitry may be responsible for the impairment in behavior.

Effects of hypoxia on the development of dopaminergic neurons, DDT, and motor neurons
To determine where in the CNS hypoxia was exerting its effects, we labeled hypoxic-treated or normoxic-treated 5 dpf zebrafish with anti-TH (Fig. 3C,B). A one-way ANOVA showed there was a significant effect of hypoxia on the number of TH 1 neurons in the posterior tuberculum (PT; F (3,33) = 13, p , 0.01) with certain hypoxia conditions. The post hoc analysis revealed there was a significantly reduced number of TH 1 dopaminergic neurons observed with 1-to 2-dpf hypoxia (1% pO 2 ) and 2-to 3-dpf hypoxia (3% pO 2 ), but not from 3-to 4-dpf hypoxia (5% pO 2 ; Fig.   3C). This was also reflected in whole zebrafish anti-TH quantification by Western blot analysis at 5 dpf following hypoxia, in which larval zebrafish showed significantly decreased TH levels at earlier stages of hypoxia exposure including 1-2 dpf (1% pO 2 ) and 2-3 dpf (3% pO 2 ), but not at 3-4 dpf (5% pO 2 ) compared with normoxic zebrafish (p = 0.91; Fig. 3D,E). We did not see any errors in pathfinding of the DDT of extraneous midline crossing (Fig. 3B, bottom row); and overall intensity of the DDT descending tracts was unchanged following hypoxia (Fig. 3F).
To determine whether hypoxia could specifically alter CNS circuitry, in the absence of changes in apoptosis or Research Article: New Research cell fate that could cause secondary changes (e.g., following hypoxia at 1-2 or 2-3 dpf), we focused analysis of hypoxia at later developmental stages (3-4 dpf with 5% pO 2 ). That is, we did not want to have confounding effects introduced by the more severe defects caused by earlier hypoxia, such as the reduction in TH1 neurons or altered axons (Fig. 3B, top panels). We counted the number of TH 1 neurons in the PT of the diencephalon at 5 dpf and did not find significant changes in counts following hypoxia exposure (normoxia, 41.9 6 2.2; hypoxia, 34.7 6 3.4, t (15) = 1.848, p = 0.08; Fig. 3C). Nor were there any difference in apoptosis (measured by TUNEL1 counts) in hypoxiatreated animals (t (12) = À1.213, p = 0.249; Fig. 3G-I). We also evaluated axon pathfinding of the longitudinal DDT track, using the transgenic reporter line Tg(otpb.A:egfpcaax) or with anti-TH immunohistochemistry. There were no observed axon pathfinding errors (Fig. 3B,G), and no change in the intensity of anti-TH labeling [normoxia, 19.09 average intensity units (AI) 6 2.73; hypoxia, 16.5 6 1.34 AI, t (13) = 0.795, p = 0.44; Fig. 3E,F], which is suggestive that the axons are not changing routes. We also characterized the effects of hypoxia on motor neurons in the spinal cord. There were no significant hypoxic effects on proliferation counts (t (10) = 0.898, p = 0.390) or apoptosis counts (t (12) = À1.213, p = 0.249) in motor neurons (Fig. 3J-M). Together, these data suggest that 5% pO 2 hypoxia from 3 to 4 dpf did not affect dopaminergic or motor neuron cell counts, apoptosis, or proliferation; and did not affect the axonal projections of the DDT.
Similarly, when exposed zebrafish larvae to a dopaminergic D4 receptor antagonist (L-745870) from 72 to 96 hpf, we observed motor impairments in distance, velocity, and rotation frequency [distance (t (58) = 3.90, p , 0.01), velocity (t (58) = 3.19, p , 0.01), and rotation frequency (t (58) = 3.93, p , 0.01); Fig. 5; Table 3], similar to the effects of hypoxia exposure. Further, inclusion of the D4 receptor antagonist together with hypoxia exposure did not cause any additional worsening of motor phenotypes, consistent with the two exposures acting via a shared or similar mechanism.

Discussion
Our work demonstrates that dopaminergic signaling is necessary for the development of the locomotor synaptic circuitry, and that disruption of the synaptic circuitry impairs motor behavior development. Hypoxia disrupts normal co-regulation of locomotion and synaptogenesis, altering CNS circuitry and leading to persistent deficits in motor behavior. These findings refine our understanding of the role for dopamine, which had previously been continued Figure 2. Hypoxia causes impaired motor behavior in larval and adult animals. A, Experimental set-up for hypoxia (a) and time line (b) of hypoxia exposure and analysis. B, Schematic of behavioral testing paradigm. C, Data plots show impaired motor behavior in hypoxia-exposed larvae, each point is a separate animal. Mean shown, ANOVA, ppppp , 0.0001, pppp , 0.001. D, top, Heat-map of adult zebrafish (six-month-old) exposed to hypoxia (3-to 4-dpf 5% pO 2 ) shows decreased swimming. Below, Hypoxia-exposed zebrafish have persistent decreases in velocity and distance swum as adults animals (normoxia n = 8, pre-hypoxia n = 10); pp , 0.05; SD shown).    (Popolo et al., 2004;Reimer et al., 2013). Although projections of the A11 group of diencephalic dopaminergic neurons into the spinal cord were first characterized in the 1970s (Björklund and Skagerberg, 1979;Hökfelt et al., 1979), early work on the DDT suggested that the DDT terminated in the dorsal horn and was primarily involved in autonomic functions (Skagerberg et al., 1982). However, TH immunoreactivity was identified near motor neurons in the spinal cord (McLean and Fetcho, 2004b), and functional and behavioral studies revealed the DDT is the source of dopamine involved in motor system development (Lambert et al., 2012), and is necessary for on-going regulation of locomotion behavior (Jay et al., 2015;Sharples et al., 2015). Since we and others have now shown roles for dopamine in motor circuitry development and in motor behavior development, this raises the possibility for a coordinating role for dopamine signaling in these processes. We found new evidence regarding the role of dopamine in co-regulation of circuitry development with locomotor development. We used the zebrafish model system, characterizing the motor neuron synapses of the spinal cord and the descending dopamine projections to them. We found a decrease in DDT to motor neuron synapses, which was associated with a decrease in swimming behaviors compared with normoxic conditions. Previous work in vertebrates as well as in invertebrates has shown that developmental hypoxia causes axonal pathfinding errors in telencephalic neurons, through activation of the hypoxia-inducible factor (hif1) pathway (Stevenson et al., 2012;Xing et al., 2015). Hypoxia has also been noted to affect synapse development (Curristin et al., 2002;Segura et al., 2016;Zhuravin et al., 2019), but in this work we identified that hypoxia could act on dopaminergic signaling to affect synapse development, including effects on synaptic circuitry, and short-and long-term behavioral effects. However, we cannot exclude that hypoxia might have multifactorial impacts on behavior and locomotor development, for example, that hypoxia could be affecting myelin development or function; or of other aspects of circuitry, for example, motor neuron to muscle synapses. This work also found new evidence for co-localization of DDT descending tract synapses with motor neuron synapses. This finding, if also observed in humans, could provide novel insights into unexplored aspects of human locomotion as well as into pathologies associated with premature birth. In mammals the A11 DDT is also dopaminergic (Koblinger et al., 2014). Premature birth is associated with hypoxic exposures during a critical period of brain development (Martin et al., 2011b(Martin et al., , 2012 from 24 to 36 weeks PCA (postconception age), and includes when axon and synaptic connections are forming. This period includes corticospinal tract extension and innervation of spinal primary motor neurons; development of the corpus callosum; thalamocortical axon formation; and the connection of cortical with subcortical areas (Eyre et al., 2000;ten Donkelaar et al., 2004;Haynes et al., 2005;Ren et al., 2006;Kostovic and Jovanov-Milosevic, 2006;Vasung et al., 2010). Hypoxia from prematurity is strongly correlated with the risk for neuromotor impairment (Martin et al., 2011b;Salmaso et al., 2014) and can affect up to 60% of infants (Williams et al., 2010). The hypoxia is secondary to a complex set of conditions, including utero-placental insufficiency and immaturity of the cardiopulmonary system. Following birth, premature infants can experience up to 600 hypoxic episodes per week, each lasting at least .10 s (Martin et al., 2011b).
The impaired locomotion from the developmental hypoxia persists into adulthood. The findings may offer insight into the adverse motor effects of prematurity and accompanying hypoxia. Each year, 13 million infants worldwide are born prematurely (Beck et al., 2010;Martin et al., 2011a), and motor impairment affects a majority of children born prematurely (Williams et al., 2010) with little insight into pathophysiology and no available treatments. Key future research areas include understanding the interaction between myelination and oligodendrocytes, the effects on circuitry from hypoxia, and the relationship of Figure 5. Dopaminergic antagonist exposure impairs zebrafish locomotor development similar to effects of hypoxia. Analysis of zebrafish larvae at 5 dpf, following exposure to L-745870 from 72 to 96 hpf. Impairments in distance, velocity, and rotation frequency (quantified data in Table 3). Each point is a separate animal. Mean shown, ANOVA; pppp , 0.001. Hyp, hypoxia; Nor, normoxia. Table 3: Motor behavior in zebrafish larvae following hypoxia or normoxia, with or without exposure to a dopaminergic D4 receptor antagonist (L-745870) from 72 to 96 hpf