Global ETD Search

31	Axonal Regrowth of Olfactory Sensory Neurons After Chemical Ablation and Removal of Axonal Debris by Microglia Chapman, Rudy 01 August 2020 (has links) Olfactory sensory neurons (OSNs) are contained within the olfactory epithelium (OE) and are responsible for detecting odorant molecules in the air. The exposure of OSNs to the external environment is necessary for their function, but it also leaves them exposed to potentially harmful elements and thus results in a high turnover rate. Despite the high turnover, the olfactory sense is maintained throughout life through the division of a population of stem cells that produce new OSNs both during normal turnover and after an injury occurs in the OE. When new OSNs are born, they must extend axons from the OE to the olfactory bulb (OB) where they make specific synaptic contacts. To determine the timeline of axon extension in normal turnover and after a methimazole-induced injury, we used fate-tracing utilizing an inducible Cre-LoxP model in which a fluorescent reporter was expressed by neuronal precursors and subsequently used to track axonal growth as the OSNs matured. Our results show that axon extension in both conditions follow the same timeline. However, markers of synaptic connectivity in the OB were delayed after injury. The delay in synaptic connectivity was also corroborated with delays in olfactory behavior after injury, which took 40 days to recover to control levels. Additionally, we investigated the process of removal of axonal debris created after an injury. Immunohistochemical analysis after injury indicated upregulation of IBA1+ cells within the 3 olfactory nerve layer of the OB, suggesting a role of microglia in this process. These microglia also showed an activated morphology and some had very large cell bodies with multiple nuclei. Furthermore, qPCR analysis of post-injury OB tissue shows upregulation of the CD11b receptor that is expressed on microglia. Our results have also shown upregulation of components of the complement pathway after injury, which is suggestive of a mechanism that underlies axonal debris removal after injury in the OB. Taken together, these results shed light on the process by which the olfactory system is able to recover after injury and could lead to discovery of mechanisms that could translate to treatments for injuries in other areas of the nervous system. olfactory sensory neurons regeneration axon microglia phagocytosis Laboratory and Basic Science Research Molecular and Cellular Neuroscience Systems Neuroscience
32	Coding of tsetse repellents by olfactory sensory neurons: towards the improvement and the development of novel tsetse repellents Souleymane, Diallo January 2021 (has links) Philosophiae Doctor - PhD / Tsetse flies are the biological vectors of human and animal trypanosomiasis and hence representant medical and veterinary importance. The sense of smell plays a significant role in tsetse and its ecological interaction, such as finding blood meal source, resting, and larvicidal sites and for mating. Tsetse olfactory behaviour can be exploited for their management; however, olfactory studies in tsetse flies are still fragmentary. Here in my PhD thesis, using scanning electron microscopy, electrophysiology, behaviour, bioinformatics and molecular biology techniques, I have investigated tsetse flies (Glossina fuscipes fuscipes) olfaction using behaviourally well studied odorants, tsetse repellent by comparing with attractant odour. Insect olfaction is mediated by olfactory sensory neurons (OSNs), located in olfactory sensilla, which are cuticular structures exposed to the environment through pore and create a platform for chemical communication. Glossina fuscipes fuscipes Feeding deterrence Olfactory sensory neurons Chemosensory proteins Odorant receptors deorphanization
33	Effect of IP3R3 and NPY on Age-Related Declines in Olfactory Stem Cell Proliferation Jia, Cuihong, Hegg, Colleen C. 01 January 2015 (has links) Losing the sense of smell because of aging compromises health and quality of life. In the mouse olfactory epithelium, aging reduces the capacity for tissue homeostasis and regeneration. The microvillous cell subtype that expresses both inositol trisphosphate receptor type 3 (IP3R3) and the neuroproliferative factor neuropeptide Y (NPY) is critical for regulation of homeostasis, yet its role in aging is undefined. We hypothesized that an age-related decline in IP3R3 expression and NPY signaling underlie age-related homeostatic changes and olfactory dysfunction. We found a decrease in IP3R3+ and NPY+ microvillous cell numbers and NPY protein and a reduced sensitivity to NPY-mediated proliferation over 24months. However, in IP3R3-deficient mice, there was no further age-related reduction in cell numbers, proliferation, or olfactory function compared with wild type. The proliferative response was impaired in aged IP3R3-deficient mice when injury was caused by satratoxin G, which induces IP3R3-mediated NPY release, but not by bulbectomy, which does not evoke NPY release. These data identify IP3R3 and NPY signaling as targets for improving recovery following olfactotoxicant exposure. injury olfactory sensory neurons olfactory stem cells olfactory-mediated behavior proliferation
34	Atf5 Links Olfactory Receptor Induced Stress Response to Proper Neuronal Function Kahiapo, Jerome Keoki January 2020 (has links) Mammalian olfaction requires the enduring expression of a single olfactory receptor (OR) gene for the life of each sensory neuron. This is due to the fact that OR proteins play multiple roles in the coherent perception of odors, first by sensing molecular cues from the external environment, and by directing the wiring of neuronal projections faithfully from the peripheral sensory neurons to the brain. Both of these processes require singular and stable OR expression in olfactory sensory neurons (OSNs. The transcription factor Atf5 has previously been shown to enforce these modes of expression, through a process that requires the unfolded protein response (UPR). The work presented in this thesis deciphers how Atf5 enables proper OR expression and neuronal function in the olfactory system. We identify the developmental window in which UPR is activated, and provide evidence that Atf5 protein expression coincides with the assembly of a multi-chromosomal enhancer hub that drives singular and robust OR transcription, opposing a model in which precocious polygenic OR transcription initiates UPR. Further, we show that Atf5 directly regulates a collection of genes that facilitate proper OR trafficking, axonogenesis, as well as transcription factors and chromatin modifiers, which we propose to be involved in stable OR expression and neuronal maturation. Finally, we find that Atf5 has a special role in the olfactory system that cannot be replaced by its ubiquitously expressed homologue, Atf4, and that this is due to a requisite interaction between Atf5 and the bZIP transcription factor Cebpγ, and potentially other transcription factors known to be critical for olfactory function. Cytology Biochemistry Molecular biology Olfactory receptor genes Smell Sensory neurons Mammals
35	Detection of respiratory gas levels by internal sensory neurons in Drosophila larvae Lu, Shan January 2022 (has links) Internal sensory neurons monitor the chemical and physical state of the body, providing critical information to the nervous system for maintaining homeostasis and survival. Across species, such neurons innervate visceral organs to detect and relay information about their chemical and physical state to the central nervous system (CNS). While electrophysiology experiments over several decades have revealed a wide of range of stimuli that can activate internal sensory neurons, how stimuli are detected at the cellular and molecular level is only beginning to be elucidated. To elucidate the cellular and molecular basis of chemosensation by internal neurons, I used a population of larval Drosophila sensory neurons, tracheal dendrite (td) neurons, as the model system for my thesis work.I first presented a detailed characterization of the morphology of td neurons and their association with the tracheal system. I found that td dendrites extend along tracheal epithelial cells across their whole length. I further described that td dendrites extend to tracheal fusion sites, and can be observed terminating as enlarged bulbs adjacent to the tube enlargements. This specialized structure formed by td dendrites in relation to the nearby tracheal tissues may serve as an end organ for td sensory functions. I then proceeded to test the sensory functions of the td neurons. I found that td neurons respond to respiratory gases, namely decreases in O2 levels and increases in CO2 levels. Furthermore, I assessed the roles of atypical soluble guanylyl cyclases (Gycs) and a gustatory receptor (Gr) in mediating these responses. I found that Gyc88E/Gyc89Db are necessary for td responses to hypoxia, and that Gr28b is necessary for td responses to CO₂. Rescue of Gr28b isoform c rescued the mutant phenotype and also generalized the response to CO₂ in the td network. Additionally, I presented data suggesting carbonic anhydrases from surrounding tissues are required for td responses to CO₂, further elucidating the sensory transduction pathway of internal CO₂ detection. I further showed that gas-sensitive td neurons are activated when larvae burrow for a prolonged duration, demonstrating a natural-like feeding condition in which td neurons are activated. I also found that Drosophila larvae tend to avoid their td neurons being activated, suggesting td activation is aversive to the animals. Together, my work identified two stimuli that are detected by partially overlapping subsets of internal sensory neurons, and established roles for Gyc88E/Gyc89Db in the detection of hypoxia, and Gr28b together with carbonic anhydrases in the detection of CO₂. Combined with our previous understanding, different td neurons express various combinations of chemosensory receptors and have distinct functions, some of which remain to be discovered, indicating that this is a multifunctional internal sensory system. In conclusion, the results I presented in my thesis established new sensory detection pathways of Drosophila larval internal sensory neurons, which may be generalized across species and facilitate understanding of internal sensory systems. Neurosciences Drosophila--Development Sensory neurons Hypoxia (Water) Carbon dioxide Respiratory gas monitoring Insects--Larvae
36	GENETIC DISSECTION OF lin-11 REGULATION IN DIFFERENTIATION OF C. elegans AMPHID SENSORY NEURONS Amon, Siavash 10 1900 (has links) <p>The expression of <em>lin-11</em> is regulated by enhancers located upstream from, as well as within, <em>lin-11</em> intronic sequences. Multiple regulatory inputs control the spatiotemporal expression pattern of <em>lin-11</em>. To better understand that process, we have investigated these regulatory enhancers by dissecting two of the biggest intronic sequences of <em>lin-11</em>: intron 3 and intron 7. Using microscopy, we show that the expression of intron 3 is required in ten head sensory neurons and that the expression of intron 7 is required in two head neurons. The truncation of intron 7 revealed that its regulatory sequence may be located within its narrow 98 base pairs (bp) region. We used bioinformatics to predict which putative transcription factor(s) may regulate AVG expression. Using a hypersensitive RNAi mutant strain, <em>eri-1; lin-15b,</em> we tested forty putative transcription factors and quantitated the number of animals in which the molecular marker <em>lin-11::GFP</em> expression is knockdown in AVG interneurons.</p> <p>Using electrotactic behavioral analysis we show that the speed of<em> lin-11</em> null allele, n389, is reduced by almost 50%, when compared to that of the wildtype animals, due to amphid sensory neuronal deformities. We determine which conserved domains of <em>lin-11</em> are required for the proper development of the neuronal and vulval cells via microinjection rescue experiments.</p> <p>We sequenced eleven <em>lin-11</em> alleles to determine which conserved domains are affected and the role of each of these domains in the development of vulval and neuronal cells. Our findings suggest that all <em>lin-11</em> conserved domains are required for proper vulval cell differentiation as well as for proper development of the amphid sensory neurons. Finally, using tissue specific markers we label vulval cells in <em>lin-11</em> mutants to show that those cells are defective, as judged by the lack of fate-specific markers in the vulval cells.</p> / Master of Biological Science (MBioSci) C. elegans lin-11 sensory neurons AVG Biology Cell and Developmental Biology Biology
37	Mechanisms of rapid receptive field reorganization in rat spinal cord Vu, Hung 08 1900 (has links) Rapid receptive field (RF) reorganization of somatosensory neurons in the rat dorsal horn was examined using extracellular single unit recording. Subcutaneous injection of lidocaine into RFs of dorsal horn neurons results in expansion of their RFs within minutes. The expanded RFs appear adjacent to or/and proximal to original RFs. Out of 63 neurons tested, 36 (58%) show RF reorganization. The data suggest that dorsal horn of spinal cord is one of the initial sites for RF reorganization. The neural mechanisms of this effect are not well understood. We propose that changes in biophysical properties (membrane conductance, length constant) of the neurons resulting from lidocaine injection contribute to RF reorganization. Iontophoretic application of glutamate onto dorsal horn neurons that show lidocaine induced RF's expansion were used to test the model. Application of glutamate produced reduction of reorganized RFs in 9 of 20 (45%) tested cells. Application of NBQX produced no effect on either original or expanded RFs indicate that RF shrinkage effects of glutamate involve NMDA receptors. The results are consistent with the prediction of the proposed model. Subcutaneous injection of capsaicin into tactile RFs of low threshold mechanoreceptive dorsal horn neurons produced no effect on the RF sizes that are consistent with other studies. Following the injection, the original RFs were completely silenced (46%) or remained responsive (54%). Sensory neurons. Rats -- Nervous system. Spinal cord. rapid receptive field dorsal horn neurons spinal cord dorsal horn capsaicin
38	Developmental Strategy for Generating Sensory Neuron Diversity Li, Qingyun January 2015 (has links) <p>Sensory neuron diversity is a common theme in the animal kingdom. It provides the cellular infrastructure that supports the accurate perception of the external world. Among all sensory systems, the olfactory system demonstrates an extreme in the extraordinarily diversified neuronal classes it holds. The system-wide cellular diversity is in sharp contrast with the individual specialization of olfactory receptor neurons (ORNs) per se. How the nervous system, particularly the olfactory system, uses limited genetic information to generate a huge variety of neurons with distinct properties remains elusive. </p><p>The adult Drosophila olfactory system is an excellent model to address this question due to its conserved organizational principles and reduced complexity. The fly olfactory appendages contain 50 ORN classes, each of which expresses a single receptor gene from a family of ~80 genes. Stereotyped clusters of 1-4 ORN classes define about 20 sensilla subtypes, belonging to 3 major morphological types. All cellular components within a sensillum are born by a single sensory organ precursor (SOP) via asymmetric divisions. The molecular mechanisms that determine SOP differentiation potentials to develop into distinct sensilla subtypes and the associated ORN classes are unknown.</p><p>From a genetic screen, we identified two mutant alleles in the rotund (rn) gene locus, which has a critical function in diversifying ORN classes. Rn is required in a subset of SOPs to confer novel sensilla subtype differentiation potentials from otherwise default ones within each sensilla type lineage. In rn mutants, ORNs in rn-positive sensilla subtypes are converted to lineage-specific default rn-negative fates, resulting in only half of the normal ORN diversity. This work is described in Chapter 2.</p><p>Based on an unbiased time-course transcriptome analysis, we discovered two critical downstream targets of Rn, Bric-à-brac (Bab) and Bar. In light of the knowledge about leg development, we found these genes, along with Apterous (Ap) and Dachshund (Dac), are part of the conserved proximal-distal (PD) gene network that play a crucial role in patterning the antennal precursor field prior to proneural gene-mediated SOP selection. Interactions between these PD genes under the influence of morphogen gradients separate the developing antennal disc into 7 concentric domains. Each ring is represented by a unique combination of the aforementioned transcription factors, coding the differentiation potentials for a limited number of sensilla subtypes. Genetic perturbations of the network lead to predictable changes in the ratios of different sensilla subtypes and corresponding ORN classes. In addition, using CRISPR/Cas9 technology, we were able to add tags to specific rn isoforms in the endogenous locus, and show positive regulation of Bab and negative regulation of Bar by the direct binding of Rn to the promoters in vivo. This work is presented in Chapter 3.</p><p>We proposed a three-step mechanism to explain ORN diversification, starting from pre-patterning of the precursor field by PD genes, followed by SOP selection by proneural genes, and ended with Notch-mediated neurogenesis. The final outcomes are greatly determined by the pre-patterning phase, which may be modified during evolution to compensate special olfactory needs by individual species. In our model, each step serves a single purpose, which displays context-dependent functions. By changing contexts, reassembly of the same logical steps may guide neuronal diversification in parallel systems with completely different identities. This step-wise mechanism seems to be a common strategy that is used by many other systems to generate neuronal diversity.</p> / Dissertation Neurosciences Developmental biology Molecular biology Drosophila Neuronal diversity Olfactory receptor neurons Olfactory system Sensory neurons Transcription factor network
39	Rôle et régulation des co-transporteurs cation-chlorure NKCC1 et KCC3 dans les neurones sensitifs / Role and regulation of the cation-chloride cotransporters NKCC1 and KCC3 in sensory neurons Lucas, Olivier 09 June 2011 (has links) L'homéostasie chlorure (HC) est un acteur essentiel dans la transmission nerveuse. Le GABA, via son récepteur GABAA, permet les mouvements d'ions chlorures en fonction de leur potentiel électrochimique. Dans les neurones sensitifs de ganglions rachidiens dorsaux (GRD), le co-transporteur cation-chlorure NKCC1 est responsable de l'accumulation intracellulaire des ions Cl- et de l'effet dépolarisant du GABA. Suite à une lésion, l'augmentation de la concentration intracellulaire en ions Cl- ([Cl-]i) permet une amélioration des capacités régénératives neuronales. Au cours de ma thèse, je me suis en premier lieu intéressé à la régulation de l'HC par interleukine 6 (IL6) en réponse à une lésion nerveuse. L'axotomie du nerf sciatique induit l'expression de l'IL6 et son récepteur IL6-Rα dans les neurones sensitifs des GRD lombaires L4-L5. Des mesures par patch perforé sur des neurones sensitifs en culture ont montré une augmentation de la [Cl-]i dépendante de l'IL6 dans une sous-population de neurones mécano- et proprioceptifs en réponse à l'axotomie. Cette régulation est permise par la phosphorylation à la membrane plasmique neuronale de NKCC1. Le co-transporteur KCC3 est impliqué dans une maladie génétique conduisant dès la naissance à une perte sensorimotrice, ce qui m'a conduit à étudier son rôle dans la régulation de l'HC des neurones sensitifs au cours du développement et chez l'adulte. Nos données ont démontré l'existence d'un « switch chlorure » développemental, diminuant la [Cl-]i. Ce switch est altéré chez la souris KCC3-/-, dans laquelle une partie des neurones a déjà diminué sa [Cl-]i. Au stade adulte, nous avons également observé un doublement de la [Cl-]i dans 30% des neurones sensitifs de souris KCC3-/-, pourcentage corrélé à la proportion de neurones WT exprimant KCC3. Ces données prouvent que KCC3 est impliqué, de manière directe ou non, dans la régulation de l'HC des neurones sensitifs au cours du développement et chez l'adulte. / Chloride homeostasis (CH) is a major component of nerve transmission. Interaction between the neurotransmitter GABA and his receptor, GABAA, allows chloride movements depending on electrochemical potential. In dorsal root ganglia (DRG) sensory neurons, the cation-chloride cotransporter NKCC1 is responsible for intracellular accumulation of chloride ions and depolarizing effects of GABA. After injury, an increase of intracellulaire chloride concentration ([Cl-]i) allows an improvement of neuronal regenerative capacities. In a first time, I worked on regulation of CH by interleukine 6 (IL6) in response to nerve injury. Axotomy of the sciatic nerve induces expression of IL6 and his receptor IL6-Rα in sensory neurons from lombar L4-L5 DRG. Perforated patch measurements of sensory neurons have demonstrated an increase of [Cl-]i depending on IL6 in a sub-population of mechano- and proprioceptors in response to lesion. This regulation is provided by phosphorylation at the neuronal plasma membrane of NKCC1. The cation-chloride cotransporter KCC3 is implicated in a hereditary syndrome leading after birth to sensorymotors defects. This is why I have studied his role in regulation of CH in sensory neurons during development and in adulthood. Data have shown the existence of a peripheral developmental “chloride switch”. This switch is abolished in KCC3-/- sensory neurons, in which a part of neurons has already decreased [Cl-]i. In adulthood, we also observed an [Cl-]i twice as much as WT in 30% of sensory neurons from KCC3-/- mice. This percentage is correlated to the proportion of WT neurons expressing KCC3. These results demonstrate for the first time that KCC3 is implicated in regulation of CH in sensory neurons during development and in adulthood. Interleukine 6 Kcc3 Homéostasie chlorure Nkcc1 Lésion périphérique Neurones sensoriels Interleukin 6 Kcc3 Chloride homeostasis Nkcc1 Peripheral injury Sensory neurons
40	Caracterização da atividade antinociceptiva de peptídeos homólogos ao C-terminal da proteína S100A9 murina. Ação sobre neurônios sensoriais via canais de cálcio dependentes de voltagem do tipo N / Characterization of the antinociceptive effect of peptides homologous to the C-terminus of murine S100A9 protein. Effects on sensory neurons, via type-N voltage-dependent calcium channels Dale, Camila Squarzoni 18 December 2006 (has links) O peptídeo idêntico ao C-terminal da proteína S100A9 murina (pS100A9mH92-G110) inibe a hiperalgesia inflamatória induzida pela carragenina. Em adição, este peptídeo inibe a hiperalgesia inflamatória induzida por tripsina, uma serino protease capaz de ativar receptores ativados por protease do tipo 2 (PAR2). O objetivo inicial deste trabalho foi caracterizar a relação estrutura/ efeito do pS100A9m, a fim de determinar a menor seqüência peptídica dotada de atividade antinociceptiva. Ainda, como parte dos objetivos, neste trabalho foram investigados os mecanismos envolvidos no efeito antinociceptivo do pS100A9m e da menor seqüência ativa sobre a hiperalgesia induzida pela ativação de PAR2. Diferentes seqüências peptídicas homólogas ao pS100A9m foram sintetizadas e avaliadas em ratos submetidos ao modelo de hiperalgesia mecânica induzida por carragenina. Dentre todas as seqüências peptídicas investigadas, o peptídeo denominado AcE97-G102 foi determinado como a menor seqüência ativa com efeito semelhante ao pS100A9m. Com relação aos estudos sobre a ativação de PAR2, os resultados obtidos demonstraram que o pS100A9m bem como o AcE97-G102 inibem a hiperalgesia térmica e mecânica decorrentes da ativação de PAR2 (induzida por um peptídeo agonista deste receptor ? PAR2AP). A análise por imuno-histoquímica demonstrou que a ativação de PAR2 aumenta a expressão da proteína Egr-1 em neurônios nociceptivos, sendo o pS100A9m capaz de inibir este efeito. Em adição, ambos pS100A9m e AcE97-G102 inibiram o influxo de cálcio induzido por PAR2AP ou tripsina, em neurônios sensoriais do gânglio da raiz dorsal da medula espinhal (DRG). Por outro lado, nenhum dos peptídeos apresentou efeito sobre a mobilização de cálcio em células HEK-293, que naturalmente expressam PAR2, ou em células KNRK transfectadas com este tipo de receptor, sugerindo que o efeito tanto do pS100A9m quanto do AcE97-G102, sobre a ativação de PAR2, seja específico para neurônios sensoriais. O pS100A9m e o AcE97-G102 inibiram o influxo de cálcio nos neurônios DRG estimulados com bradicinina, capsaicina ou KCl. Ainda, o pS100A9m inibiu a liberação de substância P induzida por PAR2. Os resultados obtidos com o tratamento de neurônios DRG com tapsigaragina ou com ionóforo de cálcio sugerem um efeito direto do pS100A9m sobre os canais de cálcio. Desta forma, foi avaliada atividade do pS100A9m e do AcE97-G102 sobre culturas de células HEK-tsA transfectadas com canais de cálcio dependente de voltagem do tipo N ou do tipo L. Os resultados obtidos demonstraram que ambos peptídeos inibirem o influxo de cálcio em células transfectadas com receptores do tipo N. Em conjunto, os dados aqui obtidos demonstram que o efeito do C-terminal da proteína S100A9 murina sobre a nocicepção experimental é devido a uma inibição de canais de cálcio do tipo N, por uma ação direta em neurônios sensoriais. Ainda, a seqüência responsável por este efeito está localizada na porção E97-G102 do domínio C-terminal da proteína S100A9 murina. / Peptide identical to the C-terminus of S100A9 protein (mS100A9pH92-G110) inhibits inflammatory hyperalgesia induced by carrageenan and trypsin, a serine protease that activates protease-activated receptors 2 (PAR2). The aim of this work was to characterize the relationship between structure and function of mS100A9p in order to identify the shortest peptide sequence endowed with antinociceptive effect. Furthermore, the mechanisms involved on the antinociceptive effect of both mS100A9p and the shortest homologous sequence on PAR2-induced hyperalgesia were also evaluated. Different peptide sequences homologous to mS100A9p were synthesized and evaluated in rats submitted to the carrageenan-induced mechanical hyperalgesia model. Among all evaluated sequences, the peptide AcE97-G102 was found to be the shortest sequence that showed an antinociceptive effect similar to that induced by mS100A9p. In regard to PAR2 activation, data obtained herein demonstrated that both mS100A9p and AcE97-G102 inhibit PAR2-induced mechanical and thermal hyperalgesia, induced by the selective agonist peptide ? PAR2AP. Imunohistochemical evaluation demonstrated that PAR2 activation increased Egr-1 protein expression on sensory neurons and mS100A9p inhibited this effect. In addition, both mS100A9p and AcE97-G102 inhibited PAR2- and trypsin-induced calcium influx in dorsal root ganglia neurons (DRG). On the other hand, no effect on the calcium influx of the peptides were observed on HEK-293 cells or KNRK-PAR2 transfected cells, suggesting that the effects of mS100A9p and AcE97-G102 on PAR2 activation are specific for sensory neurons. Both mS100A9p and AcE97-G102 inhibited DRG calcium flux when cells were stimulated with bradykinin, capsaicin or KCl. Also, mS100A9p inhibited PAR2-induced substance P release in DRG. Treatment of DRG with either thapsigargin or calcium ionophore suggest a direct effect of mS100A9p on calcium channels. To evaluate this hypothesis the effects of mS100A9p and AcE97-G102 were evaluated on N-type or L-type voltage-dependent calcium channel transfected HEK-tsA cells. Both peptides inhibited calcium influx of N-type transfected cells. In conclusion, data presented herein demonstrate that the C-terminus of murine S100A9 protein inhibits experimental nociception through a block of N-type voltage-dependent calcium channels, directly on sensory neurons. Also, the domain involved in this effect is localized on the sequence E97-G102 of the C-terminus of murine S100A9 protein. Antinocicepção Antinociception Neurônios sensoriais Nocicepção Nociception PAR2 PAR2 S100A9 S100A9 Sensory neurons Voltage dependent calcium channels

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