The toxicity of methyl iodide : in vivo and in vitro mechanistic studies in the rat nasal cavity and cerebellum

Chamberlain, Mark Peter

January 1998

No description available.

572

Glutathione; GSTs; Olfactory epithelium

Development and validation of an in vitro rat nasal epithelial model for predicting respiratory tract toxicity

Kilgour, Joanne Dawn

January 1997

No description available.

615.9

Observations on the Electrical Activity in the Olfactory Epithelium and Tract of Some Fishes / Electrical Activity in the Olfactory System of Some Fishes

van Dijk, Clasina

10 1900

In this investigation the electrophysiological response to stimulation of the olfactory epithelium in response to trout scent and some of its chemical components was studied. Recordings were made both from the lamprey nasal sac and the catfish olfactory tract and the various responses described and compared with responses measured by other authors. / Thesis / Master of Science (MS)

electric

olfactory

olfactory epithelium

fish

Olfactory Epithelium size in Mammals : A structured review

Hipp Marchidan, Gabrielle

January 2021

Members of the class Mammalia have the most advanced skeletal complexity of the nasal cavity among vertebrates. Most mammals have an olfactory epithelium that consists of basal cells, supporting cells and olfactory sensory neurons that bind odor molecules with their cilia. The olfactory epithelium is responsible for detecting odor stimuli. The surface area of olfactory epithelium varies greatly among species. Carnivores have a generally larger surface area of the olfactory epithelium than primates and ungulates of the same size. Modern odontocetes lack olfactory epithelium. To get an overview of the between-species differences of the olfactory epithelium surface area and number of olfactory receptor cells, a search of the scientific literature was performed, using the database Web of Science and references from the scientific articles. The assembled data were entered into two tables, one that contains species names, surface area of the olfactory epithelium and references, and another that includes the total number of olfactory receptor cells for the few species that have been studied in this respect so far. Methods of measuring olfactory epithelium size differ, some studies used immunohistochemistry, other measured osteological proportions, like the surface area of the olfactory turbinals. A compilation of the published data provides an overview of the range that the size of the olfactory epithelium can have and allows for between-species comparisons of this anatomical measure as well as for assessing possible correlations with olfactory capabilities.

mammal olfaction

olfactory epithelium

olfactory receptor cells

Physiology

Fysiologi

Investigations of Olfactory Mucosa to Test the Neurodevelopmental Nature of Psychoses

McCurdy, Richard D, n/a

January 2005

Evidence from various sources suggests that schizophrenia may result from altered brain development. The adult olfactory epithelium provides an available 'window' on neuronal development because new neurons are formed there throughout life. This thesis set out to test the neurodevelopmental hypothesis of psychotic disease. Two cell-based models, skin fibroblast and olfactory mucosa culture, were employed to investigate this hypothesis. In order to first demonstrate the utility of olfactory mucosa culture as a model of neurodevelopment, and to allow the candidate to gain proficiency in the culture of this tissue, an investigation of the mitogenic and differentiating properties of insulin-like growth factor-I within this system was undertaken. Insulin-like growth factor-I has multiple effects within the developing nervous system but its role in neurogenesis in the adult nervous system is less clear. The adult olfactory mucosa is a site of continuing neurogenesis that expresses insulin-like growth factor-I, its receptor, and its binding proteins. The action of insulin-like growth factor-I was assayed in several serum-free culture systems combined with bromodeoxyuridine labelling of proliferating cells and immunochemistry for specific cell types. Once proficiency in olfactory mucosa culture was gained, this model was applied to biopsied olfactory mucosa from schizophrenia and bipolar disorder patients in order to test the developmental parameters of adhesion, cell proliferation, and cell death in a neural tissue. It was previously shown that olfactory cultures from individuals with schizophrenia had increased cell proliferation and attached less frequently than cultures from healthy controls suggesting disrupted neurogenesis. An aim of this study was to replicate those observations in individuals with schizophrenia and and extend them to individuals with bipolar disorder. After completion of the cell and tissue culture assays, microarray analysis of these cell-based models was used to reveal gene expression differences present between patients and healthy controls. Microarray analysis is a complicated technique and the limited amounts of RNA that can be extracted from a single nasal biopsy further compounds this issue. In order to obtain enough material for microarray hybridization RNA samples underwent antisense amplification. Therefore, with the aim of allowing the candidate to gain proficiency in both these techniques prior to microarray analysis of olfactory biopsies from patients with schizophrenia and bipolar disorder, a pilot microarray study of cultured skin fibroblasts from schizophrenia patients and healthy controls was performed. The present findings show that insulin-like growth factor-I and its receptor were expressed by globose basal cells (the neuronal precursor), by neurons and by olfactory ensheathing cells, the special glia of the olfactory nerve. Insulin-like growth factor-I reduced the numbers of proliferating neuronal precursors, induced their differentiation into neurons, and promoted morphological differentiation of neurons. In contrast, this growth factor was mitogenic for olfactory ensheathing cells. The evidence suggests that insulin-like growth factor-I is an autocrine/paracrine signal that induces neuronal precursors to differentiate into olfactory sensory neurons and induces olfactory ensheathing cells to proliferate and that olfactory mucosa culture is valuable in modelling neurodevelopmental processes. When the olfactory musoca culture model was applied to patients with psychosis, a two-fold increase in proliferation of neural cells was found in schizophrenia compared to controls and bipolars. In bipolar cultures there was a 3-fold increase in cell death compared to controls and schizophrenia. Microarray analysis of cultured skin fibroblasts revealed differential expression of over 1000 genes between patients and controls. Inspection of the significant data showed alterations to gene expression between groups in the cell cycle, oxidative phosphorylation, TCA cycle and oxidative stress pathways. Gene expression in each of these pathways was predominately decreased in schizophrenia. Quantitative PCR analysis of selected differentially expressed genes involved with cell cycle regulation validated the increased expression of vitamin D receptor, and decreased expression of proliferating cell nuclear antigen and DEAD (Asp-GIu-Ala-Asp) box polypeptide 5 in skin fibroblasts from patients with schizophrenia. Microarray analysis of biopsied olfactory mucosa showed 146 and 139 differentially expressed genes in schizophrenia and bipolar disorder respectively, compared to controls. Consistent with increased mitosis in schizophrenia biopsy cultures three genes that function to positively influence cell cycle had increased expression. In the bipolar disorder group a dysregulation of the phosphatidylinositolsignalling pathway was seen; five genes that either directly function within or interact with this pathway had decreased expression. There is speculation that the therapeutic effect of psychotropic drugs acting upon this pathway in bipolar disorder involves reduction of neuronal cell death. Increased mitosis of neural cells has now been observed in two separate groups of schizophrenic patients indicating a robust finding. The use of fibroblast and olfactory mucosal tissue can be used to study biological and genetic aspects of neurodevelopment in living humans both with and without psychotic disease. Biopsied olfactory mucosa provides benefits over the use of autopsied material for study of psychotic disease because post-mortem duration and agonal factors that lead to tissue, protein and nucleic acid degradation are not an issue. This study provides evidence for a neurodevelopmental aetiology of schizophrenia and bipolar disorder acting at the level of cell cycle control. Subtle changes in the timing of cell cycle regulation could account for the brain pathologies observed in these diseases. Olfactory mucosa culture is a valuable model of neurodevelopmental processes.

Schizophrenia

adult olfactory epithelium

insulan-like growth factor-1

gene expression

neurodevelopment

psychotic disease

Neuronal Differentiation: A Study Into Differential Gene Expression

De las Heras, Rachel, n/a

January 2003

Neuronal differentiation encompasses an elaborate developmental program which until recently was difficult to study in vitro. The advent of several cell lines able to differentiate in culture proved to be the turning point for gaining an understanding of molecular neuroscience. In particular the olfactory epithelium provides an attractive tool with which to investigate fundamental questions relating to neuronal differentiation, as it displays a unique capacity to regenerate and to retain a neurogenetic potential from its genesis and throughout adult life. The coordinated regulation of gene expression is fundamental to the control of neuronal differentiation. In order to reveal active processes at the molecular level and to dissect key components of molecular pathways, differential gene expression studies provide a foundation for the elucidation of dynamic molecular mechanisms. This thesis identified genes involved in neuronal differentiation by utilising a clonal olfactory receptor neuronal cell line (OLF442). Gene expression levels were identified using differential display and oligonucleotide array technology before and after serum deprivation. Differential display revealed two kinases whose expression levels were elevated during the differentiation of OLF442, identified as focal adhesion kinase (FAK) related non-kinase (FRNK) and mammalian ste20 like (MST)2 kinase. Furthermore, analysis of the oligonucleotide array data confirmed the expression of genes involved in altering presentation of extracellular matrix molecules, in mediating cytoskeletal rearrangements, and in ceasing the cell cycle, supporting the use of OLF442 as a model for studying differentiation. The differentiation of OLF442 results from the synchronisation of multiple transduction cascades and cellular responses as evidenced by the microarray data. A protein that can synchronise such signalling is the non-receptor protein tyrosine kinase, FAK. Thus the finding of the endogenous FAK inhibitor FRNK by differential display was intriguing as there was no difference in the expression level of FAK induced by differentiation, contrasting that of FRNK. This induced FRNK expression was derived autonomously as it was not responsive to the caspase-3 inhibitor, DEVD-CHO. This is particularly pertinent since the primary role of FRNK is to act as an inhibitor of FAK by competing with its substrates and reducing the phosphorylation of both FAK and its associated proteins. Differential display also revealed the upregulation of another kinase, which had 90% homology with rat MST2 kinase within the 3' UTR. Both mouse MST2 kinase (sequence submitted to GenBank, accession number AY058922) and the closely related family member MST1 kinase were sequenced and cloned. Moreover, evidence to support an autonomously expressed carboxyl-terminal domain of MST2 kinase is presented in Chapter 3 and provides a unique way in which MST2 may regulate its own activity. To further understand the role of MST in neuronal differentiation, a series of stable OLF442 transfections (with mutant and wild-type MST constructs) were carried out. MST was localised with cytoplasmic structures that may represent actin stress fibres, indicating a potential cytoskeletal role during neuronal differentiation. This indicated that MST1 may play a role in the morphological processes involved in neuronal differentiation. The identification of two kinases by differential display provided the motivation to understand the cellular context of OLF442 and to determine the phosphorylation status of the mitogen-activated protein kinase (MAPK) signalling cascades. Differentiation of OLF442 induced high-level phosphorylation of a putative B-Raf isoform, MEK2 and ERK1/2. Interestingly, there was a switch between preferential phosphorylation of MEK1 in undifferentiated OLF442 to preferential phosphorylation of MEK2 following differentiation. SAPK/JNK was also phosphorylated, as was the transcription factor c-Jun, which is a common substrate of both the ERK and SAPK/JNK signalling modules. The mapping of the cellular context of differentiating OLF442 has identified a promising model of a novel MAPK module. This consists of FAK signalling through Rap1 to ERK providing sustained activation, which is buffered or terminated by the expression of the endogenous FAK inhibitor FRNK. Furthermore, MST kinase could potentially play a role in regulating the cytoskeletal re-arrangements that are necessary for neuronal differentiation. MST kinase may signal transiently via the SAPK pathway to provide concomitant activation of c-Jun that is required for neuronal differentiation. An understanding of the gene expression pattern of the normal neuronal differentiation program allows a greater understanding of potential developmental aberrations. This could provide an opportunity for therapies to be conceived, while understanding the complexity of neuronal determination could also provide opportunities for stem cell transplantation.

neuronal differentiation

cell differentiation

molecular neuroscience

gene expression

differential gene expression

olfactory epithelium

kinase

kinases

stem cell transplantation

Molecular and functional anatomy of the mouse olfactory epithelium

Vedin, Viktoria

January 2006

The olfactory system is important for social behaviors, feeding and avoiding predators. Detection of odorous molecules is made by odorant receptors on specialized sensory neurons in the olfactory epithelial sheet. The olfactory sensory neurons are organized into a few regions or “zones” based on the spatially limited expression of odorant receptors. In this thesis the zonal division and functional specificity of olfactory sensory neurons have been studied in the mouse. We find that zones 2-4 show overlapping expression of odorant receptors while the border between the regions that express a zone 1 and a zone 2 odorant receptor, respectively, is sharp. This result indicates that zone 1 and zones 2-4 are inherently different from each other. In cDNA screens, aimed at finding genes whose expression correlate to the zonal expression pattern of odorant receptors, we have identified a number of signaling proteins implicated in neural-tissue organogenesis in other systems. The differential expression pattern of identified genes suggests that regional organization is maintained during the continuous neurogenesis in the olfactory epithelium as a result of counter gradients of positional information. We show that the gene c-fos is induced in olfactory sensory neurons as a result of cell activation by odorant exposure. A zonal and scattered distribution of c-Fos-positive neurons resembled the pattern of odorant receptor expression and a change of odorant results in a switch in which zone that is activated. Whereas earlier studies suggest that the odorant receptors are relatively broadly tuned with regard to ligand specificity, the restricted patterns of c-Fos induction suggests that low concentrations of odorous molecules activate only one or a few ORs. Studies on olfactory detection abilities of mice with zonal-restricted lesions in the olfactory epithelium show that loss of a zone has severe effects on the detection of some odorants but not others. These findings lend support to a hypothesis that odorant receptors are tuned to more limited numbers of odorants. Regional differences in gene expression and differences in response to toxic compounds between the zones indicate that there may be differences in tissue homeostasis within the epithelium. We have found that there are differences in proliferation and survival of olfactory sensory neurons in regions correlating to receptor expression zones. Identified differences with regard to gene expression, tissue homeostasis and odorant detection show that the olfactory epithelium is divided into regions that transduce different stimulus features.

olfactory epithelium

odorant receptor

zone

odorant

gene expression

cell specification

c-Fos

dichlobenil

olfactometry

proliferation

Molecular biology

Molekylärbiologi

Mise en évidence de transporteurs de la résistance pléiotropique dans la muqueuse olfactive et leur implication dans la réponse aux odorants chez les rongeurs / Evidence of multidrug resistance transporters in rodents olfactory epithelium and their implication in the response to odorants

Molinas, Adrien

09 December 2011

La résistance pléiotropique (MDR) est une propriété de certaines cellules relative à la capacité de rejeter ou d’évacuer une très large variété de substances potentiellement toxiques. Les pompes à l’origine de ce rejet sont des protéines membranaires appartenant à la superfamille ABC (ATP-Binding Cassette). Deux membres de cette famille ABC confèrent la propriété de résistance pléiotropique, P-gp (P-glycoprotein) et MRP1 (Multidrug Resistance-associated Protein). Nous avons mené une étude fonctionnelle sur l’activité de ces deux transporteurs dans la muqueuse olfactive à la fois chez le rat et la souris. Nous avons employé le test fluorométrique à la calcéine-AM sur des tranches coronales de la muqueuse olfactive incubées en présence d’inhibiteurs spécifiques des transporteurs de la résistance pléiotropique, vérapamil et cyclosporine A comme inhibiteurs de Pgp ainsi que probénécide et MK571 comme inhibiteurs de MRP1. Chacun de ces quatre inhibiteurs provoque une augmentation significative de l’intensité de la fluorescence.Afin de savoir si les transporteurs de la résistance pléiotropique peuvent être impliqués dans la réponse olfactive nous avons examiné les réponses évoquées par des odorants seuls ou mélangés à l’aide d’enregistrements d’électro-olfactogrammes (EOG). En présence des deux inhibiteurs de MRP1, l’amplitude maximale des EOG est significativement réduite pour chaque stimulus odorant testé, tandis que les inhibiteurs de Pgp n’ont qu’un effet modéré ou nul. L’expression des gènes codant pour Pgp et MRP1 dans l’épithélium olfactif ont ensuite été confirmées par RT-PCR. L’ensemble de ces résultats suggère que les transporteurs MRP1 et Pgp sont présents et fonctionnels dans l’épithélium olfactif principal des rongeurs et sont impliqués dans la réponse aux odorants. Leur fonction précise dans l’olfaction reste à élucider / Multidrug resistance (MDR) is a property of various cells associated with the capacity to reject or efflux a wide range of potentially harmful substances out of the cell. Pumps that effect such efflux are membrane proteins and belong to the ATP- binding cassette (ABC) superfamily. Among the members of the ABC family two are conferring MDR, P-glycoprotein (Pgp) and the multidrug resistance-associated protein (MRP1). In this study we investigated the functional activity of MDR transporters in olfactory mucosa of two species, rat and mouse. We used the fluorometric calcein-AM uptake assay on olfactory mucosal slices incubated with specific inhibitors of the MDR-transporters, verapamil and cyclosporin A as Pgp-inhibitors, and probenecid and MK571 as MRP-inhibitors. All four inhibitors caused significant increases in fluorescence intensities. To test if MDR transporters may be involved in the olfactory response we examined odorant evoked responses to single and mixed odorants by means of electro-olfactograms recordings (EOG). In the presence of the two MRP inhibitors, maximum EOG amplitudes were significantly reduced for all odorants tested, while Pgp inhibitors had only a moderate or no effect. Expression of Pgp and MRP1 encoding genes in the olfactory epithelium was further confirmed by RT-PCR. The results together suggest that MRP and Pgp transporters are present and functional in the main olfactory epithelium of rodents and are implicated in the olfactory response. The precise functional role in olfaction remains to be elucidated.

Epithélium olfactif

Electro-olfactogramme

Résistance pléiotropique

Calcéine

Rongeurs

Olfactory epithelium

Electro-olfactogram

Multidrug resistance

Calcein

Rodents

571.6

616.8

P/Q Type Calcium Channel Cav2.1 Defines a Unique Subset of Glomeruli in the Mouse Olfactory Bulb

Pyrski, Martina, Tusty, Mahbuba, Eckstein, Eugenia, Oboti, Livio, Rodriguez-Gil, Diego J., Greer, Charles A., Zufall, Frank

04 September 2018

Voltage-gated calcium (Cav) channels are a prerequisite for signal transmission at the first olfactory sensory neuron (OSN) synapse within the glomeruli of the main olfactory bulb (MOB). We showed previously that the N-type Cav channel subunit Cav2.2 is present in the vast majority of glomeruli and plays a central role in presynaptic transmitter release. Here, we identify a distinct subset of glomeruli in the MOB of adult mice that is characterized by expression of the P/Q-type channel subunit Cav2.1. Immunolocalization shows that Cav2.1+ glomeruli reside predominantly in the medial and dorsal MOB, and in the vicinity of the necklace glomerular region close to the accessory olfactory bulb. Few glomeruli are detected on the ventral and lateral MOB. Cav2.1 labeling in glomeruli colocalizes with the presynaptic marker vGlut2 in the axon terminals of OSNs. Electron microscopy shows that Cav2.1+ presynaptic boutons establish characteristic asymmetrical synapses with the dendrites of second-order neurons in the glomerular neuropil. Cav2.1+ glomeruli receive axonal input from OSNs that express molecules of canonical OSNs: olfactory marker protein, the ion channel Cnga2, and the phosphodiesterase Pde4a. In the main olfactory epithelium, Cav2.1 labels a distinct subpopulation of OSNs whose distribution mirrors the topography of the MOB glomeruli, that shows the same molecular signature, and is already present at birth. Together, these experiments identify a unique Cav2.1+ multiglomerular domain in the MOB that may form a previously unrecognized olfactory subsystem distinct from other groups of necklace glomeruli that rely on cGMP signaling mechanisms.

Cacna1a

Cav2.1α-1a subunit

olfactory bulb

olfactory epithelium

olfactory glomerulus

olfactory subsystem

synaptic localization

voltage-gated calcium channel

Biomedical Sciences

Identificação de RNAs não codificadores expressos no epitélio olfatório / Identification of noncoding RNAs expressed in the olfactory epithelium

Nascimento, João Batista Placido do

15 May 2018

Odorantes são detectados por centenas de receptores olfatórios (ORs) que pertencem à superfamília dos receptores acoplados à proteína G. Estes receptores são expressos nos neurônios sensoriais olfatórios localizados na cavidade nasal. Cada neurônio sensorial olfatório expressa um único alelo de gene OR de uma grande família de genes OR. Este padrão característico da expressão de genes OR resulta na formação de um mapa olfatório espacial no bulbo olfatório, que é necessário para a discriminação de odorantes pelo sistema olfatório. Os mecanismos envolvidos nesta regulação ainda não são bem conhecidos. O DNA genômico em neurônios olfatórios é coberto com marcas repressivas de metilação de histonas, indicando que a regulação da estrutura da cromatina deve desempenhar um papel importante na regulação da expressão de genes OR. Trabalhos anteriores demonstraram que RNAs não codificadores (ncRNAs) estão envolvidos na deposição de marcas de histonas em determinados genes. No entanto, os ncRNAs expressos no epitélio olfatório ainda não são conhecidos. Neste trabalho, identificamos e catalogamos o repertório completo de ncRNAs anotados, incluindo os miRNAs, expressos no epitélio olfatório de camundongos recémnascidos e adultos. Muitos destes, apesar de já anotados como ncRNAs, ainda não foram descritos na literatura como expressos no MOE. Identificamos ao todo 1161 miRNAs e 295 lincRNAs expressos no epitélio olfatório, e pudemos verificar como os níveis de expressão destes RNAs variam durante o desenvolvimento. A partir deste repertório, selecionamos lincRNAs que são preferencialmente expressos no epitélio olfatório quando comparados a outros tecidos de camundongo. Dez destes lincRNAs foram selecionados para validação utilizando-se RT-PCR. Cinco lincRNAs foram validados e analisados quanto à sua expressão em diferentes tecidos. Nosso trabalho estabelece uma plataforma de dados que permitirá o estudo do papel desempenhado por ncRNAs no epitélio olfatório. Além disto, os nossos resultados mostram que a abordagem utilizada permite a identificação de novos lincRNAs que apresentam expressão restrita ou preferencial no epitélio olfatório, e que, portanto, devem apresentar uma função relevante para o olfato. / Odorants are detected by hundreds of odorant receptors (ORs) which belong to the superfamily of G protein-coupled receptors. These receptors are expressed in the olfactory sensory neurons of the nose. Each olfactory sensory neuron expresses one single OR gene allele from a large family of OR genes. This characteristic pattern of OR gene expression results in the formation of a spatial olfactory map in the olfactory bulb, which is required for odorant discrimination by the olfactory system. The mechanisms involved in this regulation are unknown. OR genomic DNA in olfactory neurons is covered with repressive histone methylation marks, indicating that the chromatin structure should play an important role in the regulation of OR gene expression. Previous studies suggest that noncoding RNAs (ncRNAs) are involved in the deposition of histone marks in certain genes. However, the ncRNAs expressed in the olfactory epithelium are completely unknown. In this work, we used RNA-seq to identify and catalogue the complete repertoire of ncRNAs, including miRNAs, expressed in the olfactory epithelium from newborn and adult mice. In this way, we were able to identify 1161 miRNAs and 295 lincRNAs and analyze how their levels of expression varies during development. Out of these repertoire, we selected lincRNAs that are preferentially expressed in the olfactory epithelium when compared to other mouse tissues. Ten out of these lincRNAs were selected for validation by using RTPCR, and five of them could be validated and further analyzed. Our work establishes a data platform which will enable the study of the role played by ncRNAs in the olfactory epithelium. In addition, our results show that our approach can be successfully used to identify ncRNAs that are restrictedly or preferentially expressed in the olfactory epithelium, and which therefore must be relevant for olfaction.

Epitélio Olfatório

Expressão gênica

lincRNAs

lincRNAs

miRNAs

miRNAs

ncRNAs

ncRNAs

Odorant receptors

Olfactory epithelium

Receptores olfatórios

RNA-seq

Sequenciamento de DNA em larga escala