Frequency preference and reliability of signal integration

Schreiber, Susanne

21 July 2004

Die Eigenschaften einzelner Nervenzellen sind von grundlegender Bedeutung für die Verarbeitung von Informationen im Nervensystem. Neuronen antworten auf Eingangsreize durch Veränderung der elektrischen Spannung über die Zellmembran. Die Spannungsantwort wird dabei durch die Dynamik der Ionenkanäle in der Zellmembran bestimmt. In dieser Arbeit untersuche ich anhand von leitfähigkeits-basierten Modellneuronen den Einfluss von Ionenkanälen auf zwei Aspekte der Signalverarbeitung: die Frequenz-Selektivität sowie die Zuverlässigkeit und zeitliche Präzision von Aktionspotentialen. Zunächst werden die zell-intrinsischen Mechanismen identifiziert, welche the Frequenz-Selektivität und die Zuverlässigkeit bestimmen. Weiterhin wird untersucht, wie Ionenkanäle diese Mechanismen modulieren können, um die Integration von Signalen zu optimieren. Im ersten Teil der Arbeit wird demonstriert, dass der Mechanismus der unterschwelligen Resonanz, so wie er bisher für periodische Signale beobachtet wurde, auch auf nicht-periodische Signale anwendbar ist und sich ebenfalls in den Feuerraten niederschlägt. Im zweiten Teil wird gezeigt, dass zeitliche Präzision und Zuverlässigkeit von Aktionspotentialen mit der Stimulusfrequenz variieren und dass, in Abhängigkeit davon, ob das Stimulusmittel über- oder unterhalb der Feuerschwelle liegt, zwei Stimulusregime unterschieden werden müssen. In beiden Regimen existiert eine bevorzugte Stimulusfrequenz, welche durch die Gesamtleitfähigkeit und die Dynamik spezifischer Ionenkanäle moduliert werden kann. Im dritten Teil wird belegt, dass Ionenkanäle die Zuverlässigkeit auch direkt über eine Veränderung der Sensitivität einer Zelle gegenüber neuronalem Rauschen bestimmen können. Die Ergebnisse der Arbeit lassen auf eine wichtige Rolle der dynamischen Regulierung der Ionenkanäle für die Frequenz-Selektivität und die zeitliche Präzision und Zuverlässigkeit der Spannungsantworten schließen. / The properties of individual neurons are of fundamental importance for the processing of information in the nervous system. The generation of voltage responses to input signals, in particular, depends on the properties of ion channels in the cell membrane. Within this thesis, I employ conductance-based model neurons to investigate the effect of ionic conductances and their dynamics on two aspects of signal processing: frequency-selectivity and temporal precision and reliability of spikes. First, the cell-intrinsic mechanisms that determine frequency selectivity and spike timing reliability are identified on the basis of conductance-based model neurons. Second, it is analyzed how ionic conductances can serve to modulate these mechanisms in order to optimize signal integration. In the first part, the frequency selectivity of subthreshold response amplitudes previously observed for periodic stimuli is proven to extend to nonperiodic stimuli and to translate into firing rates. In the second part, it is demonstrated that spike timing reliability is frequency-selective and that two different stimulus regimes have to be distinguished, depending on whether the stimulus mean is below or above threshold. In both cases, resonance effects determine the most reliable stimulus frequency. It is shown that this frequency preference can be modulated by the peak conductance and dynamics of specific ion channels. In the third part, evidence is provided that ionic conductances determine spike timing reliability beyond changes in the preferred frequency. It is demonstrated that ionic conductances also exert a direct influence on the sensitivity of the timing of spikes to neuronal noise. The findings suggest an important role for dynamic neuromodulation of ion channels with regard to frequency selectivity and spike timing reliability.

Modell-Neuronen

Ionenkanäle

zeitliche Präzision

Frequenz-Selektivität

model neurons

ion channels

spike timing reliability

frequency selectivity

570 Biowissenschaften, Biologie

32 Biologie

WW 4120

ddc:570

Resonanzverhalten und Netzwerkoszillationen in der hippokampalen Formation der Ratte in vitro

Boehlen, Anne

06 September 2010

Rhythmische neuronale Aktivität spielt vermutlich eine wichtige Rolle in der Informationsverarbeitung im zentralen Nervensystem. Oszillationen neuronaler Netze sind heterogen, von der Hirnregion und ihrer Funktion abhängig und werden entsprechend ihrer Frequenz eingeteilt. Für ihre Entstehung sind über die Verschaltung der Neuronen und der synaptischen Übertragung hinaus insbesondere die Erregbarkeit und Oszillationseigenschaften einzelner Neurone von Bedeutung. Bestimmte Zellen der hippokampalen Formation wie zum Beispiel Sternzellen (SC) der Schicht II des Entorhinalkortex zeigen oszillatorische Aktivität und antworten verstärkt auf Stimuli einer bestimmten Frequenz – sie sind resonant. Beide Phänomene werden auf spezifische spannungsabhängige Leitfähigkeiten in der Membran zurückgeführt. Es stellte sich heraus, dass die Resonanzfrequenz von SCs durch das Muster der vorhandenen Leitfähigkeiten bestimmt wird und von der Position der Zelle entlang der dorso-ventralen Achse abhängt. Dieser Gradient ist bereits in frühen Entwicklungsstadien nachweisbar. Im Zuge der weiteren Entwicklung werden SCs weniger erregbar und der Bereich der Resonanzfrequenz dehnt sich nach dorsal aus. Pharmakologische Experimente ergaben, dass die Resonanz von SCs von HCN-Kanälen abhängt und von Kv7-Kanälen moduliert wird. Außerdem konnten zwei, bisher unbekannte Klassen von oszillatorischen Interneuronen beschrieben werden, deren Resonanz ebenfalls im Theta-Bereich liegt und auf ähnliche Leitfähigkeiten zurückgeführt werden kann. Weitere, auch CA1-Pyramidenzellen einschließende Experimente ergaben, dass HCN-Kanäle die allgemeine Voraussetzung für Resonanz zu sein scheinen während Kv7-Kanäle potente Modulatoren darstellen. Die pharmakologische Blockade dieser Kanäle unterbrach Netzwerkoszillation im Hippokampus. Dies unterstützt die These, dass bestimmte Leitfähigkeiten Neuronen Resonanzeigeschaften verleihen und somit wiederum Netzwerkoszillationen unterstützen. / Rhythmic neuronal activity is thought to be crucial for information processing in the brain. Neuronal network oscillations are heterogeneous, vary with brain region and type of information processed. They are classified according to their frequency content. Their generation relies on network circuitry, synaptic transmission and neuronal properties. Oscillatory behavior of individual cells has been particularly implicated. Different cell types within the hippocampal formation such as layer II stellate cells (SC) of the medial entorhinal cortex display oscillatory activity and are resonant, i.e., respond preferentially to stimuli of a given frequency. Voltage dependent ionic conductances have been suggested to give rise to these phenomena. It was found that resonance of SCs is defined by the composition of voltage-dependent channels embedded in their membrane and changes with their position along the dorsal-ventral axis. This gradient of SC properties develops during early postnatal life. During the transition to adulthood cells become less excitable and the range of resonance frequencies expands in the dorsal direction. Pharmacological experiments reveal the resonance of SCs to depend strongly on HCN-channels and to be modulated by Kv7-channels. Also, two previously unknown classes of oscillating interneurons were identified in the stratum radiatum of the CA1 region. These are targeted by neurons from the dentate gyrus, display frequency preferences in the theta range which relies on similar membrane conductances. Further experiments including CA1 pyramidal cells suggested HCN-channels to be the primary global requirement for resonance whereas Kv7-channels appear to be effective modulators. Pharmacological blockade of these channels disrupted ongoing network oscillations in the hippocampus. This supports the notion that specific ion channels support rhythmic activity of individual cells and in turn of entire networks.

Resonanz

hippokampale Formation

Membranpotentialoszillatonen

Netzwerkoszillationen

spannungsabhängige Ionenkanäle

resonance

hippocampal formation

membrane potential oscillations

network oscillations

voltage-dependent ion channels

570 Biowissenschaften, Biologie

32 Biologie

YG 1700

ddc:570

Elektrophysiologische Charakterisierung künstlicher Ionenkanäle in lebenden Zellen

Fidzinski, Pawel

03 May 2006

Durch Ausübung physiologischer Grundfunktionen spielen Ionenkanäle eine entscheidende Rolle für die reguläre Funktion von Zellen. Zum besseren Verständnis ihrer Struktur und Funktion sind Untersuchungen natürlicher und künstlicher Ionenkanäle wichtige Werkzeuge. Großes analytisches und therapeutisches Potential ist in der Untersuchung künstlicher Kanäle in lebenden Zellen vorhanden, was bisher wenig Beachtung fand. In der vorliegenden Arbeit wurde die Wirkung der künstlichen Ionenkanäle THF-gram, THF-gram-TBDPS sowie linked-gram-TBDPS auf elektrophysiologische Eigenschaften boviner Trabekelwerkszellen des Auges anhand von Patch-Clamp-Untersuchungen im Whole-Cell-Modus analysiert. Die Untersuchung brachte folgende Erkenntnisse: 1. Die Inkorporation aller drei Verbindungen war erfolgreich, was sich durch Anstieg der Stromdichte und Verschiebung des Umkehrpotentials zeigte. 2. Einbau von THF-gram und THF-gram-TBDPS war mit dem Überleben der Zellen vereinbar, während linked-gram-TBDPS aufgrund einer sehr potenten Antwort bereits bei sehr geringen Konzentrationen zum raschen Zelltod führte. 3. Eine Asymmetrie der Stromantwort zugunsten stärkerer Auswärtsströme wurde bei THF-gram und in schwächerer Ausprägung bei THF-gram-TBDPS festgestellt. Linked-gram-TBDPS zeigte keine derartige Asymmetrie. 4. Unter Verwendung von Cs+ als Ladungsträger war der beobachtete Anstieg der Stromdichte bei allen drei Verbindungen eindeutig stärker als unter physiologischen Bedingungen (Na+/K+). 5. Die dargestellten Erkenntnisse sind ein erster Schritt zur therapeutischen Anwendung von künstlichen Ionenkanälen. Eine Weiterentwicklung in Richtung höherer Selektivität und besserer Kontrolle ist jedoch genauso erforderlich wie die Klärung der klinischen Umsetzbarkeit. / Ion channels play a pivotal role for regular cell function. To better understand their structure and function, investigation of both natural and artificial ion channels is being performed to date. Investigation of artificial channels in living cells hides a big potential, however, little attention has been paid to this field so far. In this work, the effect of the artificial ion channels THF-gram, THF-gram-TBDPS and linked-gram-TBDPS on electrophysiological properties of bovine trabecular meshwork cells was investigated with the patch-clamp-technique. Following results were obtained: 1. Incorporation of all three compounds was successful, which was proven by increase of current density and cell depolarisation. 2. The cells survived after incorporation of THF-gram and THF-gram-TBDPS but not after linked-gram-TBDPS, which resulted in cell death at very low concentrations. 3. Larger outward currents were observed with THF-gram and, at a lower extent, with THF-gram-TBDPS. Linked-gram-TBDPS did not show such an asymmetry. 4. With Cs+ as charge carrier all three compunds showed a stronger increase of current density than under physiological conditions (Na+/K+). 5. The decribed results are a first step towards therapeutic application of artificial ion channels, however, further development towards higher selectivity and better control is as necessary as clarification of clinical feasibility.

künstliche Ionenkanäle

Patch-Clamp-Technik

Gramicidin A

Trabekelwerk des Auges

artificial ion channels

patch-clamp-technique

gramicidin A

trabecular meshwork

610 Medizin

33 Medizin

WE 5460

ddc:610

Normalisation de la fréquence cardiaque et de la conduction auriculo-ventriculaire dans des modèles de bradycardie congénitale par l'inhibition pharmacologique du courant IkACh / Inhibition of IKACh current rescues bradycardia and atrioventricular block in models of congenital sino-atrial dysfunction

Chung You Chong, Antony

16 April 2019

Correction de la bradycardie et des troubles de conduction dans des modèles de dysfonction congénitale de l’automatisme cardiaque par l’inhibition pharmacologique du courant IKAChLa dysfonction du nœud sinusal (DNS) est l’une des principales pathologies de l’automatisme cardiaque. La DNS désigne une multitude de troubles caractérisées par l’incapacité du nœud sinusal (SAN) à générer ou à conduire l’impulsion cardiaque. La seule thérapie actuellement disponible pour la DNS est l’implantation d’un pacemaker électronique. Des études épidémiologiques prévoient un besoin croissant d’implantation de pacemaker électroniques au cours des 50 prochaines années à cause du vieillissement de la population. Le développement des thérapies innovantes pour la DNS est donc un enjeu médical et sociétal important. L’inhibition pharmacologique du courant potassique activé par l’acétylcholine (IKACh) pourrait constituer une nouvelle option thérapeutique pour traiter la DNS.Nous avons donc testé l’inhibition du courant IKACh par un peptide de venin d’abeille, la Tertiapine-Q, pour corriger le DNS et le dysfonctionnement de la conduction chez des souris modèle de pathologies cardiaque humaine en particulier les souris portant l’inactivation des canaux L Cav1.3 (Cav1.3-/-), les souris portant simultanément l’ablation de Cav1.3 et des canaux de type-T Cav3.1 (Cav1.3-/-/Cav3.1-/-), les souris porteuses de la perte de fonction des canaux f- (HCN4-CNBD) et les souris haplo-suffisantes Nav1.5 (Scn5a+/-).Nous avons enregistré par télémétrie, l’ECG, chez ces modèles murins avant et après l’administration de différentes doses de Tertiapine-Q.L’inhibition du courant IKACh par la Tertiapine-Q prévient des dysfonctions sinusales et améliore la conduction dans ces modèles de bradycardie congénitale suggérant la possibilité d’un développement d’un ciblage pharmacologique d’IKACh afin de parvenir à corriger la DNS et les troubles de la conduction. / Inhibition of KACh channels by the bee venom peptide tertiapin-Q rescues inherited cardiac conduction defects, sino-atrial bradycardia, and atrioventricular block in models of congenital dysfunctionSinus node dysfunction (SND) is a widespread disease of heart automaticity. SND refers to a multitude of sinus node (SAN) disorders characterized by failure to generate or conduct the cardiac impulse. The only currently available therapy for chronic SND is the implantation of an electronic pacemaker. Epidemiological studies forecast an increasing need for pacemaker implantation during the next 50 years, with the ageing of the population. It is thus an important medical and societal issue, to develop innovative therapies for SND. Pharmacologic inhibition of the G-protein activated K+ current (IKACh) could be a new therapeutic option to treat bradycardia and SND associated with other cardiac pathologies.We tested whether inhibition of IKAch by the peptide Tertiapin-Q could rescue SND and conduction dysfunction in Cav1.3-/- mice carrying concurrent ablation of L-type Cav1.3 and T-type Cav3.1 channels (Cav1.3-/-/Cav3.1-/-), mice carrying loss-of-function of f-channels (HCN4-CNBD) and Nav1.5 haploinsufficient (Scn5a+/-) mice.We employed telemetric ECG recordings of heart rate (HR), SAN pacemaking and AV dysfunction in mice before and after administration of different doses of Tertiapin-Q.Tertiapin-Q significantly improves the HR of Cav1.3-/-, Cav1.3-/-/Cav3.1-/-, and HCN4-CNBD from doses of 0.1 to 5 mg/kg. HRs of Tertiapin-Q-treated mice were similar to those recorded in untreated wild-type mice. Tertiapin-Q also improved cardiac conduction of Scn5a+/- mice by 24%.Pharmacological inhibition of IKAch by Tertiapin-Q prevents SAN dysfunction and improves conduction in three models of congenital bradycardia suggesting the possibility of pharmacologic development of IKACh targeting to manage SND and conduction disease, to delay or replace the implantation of an electronic pacemaker.

Activité pacemaker cardiaque

Canaux ioniques

Maladie rythmique

Pharmacologie

Noeud sinusal

Courant IKAch

Cardiac pacemaker activity

Ion channels

Sick sinus syndrome

Pharmacology

Sino-Atrial node

IKACh

Ionenkanäle in deaktivierter Mikroglia

Eder, Claudia

10 April 2001

In der vorliegenden Habilitationsarbeit wurden die Ionenkanäle von Mikrogliazellen mit Hilfe der Patch-clamp-Technik untersucht, nachdem die Mikrogliazellen in den deaktivierten Zustand überführt worden waren. Die Deaktivierung der Mikroglia erfolgte durch die Zugabe des astrozytenkonditionierten Mediums. Nach der Deaktivierung exprimierten die Mikrogliazellen einwärts- und auswärtsgleichrichtende sowie Ca2+-aktivierte Kaliumkanäle. Der auswärtsgleichrichtende Kaliumkanal wurde erst nach Zugabe des astrozytenkonditionierten Mediums exprimiert, wobei das durch die Astrozyten freigesetzte Zytokin transformierender Wachstumsfaktor für diesen Prozeß verantwortlich gemacht werden konnte. Zusätzlich wurden Chloridkanäle an deaktivierten Mikrogliazellen nachgewiesen, die an den Ramifizierungsprozessen der Zellen, d.h. dem Übergang von der amöboiden in die ramifizierte Zellmorphologie, beteiligt waren. Die an Mikrogliazellen exprimierten Protonenkanäle spielen offensichtlich eine wichtige Rolle bei der Generierung von reaktiven Sauerstoffradikalen und wurden im Prozeß der Deaktivierung der Mikrogliazellen herunterreguliert. / The current work describes patch clamp recordings in cultured murine microglial cells, which had been deactivated following exposure to astrocyte-conditioned medium. Deactivated microglial cells expressed inwardly rectifying, outwardly rectifying and calcium-activated potassium channels. The outwardly rectifying potassium channels were upregulated following treatment of microglial cells with the astrocyte-conditioned medium. The anti-inflammatory cytokine transforming growth factor was released by astrocytes and appeared to be responsible for the observed upregulation of outwardly rectifying potassium channels in deactivated microglia. In addition, deactivated microglial cells expressed chloride channels, which were found to be involved in microglial ramification, i.e., in the transformation of microglial cells from ameboid into ramified morphology. Voltage-gated proton channels, which are involved in processes of oxygen radical generation, were downregulated in deactivated microglial cells.

Mikroglia

Ionenkanäle

Patch-clamp-Technik

Deaktivierung

Microglia

ion channels

patch clamp technique

deactivation

610 Medizin

33 Medizin

WW 1620

ddc:610

Computer Simulation of Biological Ion Channels

Hoyles, Matthew, Matthew.Hoyles@anu.edu.au

January 2000

This thesis describes a project in which algorithms are developed for the rapid and accurate solution of Poisson's equation in the presence of a dielectric boundary and multiple point charges. These algorithms are then used to perform Brownian dynamics simulations on realistic models of biological ion channels. An iterative method of solution, in which the dielectric boundary is tiled with variable sized surface charge sectors, provides the flexibility to deal with arbitrarily shaped boundaries, but is too slow to perform Brownian dynamics. An analytical solution is derived, which is faster and more accurate, but only works for a toroidal boundary. Finally, a method is developed of pre-calculating solutions to Poisson's equation and storing them in tables. The solution for a particular configuration of ions in the channel can then be assembled by interpolation from the tables and application of the principle of superposition. This algorithm combines the flexibility of the iterative method with greater speed even than the analytical method, and is fast enough that channel conductance can be predicted. The results of simulations for a model single-ion channel, based on the acetylcholine receptor channel, show that the narrow pore through the low dielectric strength medium of the protein creates an energy barrier which restricts the permeation of ions. They further show that this barrier can be removed by dipoles in the neck of the channel, but that the barrier is not removed by shielding by counter-ions. The results of simulations for a model multi-ion channel, based on a bacterial potassium channel, show that the model channel has conductance characteristics similar to those of real potassium channels. Ions appear to move through the model multi-ion channel via rapid transitions between a series of semi-stable states. This observation suggests a possible physical basis for the reaction rate theory of channel conductance, and opens up an avenue for future research.

computer simulation

ion channels

conductance theories

electrostatics

Brownian dynamics

single-ion channel

multi-ion channel

Poisson's equation

dielectric boundary

potassium channel

The effect of long-term interleukin-1 beta exposure on sensory neuron electrical membrane properties: implications for neuropathic pain

Stemkowski, Patrick

06 1900

The effect of interleukin-1 beta (IL-1β) on the electrical properties of sensory neurons was assessed at comparable levels and exposure times to those found in animal models of neuropathic pain. Experiments involved whole cell current- or voltage-clamp recordings from rat dorsal root ganglion (DRG) neurons in defined medium, neuron enriched cultures. 5-6 days exposure to 100 pM IL-1β produced neuron specific effects. These included an increase in the excitability of medium diameter and small diameter isolectin B4 (IB4)-positive neurons that was comparable to that found after peripheral nerve injury. By contrast, a reduction in excitability was observed in large diameter neurons, while no effect was found in small diameter IB4-negative neurons. Further characterization of changes in medium and small IB4-positive neurons revealed that some, but not all, effects of IL-1β were mediated through its receptor, IL-1RI. Using appropriate voltage protocols and/or ion substitutions, it was found that neuron specific changes in several ionic currents, including alterations in hyperpolarization activated inward current (IH) and decreases in various K+ currents contribute to the increased excitability produced by IL-1β. Overall, these studies revealed that: 1. The effects of long-term exposure of DRG neurons to IL-1β are reflective of the enduring increase in primary afferent excitability reported after peripheral nerve injury. This expands the recognized role of IL-1β in acute inflammatory pain to neuropathic pain. 2. Hyperexcitability in medium neurons exposed to IL-1β likely includes mixed populations of neurons corresponding to nociceptive and non-nociceptive primary afferent fibres and, therefore, has relevance to hyperalgesia and allodynia, respectively. 3. The responsiveness of small IB4-positive neurons, but not IB4-negative, to prolonged IL-1β exposure is consistent with the suggestion that small IB4-negative afferents are involved in inflammatory pain, while small IB4-positive afferents are involved neuropathic pain. 4. The identification of receptor mediated effects and several contributing ionic mechanisms, may have relevance to the development of new therapeutic approaches to neuropathic pain. 5. IL-1β can contribute to increased neuronal excitability by mechanisms that are independent of IL-1RI signalling. This should be taken into account when targeting IL-1β, or more specifically IL-1RI, in the management of neuropathic pain.

sensory neurons

dorsal root ganglion

interleukin-1 beta

neuropathic pain

electrophysiology

cell culture

excitability

ion channels

peripheral nerve injury

central sensitization

Assessment of Cerebellar and Hippocampal Morphology and Biochemical Parameters in the Compound Heterozygous, Tottering/leaner Mouse

Murawski, Emily M.

2009 December 1900

Due to two different mutations in the gene that encodes the a1A subunit of voltage-activated CaV 2.1 calcium ion channels, the compound heterozygous tottering/leaner (tg/tgla) mouse exhibits numerous neurological deficits. Human disorders that arise from mutations in this voltage dependent calcium channel are familial hemiplegic migraine, episodic ataxia-2, and spinocerebellar ataxia 6. The tg/tgla mouse exhibits ataxia, movement disorders and memory impairment, suggesting that both the cerebellum and hippocampus are affected. To gain greater understanding of the many neurological abnormalities that are exhibited by the 90-120 day old tg/tgla mouse the following aspects were investigated: 1) the morphology of the cerebellum and hippocampus, 2) proliferation and death in cells of the hippocampal dentate gyrus and 3) changes in basic biochemical parameters in granule cells of the cerebellum and hippocampus. This study revealed no volume abnormalities within the hippocampus of the mutant mice, but a decrease in cell density with the pyramidal layer of CA3 and the hilus of the dentate gyrus. Cell size in the CA3 region was unaffected, but cell size in the hilus of the dentate gyrus did not exhibit the gender difference seen in the wild type mouse. The cerebellum showed a decrease in volume without any decrease in cerebellar cellular density. Cell proliferation and differentiation in the subgranular zone of the hippocampal dentate gyrus remained normal. This region also revealed a decrease in cell death in the tg/tgla mice. Basal intracellular calcium levels in granule cells show no difference within the hippocampus, but an increase in the tg/tgla male cerebellum compared to the wild type male cerebellum. There was no significant difference in granule cell mitochondrial membrane potential within the wild type and mutant animals in either the hippocampus or cerebellum. The rate of reactive oxygen species (ROS) production in granule cells revealed no variation within the hippocampus or cerebellum. The amount of ROS was decreased in cerebellar granule cells, but not granule cells of the hippocampus. Inducing ROS showed no alteration in production or amount of ROS produced in the hippocampus, but did show a ceiling in the amount of ROS produced, but not rate of production, in the cerebellum.

Cerebellum

Hippocampal neurogenesis

Voltage-gated calcium ion channels

Mitochondrial membrane potential

Intracellular Calcium Dynamics In Dendrites Of Hippocampal Neurons Rendered Epileptic And In Processes Of Astrocytes Following Glutamate Pretreatment

Padmashri, R

08 1900

The fundamental attribute of neurons is their cellular electrical excitability, which is based on the expression of a plethora of ligand- and voltage-gated membrane channels that give rise to prominent membrane currents and membrane potential variations that represent the biophysical substrate underlying the transfer and integration of information at the cellular level. Dendrites have both an electrical and a biochemical character, which are closely linked. In contrast, glial cells are non-electrically excitable but nevertheless display a form of excitability that is based on variations of the Ca2+ concentration in the cytosol rather than electrical changes in the membrane. Cytoplasmic Ca2+ serves as an intracellular signal that is responsible for controlling a multitude of cellular processes. The key to this pleiotropic role is the complex spatiotemporal organization of the [Ca2+]i rise evoked by extracellular agonists, which allows selected effectors to be recruited and specific actions to be initiated. Ca2+ handling in the cell is maintained by operation of multiple mechanisms of Ca2+ influx, internal release, diffusion, buffering and extrusion. Ca2+ tends to be a rather parochial operator with a small radius of action from its point of entry at the cytoplasm resulting in the concept of microdomains. Dendritic Ca2+ signaling have been shown to be highly compartmentalized and astrocytic processes have been reported to be constituted by hundreds of microdomains that represent the elementary units of the astrocyte Ca2+ signal, from where it can eventually propagate to other regions of the cell. The astrocyte Ca2+ elevation may thus act as intra and intercellular signal that can propagate within and between astrocytes, signaling to different regions of the cell and to different cells. The spatio-temporal features of neuron-to-astrocyte communication, results from diverse neurotransmitters and signaling pathways that converge and cooperate to shape the Ca2+ signal in astrocytes. Alterations in Ca2+ homeostasis have been shown to be associated with major pathological conditions of the brain such as epilepsy, ischemia and neurodegenerative diseases. Although there are evidences of Ca2+ rise in hippocampal neurons in in vitro models of epilepsy (Pal et al., 1999; Limbrick et al., 2001), there is no information on the Ca2+ regulatory mechanisms operating in discrete compartments of the epileptic neuron following Ca2+ influx through voltage gated calcium channels (VGCCs). In the first part of the work, the spatial and temporal profiles of depolarization induced changes in the intracellular Ca2+ concentration in the dendrites of cultured autaptic hippocampal pyramidal neurons rendered epileptic experimentally have been addressed. Our in vitro epilepsy model consisted of hippocampal neurons in autaptic culture that were grown in the presence of kynurenate and high Mg2+, and subsequently washing the preparation free of the blockers. To understand the differences in Ca2+ handling mechanisms in different compartments of a control neuron and the kynurenate treated neuron, a combination of whole-cell patch-clamp recording and fast Ca2+ imaging methods using the Ca2+ indicator Oregon Green 488 BAPTA-1 was applied. All our analysis was focused on localized regions in the dendrite that showed pronounced Ca2+ transients upon activation of high voltage activated (HVA) Ca2+ channels. The spatial extent of Ca2+ signals suggested the presence of distinct dendritic compartments that respond to the depolarizing stimulus. Further, the local Ca2+ transients were observed even in the presence of NMDA and AMPA receptor antagonists, suggesting that the opening of VGCCs primarily triggered the local Ca2+ changes. The prominent changes in intracellular Ca2+ observed in these dendritic regions appear to be sites where Ca2+ evoked dendritic exocytosis (CEDE) takes place. Since cellular Ca2+ buffers determine the amplitude and diffusional spread of neuronal Ca2+ signals, quantitative estimates of the time-dependent spread of intracellular Ca2+ in the dendritic compartments in the control and treated neurons were done using image processing techniques. Physiological changes in Ca2+ channel functioning were also induced by kynurenate treatment and one such noticeable difference was the observation of Ca2+ dependent inactivation in the treated neurons. We provide evidences of localized Ca2+ changes in the dendrites of hippocampal neurons that are rendered epileptic by kynurenate treatment, suggesting that these sites are more vulnerable (Padmashri et al., 2006). This might contribute to the epileptiform activity by local changes in cellular and membrane properties in complex ways that remains to be clearly understood. Status Epilepticus (SE), stroke and traumatic brain injury are all associated with large increases in extracellular glutamate concentrations. The concentration of glutamate in the extracellular fluid is around 3-4 µM and astrocytes are primarily responsible for the uptake of glutamate at the synapses. The extracellular levels of glutamate has been shown to increase dramatically (16 fold) in human SE suggesting an important role of glutamate in the mechanism of seizure activity and seizure related brain damage (Carlson et al., 1992). Several other studies have also shown a persistent increase in extracellular glutamate concentration to potentially neurotoxic concentrations in the epileptogenic hippocampus (During and Spencer, 1993; Sherwin, 1999; Cavus et al., 2005). We addressed the problem related to the effects of prolonged glutamate pretreatment on Ca2+ signaling in an individual astrocyte and its adjoining astrocyte (astrocyte pair), rather than on a syncytium of astrocytes in culture. Individual astrocytes may have functional domains that respond to an agonist through distinct receptor signaling systems. These are difficult to observe in studies that are done on glial syncytium because of spatial limits of image capture. This was examined with simultaneous somatic patch-pipette recording of a single astrocyte to evoke voltage-gated calcium currents, and Ca2+ imaging using the Ca2+ indicator Oregon Green 488 BAPTA-1 to identify the Ca2+ microdomains. Transient Ca2+ changes locked to the depolarization were observed in certain compartments in the astrocyte processes of the depolarized astrocyte and the responses were more pronounced in the adjoining astrocyte of the astrocyte pair. The Ca2+ transient amplitudes were enhanced on pretreatment of cells with glutamate (500 µM for 20 minutes). Estimation of local Ca2+ diffusion coefficients in the astrocytic processes indicated higher values in the adjoining astrocyte of the glutamate pretreated group. In order to understand the underlying mechanisms, we performed the experiments in the presence of different blockers for the metabotropic glutamate receptor, inositol 1,4,5 triphosphate (IP3) receptors and gap junctions. Ca2+ transients recorded on pretreatment of cells with glutamate showed attenuated responses in the presence of the metabotropic glutamate receptor (mGluR) antagonist α-Methyl(4-Carboxy-Phenyl) Glycine (MCPG). Intracellular heparin (an antagonist of IP3 receptor) introduced in the depolarized astrocyte did not affect the Ca2+ transients in the heparin loaded astrocyte, but attenuated the [Ca2+]i responses in the adjoining astrocyte suggesting that IP3 may be the transfer signal. The uncoupling agent 1-Octanol attenuated the [Ca2+]i responses in the adjoining cell of the astrocyte pair in both the control and glutamate pretreated astrocytes indicating the role of gap junctional communication. The findings of [Ca2+]i responses within discrete regions of astrocytic processes suggest that astrocytes may be comprised of microdomains whose properties are altered by glutamate pretreatment. The data also indicates that glutamate induced alterations in Ca2+ signaling in the astrocyte pair may be mediated through phospholipase C (PLC), IP3, internal Ca2+ stores, VGCCs and gap junction channels (Padmashri and Sikdar, 2006). Neuronal (EAAC-1) and glial (GLT-1 and GLAST) glutamate transporters facilitate glutamate reuptake after synaptic release. Transgenic mice with GLT-1 knockout display spontaneous epileptic activity (Tanaka et al., 1997) and loss of glial glutamate transporters using chronic antisense nucleotide administration was reported to result in elevated extracellular glutamate levels and neurodegeneration characteristic of excitotoxity (Rothstein et al., 1996). Dysfunction of glutamate transporters and the resulting increase of glutamate have been speculated to play an important role in infantile epilepsies (Demarque et al., 2004). We examined the effects of pretreatment with glutamate in the presence of the glutamate transport inhibitor threo-β-hydroxy-aspartate (TBHA) and in Na+-free extracellular medium to understand whether this resulted in any alteration in the astrocytic intracellular Ca2+ dynamics following activation of voltage gated calcium channels. The Ca2+ responses were found to be attenuated in both the cases indicating that the elevated levels of extracellular glutamate due to blockade of glutamate transporters may influence the responses mediated by the astrocytic glutamate receptors. Our studies indicate that the heightened extracellular glutamate concentration is not gliotoxic in our experimental system, although it may have a profound effect on altering the activity of surrounding neurons which was not addressed in the present work. Several studies have indicated that neurons control the level of gap junction mediated communication between astrocytes (Giaume and McCarthy, 1996; Rouach et al, 2000). All our earlier studies were done on process bearing astrocytes that were co-cultured with neurons. We have addressed the question as to whether the spatio-temporal changes in [Ca2+]i in astrocyte pairs differ if the astrocytes are cultured in the absence of neurons. The results indicate that there is indeed a significant reduction in the responses that are evoked in response to the depolarization pulse in the adjoining cell of the astrocyte pair. These experiments demonstrate that neurons in the cocultures may selectively enhance the Ca2+ responses possibly by increasing the coupling between the two cells.

Calcium - Biochemistry

Calcium Ion Signaling

Voltage-gated Ion Channels

Hippocampal Neurons

Astrocytes

Calcium Dynamics

Glutamate

Dendrites

Status Epilepticus (SE)

Astrocyte Pairs

Biochemistry

The effect of long-term interleukin-1 beta exposure on sensory neuron electrical membrane properties: implications for neuropathic pain

Stemkowski, Patrick

Unknown Date

No description available.

sensory neurons

dorsal root ganglion

interleukin-1 beta

neuropathic pain

electrophysiology

cell culture

excitability

ion channels

peripheral nerve injury

central sensitization