Amanda K. Wagner scite author profile

Mammalian somatosensory topographic maps contain specialized neuronal structures that precisely recapitulate the spatial pattern of peripheral sensory organs. In the mouse, whiskers are orderly mapped onto several brainstem nuclei as a set of modular structures termed barrelettes. Using a dual-color iontophoretic labeling strategy, we found that the precise topography of barrelettes is not a result of ordered positions of sensory neurons within the ganglion. We next explored another possibility that formation of the whisker map is influenced by periphery-derived mechanisms. During the period of peripheral sensory innervation, several TGF-β ligands are exclusively expressed in whisker follicles in a dynamic spatiotemporal pattern. Disrupting TGF-β signaling, specifically in sensory neurons by conditional deletion of Smad4 at the late embryonic stage, results in the formation of abnormal barrelettes in the principalis and interpolaris brainstem nuclei and a complete absence of barrelettes in the caudalis nucleus. We further show that this phenotype is not derived from defective peripheral innervation or central axon outgrowth but is attributable to the misprojection and deficient segregation of trigeminal axonal collaterals into proper barrelettes. Furthermore, Smad4-deficient neurons develop simpler terminal arbors and form fewer synapses. Together, our findings substantiate the involvement of whisker-derived TGF-β/Smad4 signaling in the formation of the whisker somatotopic maps.O ne prominent characteristic of the rodent whisker-somatosensory system is its precisely organized topographic sensory maps (1-3). Each whisker is innervated by peripheral axons of a subset of trigeminal sensory neurons whose cell bodies reside in the trigeminal ganglia (TG) and central axons project to the brainstem (4). Sensory afferents carrying information from individual whiskers segregate and converge to form modular structures termed barrelettes, whose spatial organization exactly mirrors that of the whiskers in the periphery (5). The barrelette map in the brainstem emerges during development and serves as a template for the subsequent generation of homologous upstream structures in the thalamus and cortex, termed barreloids and barrels, respectively (5, 6). Interestingly, induction of an extra whisker by exogenous expression of Shh during early development leads to the formation of an extra barrelette with a topographic position corresponding to that of the ectopic whisker (7). Together with other studies (8-10), these data suggest that the formation of the whisker map is under the strong instructive influence of the periphery. The whisker-derived signals regulating barrelette formation remain mostly unknown, however.Previous work showed that BMP4 signaling induces differential expression of genes in trigeminal sensory neurons innervating different areas of the face along the dorsoventral axis (11,12). At later developmental stages, multiple TGF-β superfamily ligands are expressed in whisker follicles during the period of sensory...

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A cell-autonomous defect in skeletal muscle satellite cells expressing low levels of survival of motor neuron protein

Hayhurst

Wagner

Cerletti

et al. 2012

Developmental Biology

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Mutations in the Survival of Motor Neuron (SMN) gene underlie the development of spinal muscular atrophy (SMA), which currently represents the leading genetic cause of mortality in infants and toddlers. SMA is characterized by degeneration of spinal cord motor neurons and muscle atrophy. Although SMA is often considered to be a motor neuron disease, accumulating evidence suggests that muscle cells themselves may be affected by low levels of SMN. Here, we examine satellite cells, tissue-resident stem cells that play an essential role in the growth and repair of skeletal muscle, isolated from a severe SMA mouse model (Smn−/−; SMN2+/+). We found similar numbers of satellite cells in the muscles of SMA and wild-type (Smn+/+; SMN2+/+) mice at postnatal day 2 (P2), and, when isolated from skeletal muscle using cell surface marker expression, these cells showed comparable survival and proliferative potential. However, SMA satellite cells differentiate abnormally, revealed by the premature expression of muscle differentiation markers, and, especially, by a reduced efficiency in forming myotubes. These phenotypes suggest a critical role of SMN protein in the intrinsic regulation of muscle differentiation and suggest that abnormal muscle development contributes to the manifestation of SMA symptoms.

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High-throughput fluorescence imaging approaches for drug discovery usingin vitroandin vivothree-dimensional models

Martínez

Titus

Wagner

et al. 2015

Expert Opinion on Drug Discovery

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Introduction High-resolution microscopy using fluorescent probes is a powerful tool to investigate individual cell structure and function, cell subpopulations, and mechanisms underlying cellular responses to drugs. Additionally, responses to drugs more closely resemble those seen in vivo when cells are physically connected in 3D systems (either 3D cell cultures or whole organisms), as opposed to traditional monolayer cultures. Combined, the use of imaging-based 3D models in the early stages of drug development has the potential to generate biologically relevant data that will increase the likelihood of success for drug candidates in human studies. Areas covered The authors discuss current methods for the culturing of cells in 3D as well as approaches for the imaging of whole-animal models and 3D cultures that are amenable to high throughput settings and could be implemented to support drug discovery campaigns. Furthermore, they provide critical considerations when discussing imaging these 3D systems for high throughput chemical screenings. Expert opinion Despite widespread understanding of the limitations imposed by the 2D versus the 3D cellular paradigm, imaging-based drug screening of 3D cellular models is still limited, with only a few screens found in the literature. Image acquisition in high throughput, accurate interpretation of fluorescent signal, and uptake of staining reagents can be challenging, as the samples are in essence large aggregates of cells. The authors recognize these shortcomings that need to be overcome before the field can accelerate the utilization of these technologies in large-scale chemical screens.

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Amanda K. Wagner

Proper formation of whisker barrelettes requires periphery-derived Smad4-dependent TGF-β signaling

A cell-autonomous defect in skeletal muscle satellite cells expressing low levels of survival of motor neuron protein

High-throughput fluorescence imaging approaches for drug discovery usingin vitroandin vivothree-dimensional models

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