RÉSUMÉ
The Florida manatee (Trichechus manatus latirostris) has well-developed keratinized dental pads at the most rostral aspect of their mouth to assist with mastication. This unique development is thought to be an adaptive response to their highly abrasive diets that contain phytoliths and sediments that may accelerate dental wear. In May 2013, two Florida manatees presented with multiple fractures in their inferior dental pads. The fractures were successfully managed with nutritional modifications, dental pad trimming, and vigilant monitoring through behavioral husbandry training. Signs of spontaneous healing were observed as early as 60 days after initial presentation with subsequent full resolution. Although surgical intervention was planned, the spontaneous healing mitigated significant health risks associated with the procedure. To the authors' knowledge, these are the first reported cases of dental pad fractures and their spontaneous healing and resolution in manatees.
Sujet(s)
Trichechus manatus , Animaux , TrichechusRÉSUMÉ
The capabilities of imaging technologies, fluorescent sensors, and optogenetics tools for cell biology are advancing. In parallel, cellular reprogramming and organoid engineering are expanding the use of human neuronal models in vitro. This creates an increasing need for tissue culture conditions better adapted to live-cell imaging. Here, we identify multiple caveats of traditional media when used for live imaging and functional assays on neuronal cultures (i.e., suboptimal fluorescence signals, phototoxicity, and unphysiological neuronal activity). To overcome these issues, we develop a neuromedium called BrainPhys™ Imaging (BPI) in which we optimize the concentrations of fluorescent and phototoxic compounds. BPI is based on the formulation of the original BrainPhys medium. We benchmark available neuronal media and show that BPI enhances fluorescence signals, reduces phototoxicity and optimally supports the electrical and synaptic activity of neurons in culture. We also show the superior capacity of BPI for optogenetics and calcium imaging of human neurons. Altogether, our study shows that BPI improves the quality of a wide range of fluorescence imaging applications with live neurons in vitro while supporting optimal neuronal viability and function.
Sujet(s)
Encéphale/imagerie diagnostique , Encéphale/physiologie , Imagerie diagnostique , Neurones/physiologie , Optogénétique , Potentiels d'action/physiologie , Animaux , Survie cellulaire , Cellules cultivées , Liquide cérébrospinal/métabolisme , Milieux de culture , Fluorescence , Humains , Cellules souches pluripotentes induites/cytologie , Cellules souches pluripotentes induites/métabolisme , Lumière , Réseau nerveux/physiologie , Concentration osmolaire , Rats , Rapport signal-bruit , Synapses/physiologieRÉSUMÉ
Neural crest cells (NCC) migrate extensively in vertebrate embryos to populate diverse derivatives including ganglia of the peripheral nervous system. Little is known about the molecular mechanisms that lead migrating trunk NCC to settle at selected sites in the embryo, ceasing their migration and initiating differentiation programs. To identify candidate genes involved in these processes, we profiled genes up-regulated in purified post-migratory compared with migratory NCC using a staged, macroarrayed cDNA library. A secondary screen of in situ hybridization revealed that many genes are specifically enhanced in neural crest-derived ganglia, including macrophage migration inhibitory factor (MIF), a ligand for CXCR4 receptor. Through in vivo and in vitro assays, we found that MIF functions as a potent chemoattractant for NCC. These results provide a molecular profile of genes expressed concomitant with gangliogenesis, thus, offering new markers and potential regulatory candidates involved in cessation of migration and onset of differentiation.
RÉSUMÉ
The neural crest (NC) is a transient population of embryonic progenitors that are implicated in a diverse range of congenital birth defects and pediatric syndromes. The broad spectrum of NC-related disorders can be attributed to the wide variety of differentiated cell types arising from the NC. In vitro models of NC development provide a powerful platform for testing the relative contributions of intrinsic and extrinsic factors mediating NC differentiation under normal and pathogenic conditions. Although differentiation is a dynamic process that unfolds over time, currently, there is no well-defined chronology that characterizes the in vitro progression of NC differentiation towards specific cell fates. In this study, we have optimized culture conditions for expansion of primary murine NC cells that give rise to both ectodermal and mesoectodermal derivatives, even after multiple passages. Significantly, we have delineated highly reproducible timelines that include distinct intermediate stages for lineage-specific NC differentiation in vitro In addition, isolating both cranial and trunk NC cells from the same embryos enabled us to make direct comparisons between the two cell populations over the course of differentiation. Our results define characteristic changes in cell morphology and behavior that track the temporal progression of NC cells as they differentiate along the neuronal, glial and chondrogenic lineages in vitro These benchmarks constitute a chronological baseline for assessing how genetic or environmental disruptions may facilitate or impede NC differentiation. Introducing a temporal dimension substantially increases the power of this platform for screening drugs or chemicals for developmental toxicity or therapeutic potential. This article has an associated First Person interview with the first author of the paper.
Sujet(s)
Techniques de culture cellulaire/méthodes , Différenciation cellulaire , Crête neurale/cytologie , Crâne/cytologie , Tronc/physiologie , Animaux , Différenciation cellulaire/génétique , Prolifération cellulaire , Auto-renouvellement cellulaire , Forme de la cellule , Cellules cultivées , Chondrocytes/cytologie , Régulation de l'expression des gènes au cours du développement , Souris , Névroglie/cytologie , Neurones/cytologie , Facteurs tempsRÉSUMÉ
Slits ligands and their Robo receptors are involved in quite disparate cell signaling pathways that include axon guidance, cell proliferation, cell motility and angiogenesis. Neural crest cells emerge by delamination from neural cells in the dorsal neural tube, and give rise to various components of the peripheral nervous system in vertebrates. It is well established that these cells change from a non-migratory to a highly migratory state allowing them to reach distant regions before they differentiate. However, but the mechanism controlling this delamination and subsequent migration are still not fully understood. The repulsive Slit ligand family members, have been classified also as true tumor suppressor molecules. The present study explored in further detail what possible Slit/Robo signals are at play in the trunk neural cells and neural crest cells by carrying out a microarray after Slit2 gain of function in trunk neural tubes. We found that in addition to molecules known to be downstream of Slit/Robo signaling, there were a large set of molecules known to be important in maintaining cells in non-motile, epithelia phenotype. Furthermore, we found new molecules previously not associated with Slit/Robo signaling: cell proliferation markers, Ankyrins and RAB intracellular transporters. Our findings suggest that neural crest cells use and array of different Slit/Robo pathways during their transformation from non-motile to highly motile cells.
Sujet(s)
Marqueurs biologiques/métabolisme , Protéines et peptides de signalisation intercellulaire/métabolisme , Protéines de tissu nerveux/métabolisme , Crête neurale/métabolisme , Récepteurs immunologiques/métabolisme , Tronc/physiologie , Animaux , Différenciation cellulaire , Mouvement cellulaire , Prolifération cellulaire , Embryon de poulet , Poulets , Crête neurale/cytologie , Tube neural/cytologie , Tube neural/métabolisme , Transduction du signal ,RÉSUMÉ
BACKGROUND: Lysophospholipids such as lysophosphatidic acid (LPA) and sphingosine-1-phosphate (S1P) are important signaling molecules that can regulate a wide range of cellular responses. We discovered that Sphingosine kinase 1 (Sphk1), a key enzyme that converts sphingosine to S1P, is expressed in neurons and progenitor cells in nascent trigeminal and dorsal root ganglia during mouse embryogenesis. METHODS AND FINDINGS: Sphk1 null mouse embryos do not display overt deficits owing to compensation by Sphk2. Thus, we analyzed embryos that are deficient in both Sphk1 and Sphk2 (which essentially eliminates S1P function) in order to investigate the role(s) of Sphk1 during sensory ganglia formation. While animals lacking 1-3 alleles of Sphk1 and Sphk2 had no obvious phenotype, embryos without both genes displayed clear developmental defects. The complete absence of Sphk1 and Sphk2 resulted in trigeminal and dorsal root ganglia with fewer neurons and progenitor cells. The profound loss in cell number could be attributed to a decrease in cell proliferation as well as an increase in apoptosis. Furthermore, Sphk1/2 double mutants displayed an overall reduction in other sphingolipids as well as an imbalance of S1P/sphingosine and S1P/ceramide ratio, thereby favoring cell death and reducing cell growth. CONCLUSIONS: Together, these results provide strong in vivo evidence that sphingosine kinase/S1P signaling plays an important role in regulating early events during development of sensory ganglia.
Sujet(s)
Ganglions sensitifs/cytologie , Ganglions sensitifs/métabolisme , Lysophospholipides/métabolisme , Neurones/cytologie , Neurones/métabolisme , Phosphotransferases (Alcohol Group Acceptor)/métabolisme , Transduction du signal/physiologie , Sphingosine/analogues et dérivés , Cellules souches/cytologie , Cellules souches/métabolisme , Animaux , Ganglions sensitifs/embryologie , Génotype , Hybridation in situ , Souris , Souches mutantes de souris , Phosphotransferases (Alcohol Group Acceptor)/génétique , Transduction du signal/génétique , Sphingosine/métabolismeRÉSUMÉ
LIN28 is an RNA-binding protein that is expressed in many developing tissues. It can block let-7 (Mirlet7) microRNA processing and help promote pluripotency. We have observed LIN28 expression in the developing mouse neural tube, colocalizing with SOX2, suggesting a role in neural development. To better understand its normal developmental function, we investigated LIN28 activity during neurogliogenesis in vitro, where the succession of neuronal to glial cell fates occurs as it does in vivo. LIN28 expression was high in undifferentiated cells, and was downregulated rapidly upon differentiation. Constitutive LIN28 expression caused a complete block of gliogenesis and an increase in neurogenesis. LIN28 expression was compatible with neuronal differentiation and did not increase proliferation. LIN28 caused significant changes in gene expression prior to any effect on let-7, notably on Igf2. Furthermore, a mutant LIN28 that permitted let-7 accumulation was still able to completely block gliogenesis. Thus, at least two biological activities of LIN28 are genetically separable and might involve distinct mechanisms. LIN28 can differentially promote and inhibit specific fates and does not function exclusively by blocking let-7 family microRNAs. Importantly, the role of LIN28 in cell fate succession in vertebrate cells is analogous to its activity as a developmental timing regulator in C. elegans.
Sujet(s)
Différenciation cellulaire/génétique , microARN/physiologie , Névroglie/physiologie , Protéines de liaison à l'ARN/physiologie , Animaux , Numération cellulaire , Prolifération cellulaire , Cellules cultivées , Séquence conservée/génétique , Séquence conservée/physiologie , Embryon de mammifère , Régulation de l'expression des gènes au cours du développement , Souris , microARN/métabolisme , Tube neural/cytologie , Tube neural/embryologie , Tube neural/métabolisme , Neurogenèse/génétique , Névroglie/cytologie , Névroglie/métabolisme , Structure tertiaire des protéines/physiologie , Protéines de liaison à l'ARN/composition chimique , Protéines de liaison à l'ARN/génétique , Protéines de liaison à l'ARN/métabolismeSujet(s)
Techniques de culture cellulaire/méthodes , Crête neurale/cytologie , Neurones afférents/cytologie , Muscles pectoraux/cytologie , Animaux , Embryon de poulet , Stade de la segmentation de l'oeuf/cytologie , Milieux de culture/pharmacologie , Immunohistochimie/méthodes , Microchirurgie/méthodes , Modèles biologiques , Muscles pectoraux/embryologieSujet(s)
Embryon de poulet , Poulets/génétique , Gènes , Séquençage par oligonucléotides en batterie/méthodes , Animaux , ADN complémentaire/biosynthèse , Traitement automatique des données/méthodes , Analyse de profil d'expression de gènes , Régulation de l'expression des gènes au cours du développement , Banque de gènes , Hybridation d'acides nucléiques , Séquençage par oligonucléotides en batterie/instrumentationRÉSUMÉ
SoxE genes (Sox8, Sox9, and Sox10) are early response genes to neural crest induction. Although the early role of Sox9 has been examined in chick and frog, later roles in neural crest migration and differentiation remain largely unexplored. We first examined which SoxE genes were expressed in trunk neural crest cells and then investigated their function using in ovo electroporation. The results of this analysis reveal that Sox10 is present in migrating neural crest cells, whereas other SoxE genes are only expressed transiently after induction. Ectopic expression of Sox10 in the neural tube at trunk level induced expression of HNK-1 in neuroepithelial cells followed by extensive emigration from all levels of the dorsoventral neuraxis, including the floor plate. Sox10-expressing cells failed to express neuronal, Schwann, or melanocyte markers up to 6 days posttransfection (E8), suggesting these cells were maintained in an undifferentiated state. Overexpression of Sox8 or Sox9 had similar but not identical effects on neuroepithelial cells. These results show that high levels of Sox10, Sox9, or Sox8 expression in the neural tube are capable of inducing a migratory neural crest-like phenotype even in the absence of dorsal signals and can maintain these cells in an undifferentiated state.
Sujet(s)
Différenciation cellulaire , Protéines de liaison à l'ADN/métabolisme , Expression des gènes , Protéines HMG/métabolisme , Crête neurale/cytologie , Crête neurale/métabolisme , Neurones/cytologie , Neurones/métabolisme , Facteurs de transcription/métabolisme , Animaux , Mouvement cellulaire , Embryon de poulet , Protéines de liaison à l'ADN/génétique , Électroporation , Cellules épithéliales/cytologie , Cellules épithéliales/métabolisme , Régulation de l'expression des gènes au cours du développement , Protéines HMG/génétique , Mésoderme/cytologie , Mésoderme/métabolisme , Protéines de répression/génétique , Protéines de répression/métabolisme , Facteurs de transcription SOX-E , Facteurs de transcription/génétiqueRÉSUMÉ
Lineage diversification in the vertebrate neural crest may occur via instructive signals acting on pluripotent cells, and/or via early specification of subpopulations towards particular lineages. Mesencephalic neural crest cells normally form cholinergic parasympathetic neurons in the ciliary ganglion, while trunk neural crest cells normally form both catecholaminergic and cholinergic neurons in sympathetic ganglia. In contrast to trunk neural crest cells, mesencephalic neural crest cells apparently fail to express the catecholaminergic transcription factor dHAND in response to BMPs in the head environment. Here, we show that migrating quail mesencephalic neural crest cells grafted into the trunk of host chick embryos colonise the sympathetic ganglia. While many express dHAND and form tyrosine hydroxylase (TH)-positive catecholaminergic neurons, the proportion that expresses either dHAND or TH is significantly smaller than that of quail trunk neural crest cells under the same conditions. Furthermore, the proportion of quail mesencephalic neural crest cells that is TH+ in the sympathetic ganglia decreases with time, while the proportion of TH+ quail trunk neural crest-derived cells increases. Thus, a subset of mesencephalic neural crest cells fails to express dHAND or TH in the sympathetic ganglia, while a further subset initiates but fails to maintain TH expression. Taken together, our results suggest that a subpopulation of migrating mesencephalic neural crest cells is refractory to catecholaminergic differentiation signals in the trunk. We suggest that this heterogeneity, together with local signals that repress catecholaminergic differentiation, may ensure that most ciliary neurons adopt a cholinergic fate.
Sujet(s)
Ganglions sympathiques/embryologie , Mésencéphale/embryologie , Crête neurale/embryologie , Animaux , Facteurs de transcription à motif basique hélice-boucle-hélice , Transplantation de tissu cérébral , Différenciation cellulaire , Mouvement cellulaire , Embryon de poulet , Coturnix , Protéines de liaison à l'ADN/génétique , Protéines de liaison à l'ADN/métabolisme , Ganglions sympathiques/cytologie , Ganglions sympathiques/métabolisme , Régulation de l'expression des gènes au cours du développement , Protéines à homéodomaine/génétique , Protéines à homéodomaine/métabolisme , Immunohistochimie , Hybridation in situ , Mésencéphale/cytologie , Mésencéphale/métabolisme , Protéines de tissu nerveux , Crête neurale/cytologie , Crête neurale/métabolisme , Transduction du signal , Facteurs de transcription/génétique , Facteurs de transcription/métabolisme , Transplantation hétérologue , Tyrosine 3-monooxygenase/génétique , Tyrosine 3-monooxygenase/métabolisme , Protéines de poisson-zèbreRÉSUMÉ
The chick ciliary ganglion is a neural crest-derived parasympathetic ganglion that innervates the eye. Here, we examine its axial level of origin and developmental relationship to other ganglia and nerves of the head. Using small, focal injections of DiI, we show that neural crest cells arising from both the caudal half of the midbrain and the rostral hindbrain contribute to the ciliary as well as the trigeminal ganglion. Precursors to both ganglia have overlapping migration patterns, moving first ventrolaterally and then rostrally toward the optic vesicle. At the level of the midbrain/forebrain junction, precursors to the ciliary ganglion separate from the main migratory stream, turn ventromedially, and condense in the vicinity of the rostral aorta and Rathke's pouch. Ciliary neuroblasts first exit the cell cycle at early E2, prior to and during ganglionic condensation, and neurogenesis continues through E5.5. By E3, markers of neuronal differentiation begin to appear in this population. By labeling the ectoderm with DiI, we discovered a new placode, caudal to the eye and possibly contiguous to the trigeminal placode, that contributes a few early differentiating neurons to the ciliary ganglion, oculomotor nerve, and connecting branches to the ophthalmic nerve. These results suggest for the first time a dual neural crest and placodal contribution to the ciliary ganglion and associated nerves.
Sujet(s)
Embryon de poulet/cytologie , Corps ciliaire/innervation , Ganglions parasympathiques/embryologie , Crête neurale/physiologie , Nerf oculomoteur/embryologie , Animaux , Différenciation cellulaire , Mouvement cellulaire , Ganglions parasympathiques/cytologie , Mésencéphale/embryologie , Mésoderme/physiologie , Nerf oculomoteur/cytologie , Rhombencéphale/embryologieRÉSUMÉ
In the chick ciliary ganglion, neuronal number is kept constant between St. 29 and St. 34 (E6-E8) despite a large amount of cell death. Here, we characterize the source of neurogenic cells in the ganglion as undifferentiated neural crest-derived cells. At St. 29, neurons and nonneuronal cells in the ciliary ganglion expressed the neural crest markers HNK-1 and p75(NTR). Over 50% of the cells were neurons at St. 29; of the nonneuronal cells, a small population expressed glial markers, whereas the majority was undifferentiated. When placed in culture, nonneuronal cells acquired immunoreactivity for HuD, suggesting that they had commenced neuronal differentiation. The newly differentiated neurons arose from precursors that did not incorporate bromodeoxyuridine. To test whether these precursors could undergo neural differentiation in vivo, purified nonneuronal cells from St. 29 quail ganglia were transplanted into chick embryos at St. 9-14. Subsequently, quail cells expressing neuronal markers were found in the chick ciliary ganglion. The existence of this precursor pool was transient because nonneuronal cells isolated from St. 38 ganglia failed to form neurons. Since all ciliary ganglion neurons are born prior to St. 29, these results demonstrate that there are postmitotic neural crest-derived precursors in the developing ciliary ganglion that can differentiate into neurons in the appropriate environment.
