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Development of the nervous system
Development of the nervous system
Development of the nervous system
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Development of organ systems

The development of the nervous system, or neural development (neurodevelopment), refers to the processes that generate, shape, and reshape the nervous system of animals, from the earliest stages of embryonic development to adulthood. The field of neural development draws on both neuroscience and developmental biology to describe and provide insight into the cellular and molecular mechanisms by which complex nervous systems develop, from nematodes and fruit flies to mammals.

Defects in neural development can lead to malformations such as holoprosencephaly, and a wide variety of neurological disorders including limb paresis and paralysis, balance and vision disorders, and seizures,[1] and in humans other disorders such as Rett syndrome, Down syndrome and intellectual disability.[2]

Vertebrate brain development

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Diagram of the vertebrate nervous system
Further information: Development of the nervous system in humans

The vertebrate central nervous system (CNS) is derived from the ectoderm—the outermost germ layer of the embryo. A part of the dorsal ectoderm becomes specified to neural ectoderm – neuroectoderm that forms the neural plate along the dorsal side of the embryo.[3][4] This is a part of the early patterning of the embryo (including the invertebrate embryo) that also establishes an anterior-posterior axis.[5][6] The neural plate is the source of the majority of neurons and glial cells of the CNS. The neural groove forms along the long axis of the neural plate, and the neural plate folds to give rise to the neural tube.[7] This process is known as neurulation.[8] When the tube is closed at both ends it is filled with embryonic cerebrospinal fluid.[9] As the embryo develops, the anterior part of the neural tube expands and forms three primary brain vesicles, which become the forebrain (prosencephalon), midbrain (mesencephalon), and hindbrain (rhombencephalon). These simple, early vesicles enlarge and further divide into the telencephalon (future cerebral cortex and basal ganglia), diencephalon (future thalamus and hypothalamus), mesencephalon (future colliculi), metencephalon (future pons and cerebellum), and myelencephalon (future medulla).[10] The CSF-filled central chamber is continuous from the telencephalon to the central canal of the spinal cord, and constitutes the developing ventricular system of the CNS. Embryonic cerebrospinal fluid differs from that formed in later developmental stages, and from adult CSF; it influences the behavior of neural precursors.[9] Because the neural tube gives rise to the brain and spinal cord any mutations at this stage in development can lead to fatal deformities like anencephaly or lifelong disabilities like spina bifida. During this time, the walls of the neural tube contain neural stem cells, which drive brain growth as they divide many times. Gradually some of the cells stop dividing and differentiate into neurons and glial cells, which are the main cellular components of the CNS.[4] The newly generated neurons migrate to different parts of the developing brain to self-organize into different brain structures. Once the neurons have reached their regional positions, they extend axons and dendrites, which allow them to communicate with other neurons via synapses. Synaptic communication between neurons leads to the establishment of functional neural circuits that mediate sensory and motor processing, and underlie behavior.[11]

Flowchart of human brain development

Induction

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During early embryonic development of the vertebrate, the dorsal ectoderm becomes specified to give rise to the epidermis and the nervous system; a part of the dorsal ectoderm becomes specified to neural ectoderm to form the neural plate which gives rise to the nervous system.[3][12] The conversion of undifferentiated ectoderm to neuroectoderm requires signals from the mesoderm. At the onset of gastrulation presumptive mesodermal cells move through the dorsal blastopore lip and form a layer of mesoderm in between the endoderm and the ectoderm. Mesodermal cells migrate along the dorsal midline to give rise to the notochord that develops into the vertebral column. Neuroectoderm overlying the notochord develops into the neural plate in response to a diffusible signal produced by the notochord. The remainder of the ectoderm gives rise to the epidermis. The ability of the mesoderm to convert the overlying ectoderm into neural tissue is called neural induction.[citation needed]

In the early embryo, the neural plate folds outwards to form the neural groove. Beginning in the future neck region, the neural folds of this groove close to create the neural tube. The formation of the neural tube from the ectoderm is called neurulation. The ventral part of the neural tube is called the basal plate; the dorsal part is called the alar plate. The hollow interior is called the neural canal, and the open ends of the neural tube, called the neuropores, close off.[13]

A transplanted blastopore lip can convert ectoderm into neural tissue and is said to have an inductive effect. Neural inducers are molecules that can induce the expression of neural genes in ectoderm explants without inducing mesodermal genes as well. Neural induction is often studied in Xenopus embryos since they have a simple body plan and there are good markers to distinguish between neural and non-neural tissue. Examples of neural inducers are the molecules noggin and chordin.[citation needed]

When embryonic ectodermal cells are cultured at low density in the absence of mesodermal cells they undergo neural differentiation (express neural genes), suggesting that neural differentiation is the default fate of ectodermal cells. In explant cultures (which allow direct cell-cell interactions) the same cells differentiate into epidermis. This is due to the action of BMP4 (a TGF-β family protein) that induces ectodermal cultures to differentiate into epidermis. During neural induction, noggin and chordin are produced by the dorsal mesoderm (notochord) and diffuse into the overlying ectoderm to inhibit the activity of BMP4. This inhibition of BMP4 causes the cells to differentiate into neural cells. Inhibition of TGF-β and BMP (bone morphogenetic protein) signaling can efficiently induce neural tissue from pluripotent stem cells.[14]

Regionalization

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In a later stage of development the superior part of the neural tube flexes at the level of the future midbrain—the mesencephalon, at the mesencephalic flexure or cephalic flexure. Above the mesencephalon is the prosencephalon (future forebrain) and beneath it is the rhombencephalon (future hindbrain).[citation needed]

The alar plate of the prosencephalon expands to form the telencephalon which gives rise to the cerebral hemispheres, whilst its basal plate becomes the diencephalon. The optical vesicle (which eventually become the optic nerve, retina and iris) forms at the basal plate of the prosencephalon.[citation needed]

Patterning

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In chordates, dorsal ectoderm forms all neural tissue and the nervous system. Patterning occurs due to specific environmental conditions - different concentrations of signaling molecules[citation needed]

Dorsoventral axis

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The ventral half of the neural plate is controlled by the notochord, which acts as the 'organiser'. The dorsal half is controlled by the ectoderm plate, which flanks either side of the neural plate.[15]

Ectoderm follows a default pathway to become neural tissue. Evidence for this comes from single, cultured cells of ectoderm, which go on to form neural tissue. This is postulated to be because of a lack of BMPs, which are blocked by the organiser. The organiser may produce molecules such as follistatin, noggin and chordin that inhibit BMPs.[citation needed]

The ventral neural tube is patterned by sonic hedgehog (Shh) from the notochord, which acts as the inducing tissue. Notochord-derived Shh signals to the floor plate, and induces Shh expression in the floor plate. Floor plate-derived Shh subsequently signals to other cells in the neural tube, and is essential for proper specification of ventral neuron progenitor domains. Loss of Shh from the notochord and/or floor plate prevents proper specification of these progenitor domains. Shh binds Patched1, relieving Patched-mediated inhibition of Smoothened, leading to activation of the Gli family of transcription factors (GLI1, GLI2, and GLI3).[citation needed]

In this context Shh acts as a morphogen - it induces cell differentiation dependent on its concentration. At low concentrations it forms ventral interneurons, at higher concentrations it induces motor neuron development, and at highest concentrations it induces floor plate differentiation. Failure of Shh-modulated differentiation causes holoprosencephaly.[citation needed]

The dorsal neural tube is patterned by BMPs from the epidermal ectoderm flanking the neural plate. These induce sensory interneurons by activating Sr/Thr kinases and altering SMAD transcription factor levels.[citation needed]

Rostrocaudal (Anteroposterior) axis

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Signals that control anteroposterior neural development include FGF and retinoic acid, which act in the hindbrain and spinal cord.[16] The hindbrain, for example, is patterned by Hox genes, which are expressed in overlapping domains along the anteroposterior axis under the control of retinoic acid. The 3 (3 prime end) genes in the Hox cluster are induced by retinoic acid in the hindbrain, whereas the 5 (5 prime end) Hox genes are not induced by retinoic acid and are expressed more posteriorly in the spinal cord. Hoxb-1 is expressed in rhombomere 4 and gives rise to the facial nerve. Without this Hoxb-1 expression, a nerve similar to the trigeminal nerve arises.[citation needed]

Neurogenesis

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Neurogenesis is the process by which neurons are generated from neural stem cells and progenitor cells. Neurons are 'post-mitotic', meaning that they will never divide again for the lifetime of the organism.[11]

Epigenetic modifications play a key role in regulating gene expression in differentiating neural stem cells and are critical for cell fate determination in the developing and adult mammalian brain. Epigenetic modifications include DNA cytosine methylation to form 5-methylcytosine and 5-methylcytosine demethylation.[17][18] DNA cytosine methylation is catalyzed by DNA methyltransferases (DNMTs). Methylcytosine demethylation is catalyzed in several sequential steps by TET enzymes that carry out oxidative reactions (e.g. 5-methylcytosine to 5-hydroxymethylcytosine) and enzymes of the DNA base excision repair (BER) pathway.[17]

Neuronal migration

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Corticogenesis: younger neurons migrate past older ones using radial glia as a scaffolding. Cajal–Retzius cells (red) release reelin (orange).

Neuronal migration is the method by which neurons travel from their origin or birthplace to their final position in the brain. There are several ways they can do this, e.g. by radial migration or tangential migration. Sequences of radial migration (also known as glial guidance) and somal translocation have been captured by time-lapse microscopy.[19]

Tangential migration of interneurons from ganglionic eminence

Radial

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Neuronal precursor cells proliferate in the ventricular zone of the developing neocortex, where the principal neural stem cell is the radial glial cell. The first postmitotic cells must leave the stem cell niche and migrate outward to form the preplate, which is destined to become Cajal–Retzius cells and subplate neurons. These cells do so by somal translocation. Neurons migrating with this mode of locomotion are bipolar and attach the leading edge of the process to the pia. The soma is then transported to the pial surface by nucleokinesis, a process by which a microtubule "cage" around the nucleus elongates and contracts in association with the centrosome to guide the nucleus to its final destination.[20]

Radial glial cells, whose fibers serve as a scaffolding for migrating cells and a means of radial communication mediated by calcium dynamic activity,[21][22] act as the main excitatory neuronal stem cell of the cerebral cortex[23][24] or translocate to the cortical plate and differentiate either into astrocytes or neurons.[25] Somal translocation can occur at any time during development.[19]

Subsequent waves of neurons split the preplate by migrating along radial glial fibres to form the cortical plate. Each wave of migrating cells travel past their predecessors forming layers in an inside-out manner, meaning that the youngest neurons are the closest to the surface.[26][27] It is estimated that glial guided migration represents 90% of migrating neurons in human and about 75% in rodents.[28]

Tangential

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Most interneurons migrate tangentially through multiple modes of migration to reach their appropriate location in the cortex. An example of tangential migration is the movement of interneurons from the ganglionic eminence to the cerebral cortex. One example of ongoing tangential migration in a mature organism, observed in some animals, is the rostral migratory stream connecting subventricular zone and olfactory bulb.[citation needed]

Axophilic

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Many neurons migrating along the anterior-posterior axis of the body use existing axon tracts to migrate along; this is called axophilic migration. An example of this mode of migration is in GnRH-expressing neurons, which make a long journey from their birthplace in the nose, through the forebrain, and into the hypothalamus.[29] Many of the mechanisms of this migration have been worked out, starting with the extracellular guidance cues[30] that trigger intracellular signaling. These intracellular signals, such as calcium signaling, lead to actin[31] and microtubule[32] cytoskeletal dynamics, which produce cellular forces that interact with the extracellular environment through cell adhesion proteins[33] to cause the movement of these cells.

Multipolar

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There is also a method of neuronal migration called multipolar migration.[34][35] This is seen in multipolar cells, which in the human, are abundantly present in the cortical intermediate zone. They do not resemble the cells migrating by locomotion or somal translocation. Instead these multipolar cells express neuronal markers and extend multiple thin processes in various directions independently of the radial glial fibers.[34]

Neurotrophic factors

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The survival of neurons is regulated by survival factors, called trophic factors. The neurotrophic hypothesis was formulated by Victor Hamburger and Rita Levi Montalcini based on studies of the developing nervous system. Victor Hamburger discovered that implanting an extra limb in the developing chick led to an increase in the number of spinal motor neurons. Initially he thought that the extra limb was inducing proliferation of motor neurons, but he and his colleagues later showed that there was a great deal of motor neuron death during normal development, and the extra limb prevented this cell death. According to the neurotrophic hypothesis, growing axons compete for limiting amounts of target-derived trophic factors and axons that fail to receive sufficient trophic support die by apoptosis. It is now clear that factors produced by a number of sources contribute to neuronal survival.[citation needed]

  • Nerve Growth Factor (NGF): Rita Levi Montalcini and Stanley Cohen purified the first trophic factor, Nerve Growth Factor (NGF), for which they received the Nobel Prize. There are three NGF-related trophic factors: BDNF, NT3, and NT4, which regulate survival of various neuronal populations. The Trk proteins act as receptors for NGF and related factors. Trk is a receptor tyrosine kinase. Trk dimerization and phosphorylation leads to activation of various intracellular signaling pathways including the MAP kinase, Akt, and PKC pathways.[citation needed]
  • CNTF: Ciliary neurotrophic factor is another protein that acts as a survival factor for motor neurons. CNTF acts via a receptor complex that includes CNTFRα, GP130, and LIFRβ. Activation of the receptor leads to phosphorylation and recruitment of the JAK kinase, which in turn phosphorylates LIFRβ. LIFRβ acts as a docking site for the STAT transcription factors. JAK kinase phosphorylates STAT proteins, which dissociate from the receptor and translocate to the nucleus to regulate gene expression.[citation needed]
  • GDNF: Glial derived neurotrophic factor is a member of the TGFb family of proteins, and is a potent trophic factor for striatal neurons. The functional receptor is a heterodimer, composed of type 1 and type 2 receptors. Activation of the type 1 receptor leads to phosphorylation of Smad proteins, which translocate to the nucleus to activate gene expression.[citation needed]

Synapse formation

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Neuromuscular junction

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Main article: Neuromuscular junction

Much of our understanding of synapse formation comes from studies at the neuromuscular junction. The transmitter at this synapse is acetylcholine. The acetylcholine receptor (AchR) is present at the surface of muscle cells before synapse formation. The arrival of the nerve induces clustering of the receptors at the synapse. McMahan and Sanes showed that the synaptogenic signal is concentrated at the basal lamina. They also showed that the synaptogenic signal is produced by the nerve, and they identified the factor as Agrin. Agrin induces clustering of AchRs on the muscle surface and synapse formation is disrupted in agrin knockout mice. Agrin transduces the signal via MuSK receptor to rapsyn. Fischbach and colleagues showed that receptor subunits are selectively transcribed from nuclei next to the synaptic site. This is mediated by neuregulins.[citation needed]

In the mature synapse each muscle fiber is innervated by one motor neuron. However, during development, many of the fibers are innervated by multiple axons. Lichtman and colleagues have studied the process of synapses elimination.[36] This is an activity-dependent event. Partial blockage of the receptor leads to retraction of corresponding presynaptic terminals. Later they used a connectomic approach, i.e., tracing out all the connections between motor neurons and muscle fibers, to characterize developmental synapse elimination on the level of a full circuit. Analysis confirmed the massive rewiring, 10-fold decrease in the number of synapses, that takes place as axons prune their motor units but add more synaptic areas at the NMJs with which they remain in contact.[37]

CNS synapses

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Agrin appears not to be a central mediator of CNS synapse formation and there is active interest in identifying signals that mediate CNS synaptogenesis. Neurons in culture develop synapses that are similar to those that form in vivo, suggesting that synaptogenic signals can function properly in vitro. CNS synaptogenesis studies have focused mainly on glutamatergic synapses. Imaging experiments show that dendrites are highly dynamic during development and often initiate contact with axons. This is followed by recruitment of postsynaptic proteins to the site of contact. Stephen Smith and colleagues have shown that contact initiated by dendritic filopodia can develop into synapses.[citation needed]

Induction of synapse formation by glial factors: Barres and colleagues made the observation that factors in glial conditioned media induce synapse formation in retinal ganglion cell cultures. Synapse formation in the CNS is correlated with astrocyte differentiation suggesting that astrocytes might provide a synaptogenic factor. The identity of the astrocytic factors is not yet known.[citation needed]

Neuroligins and SynCAM as synaptogenic signals: Sudhof, Serafini, Scheiffele and colleagues have shown that neuroligins and SynCAM can act as factors that induce presynaptic differentiation. Neuroligins are concentrated at the postsynaptic site and act via neurexins concentrated in the presynaptic axons. SynCAM is a cell adhesion molecule that is present in both pre- and post-synaptic membranes.[citation needed]

Assembly of neural circuits

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Further information: Activity-dependent plasticity

The processes of neuronal migration, differentiation and axon guidance are generally believed to be activity-independent mechanisms and rely on hard-wired genetic programs in the neurons themselves. Research findings however have implicated a role for activity-dependent mechanisms in mediating some aspects of these processes such as the rate of neuronal migration,[38] aspects of neuronal differentiation[39] and axon pathfinding.[40] Activity-dependent mechanisms influence neural circuit development and are crucial for laying out early connectivity maps and the continued refinement of synapses which occurs during development.[41] There are two distinct types of neural activity we observe in developing circuits -early spontaneous activity and sensory-evoked activity. Spontaneous activity occurs early during neural circuit development even when sensory input is absent and is observed in many systems such as the developing visual system,[42][43] auditory system,[44][45] motor system,[46] hippocampus,[47] cerebellum[48] and neocortex.[49]

Experimental techniques such as direct electrophysiological recording, fluorescence imaging using calcium indicators and optogenetic techniques have shed light on the nature and function of these early bursts of activity.[50][51] They have distinct spatial and temporal patterns during development[52] and their ablation during development has been known to result in deficits in network refinement in the visual system.[53] In the immature retina, waves of spontaneous action potentials arise from the retinal ganglion cells and sweep across the retinal surface in the first few postnatal weeks.[54] These waves are mediated by neurotransmitter acetylcholine in the initial phase and later on by glutamate.[55] They are thought to instruct the formation of two sensory maps- the retinotopic map and eye-specific segregation.[56] Retinotopic map refinement occurs in downstream visual targets in the brain-the superior colliculus (SC) and dorsal lateral geniculate nucleus (LGN).[57] Pharmacological disruption and mouse models lacking the β2 subunit of the nicotinic acetylcholine receptor has shown that the lack of spontaneous activity leads to marked defects in retinotopy and eye-specific segregation.[56]

Recent studies confirm that microglia, the resident immune cell of the brain, establish direct contacts with the cell bodies of developing neurons, and through these connections, regulate neurogenesis, migration, integration and the formation of neuronal networks in an activity-dependent manner.[58]

In the developing auditory system, developing cochlea generate bursts of activity which spreads across the inner hair cells and spiral ganglion neurons which relay auditory information to the brain.[59] ATP release from supporting cells triggers action potentials in inner hair cells.[60] In the auditory system, spontaneous activity is thought to be involved in tonotopic map formation by segregating cochlear neuron axons tuned to high and low frequencies.[59] In the motor system, periodic bursts of spontaneous activity are driven by excitatory GABA and glutamate during the early stages and by acetylcholine and glutamate at later stages.[61] In the developing zebrafish spinal cord, early spontaneous activity is required for the formation of increasingly synchronous alternating bursts between ipsilateral and contralateral regions of the spinal cord and for the integration of new cells into the circuit.[62] Motor neurons innervating the same twitch muscle fibers are thought to maintain synchronous activity which allows both neurons to remain in contact with the muscle fiber in adulthood.[37] In the cortex, early waves of activity have been observed in the cerebellum and cortical slices.[63] Once sensory stimulus becomes available, final fine-tuning of sensory-coding maps and circuit refinement begins to rely more and more on sensory-evoked activity as demonstrated by classic experiments about the effects of sensory deprivation during critical periods.[63]

Contemporary diffusion-weighted MRI techniques may also uncover the macroscopic process of axonal development. The connectome can be constructed from diffusion MRI data: the vertices of the graph correspond to anatomically labelled gray matter areas, and two such vertices, say u and v, are connected by an edge if the tractography phase of the data processing finds an axonal fiber that connects the two areas, corresponding to u and v.

Consensus Connectome Dynamics

Numerous braingraphs, computed from the Human Connectome Project can be downloaded from the http://braingraph.org site. The Consensus Connectome Dynamics (CCD) is a remarkable phenomenon that was discovered by continuously decreasing the minimum confidence-parameter at the graphical interface of the Budapest Reference Connectome Server.[64][65] The Budapest Reference Connectome Server (http://connectome.pitgroup.org) depicts the cerebral connections of n=418 subjects with a frequency-parameter k: For any k=1,2,...,n one can view the graph of the edges that are present in at least k connectomes. If parameter k is decreased one-by-one from k=n through k=1 then more and more edges appear in the graph, since the inclusion condition is relaxed. The surprising observation is that the appearance of the edges is far from random: it resembles a growing, complex structure, like a tree or a shrub (visualized on the animation on the left).

It is hypothesized in [66] that the growing structure copies the axonal development of the human brain: the earliest developing connections (axonal fibers) are common at most of the subjects, and the subsequently developing connections have larger and larger variance, because their variances are accumulated in the process of axonal development.

Synapse elimination

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Main article: Synaptic pruning

Several motorneurons compete for each neuromuscular junction, but only one survives until adulthood.[36] Competition in vitro has been shown to involve a limited neurotrophic substance that is released, or that neural activity infers advantage to strong post-synaptic connections by giving resistance to a toxin also released upon nerve stimulation. In vivo, it is suggested that muscle fibres select the strongest neuron through a retrograde signal or that activity-dependent synapse elimination mechanisms determine the identity of the "winning" axon at a motor endplate.[37]

Mapping

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Brain mapping can show how an animal's brain changes throughout its lifetime. As of 2021, scientists mapped and compared the whole brains of eight C. elegans worms across their development on the neuronal level[67][68] and the complete wiring of a single mammalian muscle from birth to adulthood.[37]

Adult neurogenesis

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Main article: Adult neurogenesis

Neurogenesis also occurs in specific parts of the adult brain.

See also

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References

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[edit]
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Development of the nervous system

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The development of the nervous system encompasses the intricate embryological and postnatal processes that form the (CNS), including the and , as well as the peripheral nervous system (PNS), beginning in the third week of and extending through . This process starts with , where the folds to create the , induced by signals from the underlying , and differentiates into the foundational structures of the CNS by the end of the eighth gestational week. Key phases include neural induction, proliferation, neuronal migration, differentiation into specialized cell types, exuberant followed by , and progressive myelination, all genetically programmed yet modulated by environmental factors. During early embryogenesis, establishes the three germ layers, with the giving rise to the around days 17–18 post-fertilization. The secretes signaling molecules like Sonic to induce formation, leading to the elevation and fusion of neural folds into the by days 25–28, when the anterior and posterior neuropores close. Concurrently, cells delaminate from the dorsal to migrate and contribute to the PNS, including sensory and autonomic ganglia, as well as non-neural structures like melanocytes and . Disruptions during this primary neurulation (days 17–28) can result in severe congenital malformations such as or , highlighting the period's vulnerability to teratogens like . The then regionalizes into the and : the rostral portion expands into three primary brain vesicles by the fourth week—prosencephalon (), mesencephalon (), and rhombencephalon ()—which further subdivide into five secondary vesicles by the fifth week, laying the groundwork for cerebral hemispheres, , , and . The develops from the caudal , forming three layers: the ventricular zone ( site), (gray matter precursors), and marginal zone ( tracts). peaks between gestational weeks 8 and 20 in the ventricular and subventricular zones, producing approximately 86 billion neurons through asymmetric division of progenitor cells. Post-neurogenesis, migrating neurons follow radial glial scaffolds to establish cortical layers, a process active from weeks 8 to 24, with deeper layers forming first. Differentiation follows, where post-mitotic neurons extend axons and dendrites to form circuits, such as thalamocortical connections by week 26. begins prenatally but surges postnatally, reaching a peak density around age 2–3 years before selective pruning refines connectivity through , influenced by sensory experience and activity-dependent mechanisms. Myelination, insulating axons for efficient signaling, commences in the fetal period via in the CNS and Schwann cells in the PNS, but continues into the third decade, particularly in association fibers. This protracted development underscores the nervous system's plasticity, with critical periods where genetic factors (e.g., transcription factors like and Emx2) interact with extrinsic cues to shape regional identity and function, while vulnerabilities persist, as seen in teratogen effects during weeks 3–8. Overall, these coordinated events transform a simple into a highly organized network capable of processing information, adapting to the environment, and supporting complex behaviors.

Embryonic Induction and Formation

Neural Induction

Neural induction is the process by which presumptive ectodermal cells are specified to adopt a neural fate during early embryogenesis, primarily through signaling from the dorsal known as the Spemann-Mangold organizer. In landmark experiments conducted in 1924, and Hilde Mangold transplanted the dorsal lip of the blastopore from one amphibian gastrula to the ventral side of another, resulting in the induction of a secondary embryonic axis complete with neural tissue. This demonstrated that the dorsal acts as an organizer, emitting signals that direct overlying to form the instead of , establishing the concept of embryonic induction. At the molecular level, neural induction involves the secretion of BMP antagonists from the organizer, which inhibit (BMP) signaling in the to promote neural fate. Key molecules include Noggin, identified as a secreted protein from the Spemann organizer that directly induces neural markers in ectodermal explants.90317-4) Chordin, another organizer-derived factor, similarly neuralizes by binding and sequestering BMPs, preventing their interaction with receptors. contributes by antagonizing BMP activity through direct binding, thereby facilitating neural specification in vivo.90200-X) These inhibitors establish a of BMP signaling, with high levels promoting epidermal fate ventrally and low or absent levels dorsally leading to formation. The ectoderm's competence to respond to these inductive signals is modulated by Wnt and FGF pathways, which prime cells during pre-gastrulation stages. FGF signaling, particularly from endomesodermal sources, is essential for conferring neural competence in ectoderm, enabling it to interpret BMP inhibition as a neural cue. Wnt pathways similarly influence ectodermal responsiveness, often by restricting non-neural fates and supporting the transition to neural progenitors. In vertebrates, neural induction occurs during : in amphibians and around the mid-gastrula stage, in birds and mammals shortly after primitive streak formation, and in humans approximately during the third week of (days 16-21). This process culminates in the establishment of the , setting the stage for subsequent patterning and morphogenesis.

Neurulation

Neurulation is the morphological process by which the , induced by underlying mesodermal signals, transforms into a hollow that will develop into the . This occurs through coordinated cellular shape changes, tissue bending, and fusion events in the . Primary forms the majority of the anterior , while secondary completes the posterior portion. In primary neurulation, the flat first elongates along the anteroposterior axis through convergent extension, where cells intercalate to narrow and lengthen the tissue. The plate then thickens at its edges to form neural folds, separated by a central neural groove, driven by differential and changes. The neural folds elevate and converge toward the midline due to apical constriction of neuroepithelial cells, where the apical surface narrows, adopting a wedge-like that facilitates bending at medial and dorsolateral hinge points. This constriction is powered by actomyosin contractility, involving non-muscle II and actin filaments that generate contractile forces at adherens junctions, often organized into circumferential cables. Planar cell polarity (PCP) signaling, mediated by core PCP proteins like Van Gogh-like 2 (Vangl2), orients these actomyosin networks along the mediolateral axis, ensuring anisotropic tension that promotes fold elevation and midline fusion. Once the folds meet and zipper together, starting at the future hindbrain-cervical junction around embryonic day 22 in humans, the overlying surface separates, and the detaches to form a closed . Anterior neuropore closure occurs around day 25, and posterior neuropore closure by day 28 post-fertilization. Secondary neurulation, which follows primary neurulation in the caudal region at the future sacral level, involves the formation of a solid rod of mesenchymal cells called the medullary cord from the remnants. This cord aggregates, sinks deeper into the , and undergoes —a process of lumen formation through and fluid accumulation—to connect seamlessly with the primary . Unlike primary neurulation, it lacks prominent folding and relies more on mesenchymal-to-epithelial transition. In humans, this process begins after 30 and completes the lowermost . Failure of these processes leads to neural tube defects (NTDs), severe congenital anomalies. Anterior neurulation failure results in anencephaly, where the cranial remains open, leading to absence of the forebrain and calvaria due to degeneration of exposed neural tissue; this is linked to disruptions at initial closure sites during primary . Posterior failure causes spina bifida, such as myelomeningocele (open spina bifida), where the spinal does not close, exposing the cord and and often causing paralysis and ; open forms arise from primary arrest, while some closed spina bifida variants involve secondary defects. These NTDs highlight the precision of , with multifactorial causes including genetic mutations in PCP pathways and environmental factors like .

Patterning Mechanisms

Rostrocaudal Axis

The rostrocaudal axis, also known as the anterior-posterior axis, establishes the head-to-tail organization of the vertebrate during embryonic development, dividing the into distinct regions including the , , , and . This patterning occurs through a combination of transcriptional regulators and diffusible signaling molecules that provide positional information to neural progenitor cells. play a central role in this process, with their expression patterns conferring segment-specific identities along the axis. In vertebrates, are organized into four clusters (HoxA, HoxB, HoxC, and HoxD) on different chromosomes, and their expression follows spatial and temporal colinearity, where genes at the 3' end of each cluster are activated earlier and in more anterior positions, while 5' genes are expressed later and more posteriorly. This combinatorial code of expression specifies regional identities, such as cervical, thoracic, or segments in the , and influences neuronal subtype diversification. For instance, Hox6 paralogs are associated with brachial motor neuron pools, while Hox9-10 genes define thoracic identities. Several signaling centers act as secondary organizers to refine rostrocaudal boundaries. The anterior neural ridge (ANR) at the rostral end secretes fibroblast growth factor 8 (FGF8), promoting forebrain development and inhibiting posterior fates. The isthmic organizer, located at the midbrain-hindbrain junction, expresses Wnt1 and Fgf8 to demarcate the midbrain and cerebellum. More posteriorly, the zona limitans intrathalamica (ZLI) in the diencephalon produces Sonic hedgehog (Shh), which patterns thalamic and prethalamic regions while being modulated by opposing signals from adjacent organizers. Gradient-based models further contribute to patterning, with retinoic acid (RA) acting as a posteriorizing signal derived from the somites and node, activating Hox genes and promoting hindbrain and spinal cord fates in a concentration-dependent manner. Opposing this, anterior structures such as the visceral endoderm secrete Wnt antagonists like Dickkopf-1 (Dkk1), which inhibit posteriorizing Wnt signals and maintain forebrain identity by suppressing posterior markers such as certain Hox genes. These mechanisms interact dynamically to establish sharp boundaries and ensure proper regionalization. The core elements of rostrocaudal patterning, including deployment and organizer functions, are evolutionarily conserved across vertebrates, from lampreys to mammals, reflecting an ancient bilaterian origin for axial neural organization. Comparative studies show similar Hox expression profiles in the spinal cords of jawless and jawed vertebrates, underscoring the stability of these systems despite diversification in brain complexity.

Dorsoventral Axis

The dorsoventral axis of the is established through opposing that specify distinct domains, leading to the formation of sensory (alar plate) and motor (basal plate) regions. In the ventral , Sonic hedgehog (Shh) secreted by the and induced floor plate creates a concentration that promotes ventral fates in a dose-dependent manner. High levels of Shh induce the floor plate and ventral (p3 domain), while lower concentrations specify (pMN domain) and more dorsal domains (p0-p2). This ventralizing signal acts by repressing dorsal genes and activating ventral-specific transcription factors through Gli mediator proteins. Dorsalization occurs via bone morphogenetic protein (BMP) signaling from the roof plate and overlying , antagonized by secreted inhibitors such as chordin and dickkopf (Dkk). BMPs promote dorsal progenitor identities, including those expressing Pax7 in the alar plate, while chordin binds and sequesters BMPs to refine the gradient and prevent ectopic ventralization. The interplay of Shh and BMP gradients ensures sharp boundaries between domains, with intermediate regions like the p2 domain influenced by balanced signaling. Progenitor domains are defined by cross-repressive networks of transcription factors that interpret these gradients. Dorsally, Pax7 marks sensory progenitors; intermediately, Irx3 delineates the p2/p1 boundary; and ventrally, Nkx2.2 specifies the p3 domain adjacent to the floor plate. Gradient interpretation involves planar diffusion of Shh within the neuroepithelium, allowing direct signaling across cells, and regulation of proliferation via phospho-histone H3 (pH3) marking, where high Shh sustains mitotic activity in ventral progenitors. Planar cell polarity signaling further coordinates tissue alignment to facilitate uniform gradient propagation and domain organization. In humans, defects in the Shh pathway, including mutations in the SHH gene, disrupt dorsoventral patterning and are a primary cause of , a severe midline malformation characterized by incomplete division. These mutations attenuate Shh signaling, leading to ventral deficits and fused cerebral hemispheres, highlighting the pathway's conserved role in neural axis formation.

Neurogenesis and Proliferation

Neural Progenitor Dynamics

Neural progenitors, primarily radial glial cells and intermediate progenitor cells, reside in specialized germinal zones during embryonic development, where they undergo proliferative divisions to expand the progenitor pool and generate neurons over time. The ventricular zone (VZ), lining the neural tube's lumen, serves as the primary site of early , housing apical progenitors that contact both the ventricular surface and the via radial processes. Adjacent to the VZ, the (SVZ) emerges later as a secondary germinal layer, particularly prominent in the developing telencephalon, containing basal progenitors that contribute to increased neuronal output in gyrencephalic brains like humans. These zones enable spatiotemporal control of , with progenitors transitioning from proliferative to differentiative states to build neural circuits. Progenitor proliferation involves a balance between symmetric and asymmetric cell divisions, regulated by signaling pathways that maintain stemness while allowing timely production. Symmetric divisions, which produce two s, predominate early to expand the pool, whereas asymmetric divisions generate one and one or intermediate , depleting the reservoir over time. The Notch/Delta pathway critically governs this balance: Delta-like ligands on differentiating daughter cells activate Notch receptors on neighboring s, promoting their maintenance through transcriptional repression of proneural genes like Neurogenin, thus favoring symmetric or self-renewing outcomes. Inhibition of Notch, conversely, drives asymmetric divisions by allowing proneural factor expression, ensuring progressive without premature exhaustion of the pool. Cell cycle dynamics further fine-tune progenitor behavior, with regulators enforcing quiescence or proliferation to match developmental demands. , a G1-phase cyclin, drives progenitor expansion by shortening the and promoting symmetric divisions; its overexpression in mouse models increases intermediate progenitor numbers and cortical thickness, highlighting its role in scaling neuronal production. Conversely, the cyclin-dependent kinase inhibitor p27Kip1 enforces quiescence in adult-like neural stem cells, restraining entry into the ; p27Kip1 knockout in hippocampal progenitors leads to excessive proliferation and disrupted , underscoring its necessity for temporal gating of activation during development. This regulated proliferation results in a temporal progression of , where early divisions yield deep-layer neurons (e.g., layers 5/6 in the cortex), and later ones produce superficial layers (layers 2/3), establishing an inside-out laminar pattern. In the mammalian , this birthdate-dependent sequence ensures older neurons occupy deeper positions while younger ones migrate past them to form upper layers, a process conserved across but amplified in for expanded cortical surface area.

Cell Fate Determination

Cell fate determination in the developing nervous system refers to the processes by which neural cells commit to specific lineages, such as or , and further differentiate into distinct neuronal subtypes. This commitment is orchestrated by a balance of intrinsic genetic programs and extrinsic signaling cues, ensuring the generation of diverse cell types required for assembly. During early , progenitors preferentially produce neurons, but temporal shifts enable subsequent gliogenesis, with subtype identities emerging through networks that interpret positional and temporal information. Intrinsic factors, particularly proneural basic helix-loop-helix (bHLH) such as Neurogenin 2 (Neurog2) and Achaete-scute family bHLH 1 (Ascl1), play a pivotal role in promoting over gliogenesis. These factors activate neuronal differentiation genes while repressing glial fates in neural progenitors, thereby driving the initial wave of neuron production in regions like the and . For instance, Neurog2 and Ascl1 co-expression in cortical progenitors establishes landscapes that favor neuronal subtype identities, highlighting their function in both fate choice and diversification. Loss of these proneural genes results in reduced and premature gliogenesis, underscoring their essential role in timing fate decisions. Following the neurogenic phase, extrinsic signals shift progenitors toward glial fates, with cytokines like (LIF) and ciliary neurotrophic factor (CNTF) acting as key inducers of astrogliogenesis. These factors activate the in cortical progenitors, promoting astrocytic differentiation while inhibiting neuronal production, thus coordinating the transition from to gliogenesis in late embryonic and early postnatal stages. This extrinsic regulation ensures that gliogenesis occurs after sufficient neurons have been generated, maintaining developmental balance. For neuronal subtype specification, transcription factors such as Fezf2 and Lhx2 direct progenitors toward specific identities within the cortex. Fezf2 acts as a selector in deep-layer progenitors, regulating sets that define corticospinal identity, including axonal projection patterns to subcortical targets. In contrast, Lhx2 functions as a cortical selector, maintaining neocortical identity in progenitors and suppressing alternative fates like hippocampal organizer development, thereby ensuring proper laminar and areal organization of cortical neurons. Recent advances in single-cell RNA sequencing (scRNA-seq) have illuminated the vast diversity of neuronal subtypes arising from stem cell-derived progenitors. In a 2025 study from , researchers used scRNA-seq-coupled patterning screens on human induced pluripotent stem cells to generate and characterize over 400 distinct neuronal subtypes, far exceeding prior efforts and providing a comprehensive atlas for modeling human neural development and disease. This approach revealed how combinatorial overexpression and signaling recapitulate subtype diversification, offering new insights into fate determination mechanisms.

Neuronal Migration

Radial Migration

Radial migration is a critical process in the development of the , where newly generated projection neurons ascend from the ventricular and subventricular zones along radial glial scaffolds to establish the six-layered architecture. This migration ensures that neurons destined for superficial layers pass through those fated for deeper layers, forming an inside-out pattern of cortical lamination. Radial , which span from the ventricular surface to the pial surface, serve as guiding fibers, providing both structural support and molecular cues for neuronal positioning. Two primary modes characterize radial migration: glia-guided locomotion and somal translocation. In glia-guided locomotion, extend a leading process that attaches to the radial glial fiber, followed by nucleokinesis where the soma advances along the process in a climbing manner, enabling rapid traversal of the cortical wall. This mode predominates for migrating longer distances to deeper cortical layers. In contrast, somal translocation involves the extending a thin process to the pial surface while the soma pulls itself upward along this process, often in closer association with radial glia but with less direct adhesion; this mode is more common for shorter migrations to superficial layers. Both modes rely on dynamic cytoskeletal rearrangements, including in the leading process and microtubule organization for somal movement. The termination of radial migration at appropriate laminar positions in the cortical plate is regulated by Reelin signaling. Reelin, a large extracellular secreted by Cajal-Retzius cells in the marginal zone, binds to lipoprotein receptors ApoER2 and VLDLR on migrating neurons, recruiting the adaptor protein Disabled-1 (Dab1). Phosphorylation of Dab1 by Src family kinases activates downstream pathways, including inhibition of actin depolymerization via cofilin phosphorylation, which detaches neurons from radial glia and halts their ascent as a "stop" signal upon entering the Reelin-rich zone. VLDLR primarily mediates this detachment in the cortical plate, while ApoER2 supports earlier phases of migration orientation. In the human , radial migration is dominant during cortical layering from approximately gestational weeks 8 to 20, coinciding with peak and the expansion of the cortical plate. Disruptions in this process, such as biallelic mutations in the gene encoding , lead to with , characterized by a smooth cerebral surface due to failed neuronal layering and inverted cortical architecture. These defects highlight Reelin's essential role in precise laminar organization.

Tangential and Other Modes

Tangential migration represents a distinct mode of neuronal movement in the developing , characterized by displacement parallel to the pial surface rather than perpendicular to it, allowing neurons to travel long distances from their origins to distant cortical regions. This process is essential for populating the cortex with specific neuronal subtypes, particularly those originating outside the . Cajal-Retzius cells, which arise from the cortical hem and play a key role in cortical lamination, undergo tangential migration guided by meningeal-derived signals. Specifically, the CXCL12 (also known as SDF-1) secreted by the acts through the receptor on these cells to direct their stream-like movement into the . Disruption of this CXCL12/CXCR4 pathway leads to impaired distribution of Cajal-Retzius cells, highlighting its precision in controlling their tangential paths. GABAergic interneurons, which originate in the subpallium (including the medial and caudal ganglionic eminences), similarly rely on tangential migration via dedicated streams to reach the cortex, contributing to inhibitory circuitry. These navigate through multiple zones, including the and marginal zone, using a combination of attractive and repulsive cues. The Slit proteins, secreted from sites like the and ventral midline, bind Robo receptors on migrating to provide chemorepulsive guidance, preventing ectopic invasion into non-target areas and shaping their trajectories.80801-6) Complementing this, /CXCR4 signaling attracts toward the cortex while repelling them from certain barriers, ensuring efficient colonization of cortical layers. Studies in models demonstrate that loss of Slit/Robo function results in disorganized interneuron streams and reduced cortical inhibition, underscoring the pathway's impact on network assembly. Beyond tangential streams, axophilic migration involves neurons following pioneer axons as scaffolds, a mode prominent in the . In the developing , (GnRH) neurons originate in the nasal placode and migrate centrally along bundles of olfactory sensory axons, using them as physical guides to reach the . This axon-dependent pathfinding ensures proper positioning for reproductive neuroendocrine functions, with disruptions in axon-neuron adhesion molecules like DCC leading to migration defects and associated disorders such as . Multipolar migration serves as an intermediate mode during radial neuronal ascent, where post-mitotic neurons in the intermediate zone adopt a multipolar morphology, extending multiple short processes to probe the environment before transitioning to directed locomotion. This phase allows neurons to extend axons while navigating the subplate and intermediate zone, facilitating initial polarity establishment prior to the radial phase along glial fibers. Unlike pure tangential or radial modes, multipolar migration involves dynamic centrosomal reorientation and process retraction, enabling neurons to cover lateral distances en route to their laminar destinations. Recent advances reveal that glia-neuron interactions via components critically regulate multipolar transitions. Radial glial cells secrete tenascin-C, which assembles with neuron-derived neurocan and hyaluronan in the subplate/intermediate zone to form a supportive scaffold, promoting the shift from multipolar to bipolar morphology essential for subsequent radial migration. In models, disruption of this ternary complex impairs the transition, resulting in delayed neuronal polarity and cortical layering, as observed between embryonic days 14.5 and 17.5.

Differentiation and Connectivity

Neurotrophic Support

Neurotrophic factors play a crucial role in sustaining neuronal survival and promoting differentiation after migration during development. These factors, primarily the family, include (NGF), (BDNF), (NT-3), and neurotrophin-4 (NT-4), which bind with high affinity to specific receptors: NGF to TrkA, BDNF and NT-4 to TrkB, and NT-3 predominantly to TrkC, though with some cross-reactivity. Activation of these triggers intracellular signaling cascades, such as the MAPK/ERK and PI3K/Akt pathways, that enhance neuronal survival, growth, and maturation. Additionally, the p75 neurotrophin receptor (p75NTR), a low-affinity pan-neurotrophin receptor, modulates Trk signaling by facilitating binding and receptor trafficking, while also independently promoting in the absence of Trk activation through pathways involving JNK and . A key mechanism of neurotrophic support is target-derived , where secreted by target tissues bind to axonal terminals, are internalized into signaling endosomes, and transported retrogradely to the cell body to prevent . This process ensures that only neurons successfully innervating appropriate targets receive sufficient trophic support, thereby refining neural circuits. For instance, in sympathetic and sensory neurons, NGF-TrkA signaling complexes are retrogradely transported via motors, activating anti-apoptotic genes like upon reaching the soma. Disruption of this retrograde transport, as seen in models with blocked endosomal signaling, leads to increased , underscoring its essential role in development. The dosage effects of are critical, as their limited availability from target tissues creates competition among innervating neurons, resulting in the selective survival of approximately 50% of the neuronal population during development. This phenomenon, central to the neurotrophic theory proposed by and , explains naturally occurring in vertebrates, where excess neurons are generated and culled based on trophic factor scarcity to match target size. Experimental supplementation of , such as BDNF or NT-3, can rescue a significant portion of these dying neurons, confirming the dosage-dependent nature of survival. In humans, variations in neurotrophic factor genes, particularly BDNF polymorphisms like Val66Met (rs6265), have been implicated in neurodevelopmental disorders by altering BDNF secretion and TrkB signaling efficiency. The Met allele reduces activity-dependent BDNF release, potentially disrupting neuronal maturation and , and is associated with increased risk for conditions such as autism spectrum disorder, , and attention-deficit/hyperactivity disorder. These genetic insights highlight the translational relevance of neurotrophic mechanisms to clinical neurodevelopment.

Axon Pathfinding

Axon pathfinding refers to the process by which extending neuronal navigate to their appropriate targets during development, primarily guided by molecular cues that influence behavior. These cues include secreted chemoattractants and repellents that create gradients to direct axon orientation, as well as contact-mediated signals from surrounding cells and . The , a dynamic structure at the axon tip, senses these cues through specific receptors, leading to cytoskeletal rearrangements that promote attraction, repulsion, or stabilization. Key among these are the netrin family of secreted proteins, which act as bifunctional guidance molecules. Netrin-1, expressed by floor plate cells in the ventral , attracts commissural axons via binding to the receptor DCC (deleted in colorectal ), promoting anterograde extension toward the midline. In contrast, when netrin-1 binds to UNC5 family receptors (such as UNC5A-D), it elicits repulsion, as seen in trochlear motor axons that are diverted away from the floor plate. This dual functionality allows netrins to shape axonal trajectories in both attractive and repulsive contexts. Slit proteins, secreted from midline structures like the floor plate, function primarily as repellents to prevent inappropriate midline recrossing by post-commissural axons. They bind to (Robo) receptors (Robo1-3 in mammals), activating downstream signaling that collapses s and inhibits adhesion. Robo receptors exhibit combinatorial expression, with higher levels of Robo1 and Robo2 correlating with stronger repulsion to position axons laterally away from the midline. Semaphorins, a diverse family of secreted and transmembrane proteins, typically mediate repulsion through Plexin receptors, often in complex with co-receptors like neuropilins. For instance, semaphorin-3A (Sema3A) binds Plexin-A1 and neuropilin-1 on sensory and cortical axons, inducing collapse and directing avoidance of inhibitory zones. Transmembrane semaphorins, such as Sema4D, signal via Plexin-B1 to regulate fascicle branching and target selection in the . Ephrins and their Eph receptors provide bidirectional signaling for topographic mapping, particularly in retinotectal projections. Ephrin-A ligands, expressed in gradients in the , bind EphA receptors on axons, eliciting repulsion that refines temporal-nasal mapping; higher ephrin-A levels in posterior colliculus terminate temporal axons. Ephrin-B and EphB interactions similarly guide dorsoventral projections, with reverse signaling in ephrins promoting adhesion or attraction in certain contexts. In addition to diffusible cues, pioneer axons— the first to extend in a tract—lay down pathways that subsequent follower axons follow through , mediated by molecules (CAMs). NCAM () promotes homophilic adhesion between axons, stabilizing bundles in the and spinal tracts. L1-CAM similarly drives via homophilic and heterophilic interactions, as demonstrated in cerebellar and cortical projections where L1 mutants exhibit defasciculated axons. Commissural axons in the spinal cord exemplify integrated guidance, particularly during floor plate crossing. These axons are initially insensitive to Slit repulsion due to expression of Robo3 (also known as Rig-1), which suppresses Robo1/2 signaling and allows midline entry. Post-crossing, Robo3 downregulation enables Slit-mediated repulsion, directing axons ventrally away from the midline. Recent advances using human stem cell-derived organoids have highlighted species-specific aspects of axon pathfinding. In 2025, midline assembloids—fusions of floor plate and spinal cord organoids from the Pasca laboratory—modeled commissural axon guidance and robust floor plate crossing in humans, identifying human-enriched regulators of midline crossing including netrin-1 secretion and SHH-mediated ventral patterning. These models underscore human-specific molecular dynamics in guidance, with implications for neurodevelopmental disorders.

Synaptogenesis

Peripheral Synapses

The development of peripheral synapses, exemplified by the (NMJ), represents a paradigmatic model for synapse formation in the peripheral , where axons connect with fibers to enable voluntary movement. This process involves coordinated signaling between presynaptic and postsynaptic elements to establish functional transmission. Central to this is the agrin-MuSK-LRP4 pathway, which orchestrates postsynaptic differentiation. Agrin, a secreted by axons, binds to receptor-related protein 4 (LRP4) on the surface, thereby recruiting and activating muscle-specific (MuSK), a . This ternary complex formation induces downstream signaling that clusters acetylcholine (AChRs) at the postsynaptic membrane, essential for synaptic efficacy. LRP4 acts as the primary agrin receptor, enhancing MuSK dimerization and , which in turn activates intracellular adapters like Dok-7 to promote AChR aggregation via rapsyn. Disruption of this pathway, as seen in LRP4 or MuSK models, abolishes AChR clustering and prevents NMJ formation. NMJ synaptogenesis proceeds through sequential steps initiated by axon-muscle contact. Motor axons first reach pre-patterned AChR clusters on immature muscle fibers around embryonic day 12.5–14.5 in mice, stabilizing central clusters while dispersing peripheral ones. Upon contact, presynaptic differentiation follows, with axons releasing agrin and other factors to form active zones, accumulate synaptic vesicles, and initiate (ACh) release; this is supported by ensheathment and neuregulin signaling from the axon. Postsynaptic maturation then ensues, involving AChR clustering, of the muscle into junctional folds, and transcriptional upregulation of synaptic genes in nearby nuclei, leading to a mature endplate structure. In mice, functional NMJs capable of evoked transmission emerge by embryonic day 18, as evidenced by electrophysiological recordings of endplate potentials and muscle contractions in response to stimulation. These early synapses support fetal movements, with further refinement occurring postnatally through synapse elimination and stabilization. Mutations in the MuSK gene underlie rare forms of congenital myasthenic syndromes (CMS), characterized by impaired NMJ function, fatigable weakness, ptosis, and respiratory distress from birth. These loss-of-function variants reduce MuSK kinase activity and AChR clustering, leading to defective synaptic transmission; for instance, the p.Arg333Gln mutation diminishes protein stability and signaling. Treatment often involves acetylcholinesterase inhibitors or 3,4-diaminopyridine to enhance ACh availability. This peripheral model shares mechanistic parallels with central synapse assembly, such as reliance on for maturation, though NMJ formation emphasizes agrin-dependent clustering over neuronal- neuronal interactions.

Central Synapse Assembly

Central synapse assembly in the (CNS) involves the coordinated formation of excitatory and inhibitory synapses between diverse neuronal types, establishing functional neural circuits during development. This process begins with initial axonal-dendritic contacts in the late embryonic period and progresses through molecular recognition, stabilization, and maturation of presynaptic and postsynaptic specializations. molecules play a pivotal role in conferring specificity, while activity-dependent mechanisms ensure long-term viability of these connections. Unlike the highly stereotyped neuromuscular junctions in the periphery, CNS synapses exhibit remarkable diversity in structure and function, adapting to the brain's complex wiring requirements. The process intensifies postnatally, peaking in . Key adhesion molecules, such as neurexins and neuroligins, mediate trans-synaptic interactions that drive specification. Presynaptic neurexins, expressed on axons, bind extracellularly to postsynaptic neuroligins on dendrites, triggering bidirectional differentiation: neuroligins induce presynaptic vesicle clustering and active zone assembly, while neurexins promote postsynaptic receptor recruitment. enhances specificity; for s, neuroligin-1 with an insert at splice site B (+B) pairs preferentially with β-neurexins lacking an insert at site 4 (−S4), recruiting and NMDA receptors. In contrast, neuroligin-2 (−B) and β-neurexins with a site 4 insert (+S4) favor inhibitory synapses by enhancing clustering, with neuroligin-2 knockdown reducing inhibitory postsynaptic currents by approximately 40–50%. Complementing this, transmembrane proteins (LRRTMs), particularly LRRTM1 and LRRTM2, bind neurexins (−S4 variants) in a calcium-dependent manner to promote excitatory synapse density, competing with neuroligin-1 for binding sites and synergistically boosting PSD-95 recruitment for postsynaptic organization. Presynaptic maturation relies on synaptotagmin-1, which couples calcium influx to , ensuring rapid release essential for functionality. Localized at the active zone via interactions with RIM proteins, synaptotagmin-1's C2 domains bind Ca²⁺ within milliseconds, clamping SNARE complexes (synaptobrevin, syntaxin-1, SNAP-25) until triggered, thus synchronizing vesicle fusion with action potentials during early circuit assembly. Postsynaptically, PSD-95 serves as a core scaffolding protein in the postsynaptic density (PSD), anchoring glutamate receptors and signaling molecules to stabilize nascent contacts. Overexpression of PSD-95 increases spine density and PSD area by approximately 2- to 3-fold, promoting multi-innervated spines through nitric oxide synthase interactions that drive presynaptic differentiation via cGMP signaling. Activity-dependent Hebbian mechanisms further refine assembly by stabilizing correlated pre- and postsynaptic firing. Long-term potentiation (LTP)-like processes strengthen active synapses through NMDA receptor activation and calcium influx, while long-term depression (LTD) weakens inactive ones, preventing network instability during development. This "cells that fire together wire together" principle, balanced by homeostatic adjustments, ensures selective retention of functional contacts. Recent advances in human cerebral organoids from induced pluripotent stem cells have enabled modeling of diverse neuronal cell types, including multiple excitatory and inhibitory subtypes forming functional synapses, recapitulating Alzheimer's disease pathologies like amyloid-β accumulation and synaptic loss for therapeutic screening. These organoid models highlight cell-type-specific synapse vulnerabilities in neurodegenerative contexts, bridging in vitro assembly studies with disease mechanisms.

Circuit Refinement

Synapse Elimination

Synapse elimination, also known as synaptic pruning, is a critical developmental process that refines neural circuits by selectively removing excess synaptic connections formed during earlier stages of synaptogenesis. This activity-dependent mechanism ensures that stronger, more functional inputs are preserved while weaker or inappropriate ones are withdrawn, optimizing circuit efficiency and specificity. In the central nervous system, pruning occurs postnatally and involves competitive interactions among synapses, where heightened neuronal activity promotes the survival of active connections and tags less active ones for elimination. The process is mediated by the complement cascade, where proteins such as C1q and C3 tag synapses for removal based on their relative strength. During activity-dependent competition, weaker synapses are opsonized by C1q, which initiates the and leads to C3 deposition, marking them as targets for . , the brain's resident immune cells, recognize these complement-tagged synapses via receptors like CR3 and engulf them through phagocytic processes, thereby sculpting refined connectivity. This mechanism was first demonstrated in the developing retinogeniculate pathway, where C1q and C3 are essential for eliminating polyinnervated synapses onto relay neurons. Synapse elimination follows a temporally regulated timeline, with peaks occurring during in humans, when synaptic density declines sharply after reaching a maximum in . For instance, in the retinogeniculate system of , refinement begins perinatally and intensifies around eye opening (postnatal days 10-20), driven by spontaneous and sensory-evoked activity to segregate eye-specific inputs. This extends into across cortical regions, reducing overall numbers by up to 50% to support mature circuit function. Disruptions in this process, such as excess retention of synapses, are implicated in neurodevelopmental disorders like autism spectrum disorder (ASD), where postmortem studies reveal elevated synaptic density in prefrontal and temporal cortices, potentially due to impaired microglial . Recent research has highlighted the role of glia-glia signaling in coordinating during critical periods. A 2025 study identified intercellular pathways between and that enhance experience-dependent elimination, where neuronal activity triggers glial signaling to amplify phagocytic efficiency and refine circuits. This glia-glia communication integrates with complement tagging to ensure precise removal of surplus synapses, underscoring the collaborative role of non-neuronal cells in neural development.

Activity-Dependent Mapping

Activity-dependent mapping refers to the process by which patterned neural activity refines the topographic and functional connectivity of neural circuits during development, ensuring precise alignment between sensory inputs and cortical representations. This refinement occurs through mechanisms that strengthen or weaken synapses based on the temporal correlation of neuronal firing, integrating molecular guidance cues with experience-driven signals to sculpt circuit . Such mapping is essential for establishing sensory maps that mirror the spatial arrangement of the periphery, as disruptions in activity patterns lead to disorganized projections and impaired . A key mechanism underlying activity-dependent mapping is spike-timing-dependent plasticity (STDP), where the precise timing of presynaptic and postsynaptic spikes determines synaptic modification. In STDP, if a presynaptic neuron fires shortly before the postsynaptic neuron (within ~20 ms), the synapse undergoes (LTP), strengthening the connection; conversely, postsynaptic firing preceding presynaptic activity induces long-term depression (LTD), weakening it. This Hebbian-like rule, first demonstrated in cultured hippocampal neurons, promotes the clustering of correlated inputs and the segregation of uncorrelated ones, thereby refining topographic maps by reinforcing activity-synchronized pathways. Topographic maps, such as in the , emerge through the interplay of molecular gradients and activity patterns. Retinotopic mapping relies on countergradients of EphA receptors in retinal ganglion cells and ephrin-A ligands in target structures like the , which provide topographic guidance by repelling axons in a concentration-dependent manner; however, spontaneous —correlated bursts of activity during early postnatal stages—further refine these maps by driving activity-dependent competition for target space. Similarly, somatotopic maps in the somatosensory cortex, exemplified by organization representing individual , are initially guided by thalamocortical afferents but refined by sensory-evoked activity that stabilizes columnar arrangements and eliminates ectopic connections. Critical periods represent discrete windows when neural circuits are particularly sensitive to activity for wiring refinement, such as in thalamocortical projections where spontaneous waves of activity propagate from sensory periphery to cortex, instructing map alignment. In the , waves during the first two postnatal weeks in drive the segregation of eye-specific inputs in the and sharpen retinotopic maps via NMDA receptor-dependent plasticity; analogous waves in the somatosensory organize barrel patterns by synchronizing whisker-related inputs. These periods close as inhibitory circuits mature, limiting further plasticity. In humans, (fMRI) reveals activity-driven maturation of organization, with topographic maps emerging in infancy and refining through sensory experience during early childhood. Resting-state fMRI studies show that functional connectivity in ventral visual areas strengthens with age, correlating with behavioral improvements in , while task-based fMRI during critical periods demonstrates heightened plasticity, as seen in cross-modal reorganization following early . These findings underscore how patterned activity shapes human cortical maps, with implications for developmental disorders.

Glial Development

Macroglia Formation

Macroglia, comprising , , and ependymal cells, arise during gliogenesis, a process that temporally follows in the developing . This sequential progression ensures the establishment of neural circuits before glial support structures form, with gliogenesis primarily occurring in late embryonic and early postnatal stages in mammals. The transition is regulated by key transcription factors, including for astrocyte differentiation and Olig2 for lineage specification. activation, often triggered by cytokines like (LIF), binds to the GFAP promoter to initiate astrogliogenesis, while Olig2 promotes the commitment of progenitors to the fate by repressing neuronal genes and activating myelin-related pathways. Radial glia serve as the primary progenitors for macro, undergoing transformation to generate , , and ependymal cells. These multipotent cells, initially focused on , shift competence during mid-to-late gestation; some directly differentiate into astrocytes through processes involving STAT3-mediated epigenetic changes that demethylate glial genes, while others transform into ependymal cells lining the ventricles, with maturation continuing postnatally. For , radial glia produce intermediate progenitors that further specify into oligodendrocyte precursor cells (OPCs), a lineage progression marked by Olig2 expression. This dual potential highlights radial glia's role in diversifying the glial population to support neuronal migration, , and eventual circuit maturation. Oligodendrocytes contribute to myelination, a critical aspect of macroglial function, where OPCs migrate extensively along axons before differentiating and wrapping lipid-rich membranes around them. This process is tightly controlled by Sox10, a that drives OPC maturation, gene expression (such as MBP and PLP1), and the formation of compact sheaths, ensuring efficient axonal conduction. Defects in Sox10 disrupt OPC wrapping and lead to hypomyelination, underscoring its essential role. While much research emphasizes rodent models, human macroglia formation exhibits distinct timing, with significant maturation and myelination occurring between 20 and 40 weeks of —a period often underemphasized in comparative studies. This late gestational surge aligns with rapid expansion and supports the unique protracted development of the . may briefly interact with these progenitors to modulate their proliferation, though detailed mechanisms remain under investigation.

Microglia Involvement

Microglia, the resident immune cells of the (CNS), originate from primitive macrophages that emerge in the during early embryonic development. These progenitors, derived from erythro-myeloid precursors, colonize the CNS around embryonic day 9.5 in mice, establishing a self-renewing population independent of contributions postnatally. This early infiltration supports microglial roles in and circuit maturation before the formation of the blood-brain barrier. During neural development, contribute to circuit refinement through , particularly mediated by the CX3CR1 receptor. CX3CR1, expressed on , binds to neuronal fractalkine (), enabling recognition and engulfment of less active synapses, which is essential for establishing mature connectivity in regions like the hippocampus. In CX3CR1-deficient models, synaptic density remains elevated postnatally, leading to impaired functional connectivity and social behavior deficits. Beyond , provide trophic support by releasing (BDNF), which promotes formation and neuronal plasticity during learning-dependent remodeling. Microglial BDNF enhances TrkB in neurons, facilitating structural changes in dendritic spines and supporting experience-driven circuit assembly. Recent advances highlight glia-glia signaling in experience-dependent , where interact with via Wnt pathways to regulate synaptic elimination during critical periods. This crosstalk, involving microglial engulfment of astrocytic processes, modulates glutamate clearance and synaptic strength in response to sensory input, as observed in visual and olfactory circuits. Such mechanisms underscore microglia's role in activity-dependent refinement, potentially referencing macroglial scaffolds for positional guidance without direct involvement in myelination. Dysfunction in microglial development and signaling is implicated in neurodevelopmental disorders like , where altered (excessive) contributes to reduced synaptic connectivity and cognitive impairments. Postmortem studies reveal microglial and reduced trophic support in brains, linking early yolk sac-derived colonization deficits to disrupted circuit maturation during adolescence. Genetic variants affecting CX3CR1 pathways exacerbate these effects, highlighting as a therapeutic target for preventing synaptic imbalances.

Adult Neurogenesis

Germinal Zones

Adult neurogenesis persists in specific germinal zones of the mammalian , primarily the (SVZ) lining the and the subgranular zone (SGZ) in the of the hippocampus. These niches serve as reservoirs for neural stem cells that generate new neurons throughout life, contributing to plasticity and repair. The SVZ produces neuroblasts that migrate to the , while the SGZ generates granule cells that integrate into hippocampal circuits. Within the SVZ, the neurogenic lineage begins with type B cells, which are quiescent neural stem cells exhibiting astrocyte-like characteristics and expressing (GFAP). These type B cells asymmetrically divide to produce type C transit-amplifying progenitors, which are highly proliferative and express (EGFR). Type C cells then generate type A neuroblasts, immature neurons that migrate tangentially through the rostral migratory stream. In the SGZ, analogous populations include quiescent radial glia-like stem cells (type 1), transit-amplifying intermediate progenitors (type 2), and neuroblasts (type 3), though nomenclature aligns closely with the SVZ . Regulation of proliferation in these zones involves extrinsic and intrinsic factors. Physical exercise enhances by increasing progenitor proliferation in both the SVZ and SGZ, potentially through elevated levels of (BDNF) and (VEGF). Wnt/β-catenin signaling similarly promotes proliferation, as its activation in neural s upregulates expression and progression, counteracting inhibitory signals like secreted frizzled-related protein 3 (sFRP3). Conversely, aging diminishes via chronic low-grade , where pro-inflammatory cytokines such as interleukin-6 (IL-6) and tumor necrosis factor-alpha (TNF-α) from activated suppress activation and survival. Species differences highlight variations in adult neurogenesis robustness. In rodents, these processes are prolific, with thousands of new neurons added daily to the hippocampus and , supporting robust plasticity. In s, evidence from dating of genomic DNA indicates ongoing into adulthood, albeit at much lower rates—approximately 700 new neurons per day in young adults, declining sharply with age—though a 2025 genetic study further confirms ongoing hippocampal neurogenesis into late adulthood; detection in the SVZ remains more contentious. These findings underscore the need for cautious extrapolation from models to .

Functional Integration

New neurons generated in the adult (SVZ) migrate tangentially along the rostral migratory stream (RMS) toward the , where they differentiate into granule cells and periglomerular that integrate into local circuits. This chain-like migration, guided by such as and supported by forming a scaffold, allows neuroblasts to travel up to several millimeters daily while avoiding aberrant integration into surrounding brain tissue. Upon reaching the , these cells disperse radially, extend dendrites to glomeruli, and form synaptic connections with mitral and tufted cells, contributing to odor processing within weeks of arrival. In contrast, neurons born in the subgranular zone (SGZ) of the hippocampal undergo local integration without long-distance migration, maturing into granule cells that extend axons via the mossy fiber pathway to the CA3 region. This process involves radial migration over short distances, followed by dendritic arborization in the molecular layer and axonal that establishes excitatory synapses with pyramidal neurons and . Adult-born granule cells in the SGZ display heightened plasticity during a critical 4-6 week window, forming more synapses per than their developmentally born counterparts, which facilitates their incorporation into the trisynaptic hippocampal circuit. The of these adult-born neurons is highly activity-dependent, with approximately 50-80% undergoing if deprived of sensory or environmental stimulation during early maturation. In the hippocampus, spatial learning or voluntary exercise enhances by activating NMDA receptors and promoting dendritic growth, while in the , enrichment similarly boosts integration rates. Mossy from adult-born granule cells further refines this integration, forming recurrent excitatory connections that preferentially target in the dentate hilus, potentially modulating network excitability. Functionally, adult hippocampal neurogenesis supports memory formation and separation, enabling the of similar contexts or events through sparse encoding in the . In the , new enhance odor by refining sensory representations and adapting to novel olfactory environments, as evidenced by impaired fine odor differentiation in models with reduced . These roles underscore the adaptive value of adult in maintaining across sensory and mnemonic domains.

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