Kv1.1 RNA Editing: Physiological Roles and its Implications for Episodic Ataxia Type-1

Kiddie, Elizabeth Ferrick

16 March 2017

Kv1.1 voltage-gated potassium channels serve as key regulators of neuronal function and mutations in Kv1.1 lead to the human movement and epilepsy-related disorder, Episodic Ataxia type-1 (EA1). Transcripts encoding Kv1.1 may be modified by a site-specific adenosine-to-inosine RNA editing event, leading to the expression of an altered protein with an isoleucine to valine change at amino acid 400 (I400V). The non-edited [Kv1.1(I)] and edited [Kv1.1(V)] channels display altered functions in heterologous expression systems, but their significance in normal physiology and with regard to EA1 have not been characterized. We have developed new mouse models which solely express either the non-edited [Kv1.1(I)] or edited [Kv1.1(V)] isoforms of the channel. Our studies have revealed that both mice display conditional postnatal lethality and that the non-edited [Kv1.1(I)] mice exhibit an EA1-like disorder, stress-induced motor dyscoordination. In addition, we observed that editing altered drug-induced seizure-susceptibility for these mutant mouse models. Mice expressing the non-edited [Kv1.1(I)] channel exhibited a lowered threshold for drug-induced seizures, whereas mutant animals expressing the edited [Kv1.1(V)] channel exhibited an increased threshold. To further characterize the collective effects of Kv1.1 editing in transcripts containing human EA1 mutations, we discovered that three mutations (V404I, I407M, and V408A), in close proximity to the editing site, decreased Kv1.1 RNA editing in vitro. Utilizing the V408A/+ mouse model of EA1, we confirmed that the V408A mutation leads to decreases in Kv1.1 RNA editing in vivo. Electrophysiological characterization of the edited EA1 mutant channels also indicated that these channel isoforms display channel dysfunctions unique to each mutation, as compared to their respective non-edited EA1 channels. Thus, Kv1.1 RNA editing has a substantial impact on normal physiology and may be dysregulated in the EA1 disorder, as well as contribute to the wide variety in symptom severity observed in EA1 patients.

Molecular Physiology and Biophysics

Exploring the Function of G6PC2 in Pancreatic Islet Beta Cells

Boortz, Kayla

03 October 2016

MOLECULAR PHYSIOLOGY & BIOPHYSICS Exploring the Function of G6PC2 in Pancreatic Islet Beta Cells Kayla Boortz Dissertation under the direction of Professor Richard OâBrien, Ph.D. G6PC2 encodes an islet-specific glucose-6-phosphatase catalytic subunit. Together with glucokinase, G6PC2 forms a substrate cycle that determines the glucose sensitivity of insulin secretion. Genetic and molecular studies show that elevated G6PC2 expression raises fasting blood glucose (FBG) but because chronically elevated FBG is detrimental, increasing type 2 diabetes risk, it is unclear why G6PC2 evolved. Studies have shown that single nucleotide polymorphisms (SNPs) in G6PC2 associate with variation in FBG and body mass index (BMI) in humans. Previously we confirmed these findings in mice and showed that FBG is repressed in G6pc2 knockout (KO) mice relative to wild type (WT) on a mixed or pure C57BL/6J genetic background. I further confirmed that 129SvEv KO mice also have reduced FBG. Moreover, I identified a glucocorticoid response element in the human and 129SvEv G6pc2 promoter that confers glucocorticoid responsiveness and induction of G6PC2 gene expression following treatment with Dexamethasone (Dex), 11-dehydrocorticosterone (11-DHC) or physical restraint in 129SvEv and C57BL/6J mice. Following stress generated by Dex or physical restraint, FBG is repressed in 6 hour fasted 129SvEv and C57BL/6J KO mice, respectively, enhancing the difference in FBG relative to controls. These data suggest that G6PC2 evolved to modulate FBG under conditions of glucocorticoid-related stress thereby conferring a transient, beneficial modulation of the set point for FBG. This thesis also addresses the observation that the common rs560887 G6PC2 SNP is associated with variation in BMI and adiposity. The results described here indicate that the effect of G6pc2 deletion on the response to diet induced obesity is dependent on genetic modifiers. Finally, an indirect analysis of the effects of human G6PC2 SNPs on protein expression and enzyme activity indicates that mutations at catalytically conserved residues may be critical for proper enzyme function and protein expression.

Molecular Physiology and Biophysics

Mechanism of Hic-5/ARA55 action, a novel stromal-specific nuclear receptor coactivator

Heitzer, Marjet Danteel

20 December 2005

Hydrogen peroxide inducible clone-5/Androgen Receptor Activator 55 (Hic-5/ARA55) is a group III LIM domain protein that functions at focal adhesion complexes as well as in the nucleus as a nuclear receptor coactivator. Because the interaction of the androgen receptor (AR) with Hic-5/ARA55 results in enhanced androgen-induced transcription, we analyzed Hic-5/ARA55 expression in prostate tissue sections from normal human donors and prostate cancer patients. In each sample, Hic-5/ARA55 expression was confined to the stromal compartment of the prostate. Furthermore, in a human prostate stromal cell line (i.e. WPMY-1 cells) Hic-5/ARA55 was localized both at focal adhesion complexes and within the soluble cytoplasmic compartment. The ability of Hic-5/ARA55 to shuttle between the nuclear and cytoplasmic compartments within WPMY-1 cells was revealed upon inhibition of nuclear export with leptomycin B (LMB). siRNA ablation experiments established endogenous Hic-5/ARA55 as a coactivator for both viral and endogenous cellular AR-regulated genes. Furthermore, chromatin immunoprecipitation (ChIP) analysis showed androgen-dependent recruitment of Hic-/ARA55 to the promoter of the stromal androgen-responsive KGF gene. Using the A1-2 derivative of T47D breast cancer cells, we examined the mechanism by which Hic-5/ARA55 potentiates nuclear receptor transactivation. Hic-5/ARA55 was found to be an important component of glucocorticoid receptor (GR)-coactivator complexes in A1-2 cells since ablation of Hic-5/ARA55 expression by RNA interference-mediated silencing reduced GR transactivation. As shown by ChIP assays, Hic-5/ARA55 is recruited to glucocorticoid-responsive promoters of the MMTV, c-fos, and p21 genes in response to glucocorticoid treatment. Results from sequential ChIP assays established that Hic-5/ARA55 associates with the corepressor, NCoR, in the absence of glucocorticoids. However, upon glucocorticoid stimulation, Hic-5/ARA55 interacts with GR-coactivator containing complexes at these promoters. Ablation of Hic-5/ARA55 expression resulted in reduction of both TIF-2 and p300 recruitment to glucocorticoid-responsive promoters. These data provide the first demonstration of a stromal-specific AR coactivator that has an impact on an androgen regulated growth factor that is essential for stromal/epithelial cell communication in the prostate. Furthermore, these results suggest that Hic-5/ARA55 is required for optimal GR-mediated gene expression possibly by providing a scaffold that organizes or stabilizes coactivator complexes at some hormone-responsive promoters.

Cell Biology and Molecular Physiology

Regulation of apical vesicle formation from the trans-Golgi network

Ellis, Mark A

27 April 2006

Polarized epithelial cells efficiently sort newly-synthesized apical and basolateral proteins into distinct transport carriers that emerge from the trans-Golgi network (TGN), and this sorting may be recapitulated in nonpolarized cells. While the targeting signals of basolaterally-destined proteins are generally cytoplasmically-disposed, apical sorting signals are not typically accessible to the cytosol, and the transport machinery required for segregation and export of apical cargo remain largely unknown. We are interested in identifying the molecular requirements for TGN export of the apical marker influenza hemagglutinin (HA). To identify cytosolic proteins responsible for HA export from the TGN, we developed an in vitro assay to measure this process. We found that HA export does not require the brefeldin A-sensitive GTPase ARF1, but does depend on the GTPase dynamin 2. Furthermore, using biochemical fractionation, we identified the adaptor protein 14-3-3 epsilon as an effector of HA export from the TGN. This work 1) establishes a method to accurately observe anterograde TGN export of an apical cargo, 2) characterizes a requirement for GTP in vesicle formation, and 3) identifies a novel component in trafficking from the TGN. We expand these studies by comparing HA export to the release of basolateral cargo, showing that nonpolarized cells are capable of differentially sorting distinct classes of cargo into discrete vesicles derived from the TGN. Together, these data further our understanding of the regulatory mechanisms underlying apical transmembrane protein export from the TGN.

Cell Biology and Molecular Physiology

Muscle Insulin Resistance: Novel Mechanisms and New Treatment Targets

Bonner, Jeffrey Scott

28 May 2013

This project investigated the significance of extramyocellular barriers to the pathogenesis of skeletal muscle insulin resistance and their potential as therapeutic targets. The goals of this dissertation were to determine the impact of capillary rarefaction to muscle insulin resistance, the efficacy of the vasoactive and extracellular matrix degrading hormone relaxin to rescue muscle insulin resistance, and the effects of high fat-feeding on caveolae microstructures within skeletal muscle capillaries. Data from obese patients and animal experiments describe a strong association between peripheral insulin resistance and attenuation of skeletal muscle capillary density. Whether the relationship of capillary density and the development of skeletal muscle insulin resistance are casual remains to be elucidated. We utilized a genetic mouse model with muscle-specific deletion of vascular endothelial growth factor-A (VEGF) to induce capillary rarefaction in otherwise lean, healthy mice. VEGF deficient mice had 60% fewer muscle capillaries inducing impairment in muscle insulin action. Furthermore, we investigated the therapeutic potential of targeting the vascular dysfunction and extracellular matrix remodeling associated with a high fat diet with a pharmacological dose of the endogenous hormone relaxin. A 3 week relaxin intervention in high fat-fed C57BL/6J mice rescued the metabolic and vascular dysfunction caused by the diet. The interplay between vascular and metabolic disease are significant mortality risk factors and the extramyocellular adaptations to an obesogenic diet are viable pharmacological targets. The transport of insulin across the capillary wall is rate-limiting to the onset of skeletal muscle insulin action. Transendothelial insulin transport is dependent on caveolae structures of the endothelial layer of muscle capillaries. Employing transmission electron microscopy, we show for the first time that caveolae number in muscle capillaries of 16 week high-fat fed mice are diminished compared to low fat-fed controls. These data suggest a contribution of diminished caveolae density in transendothelial insulin transport, thus augmenting the barrier for insulin delivery. In conclusion, the experiments performed in this dissertation support the paradigm that extramyocellular barriers to insulin-stimulated muscle glucose uptake are significant to the etiology of insulin resistance and these barriers provide novel targets for the treatment of vascular and metabolic disorders associated with obesity.

Molecular Physiology and Biophysics

OBESITY DYSLIPIDEMIA: THE EFFECT OF CENTRAL NERVOUS SYSTEM NEUROPEPTIDE Y ON HEPATIC LIPOPROTEIN METABOLISM

Rojas, Jennifer Marie

22 March 2013

Elevated very low-density lipoprotein (VLDL)-triglyceride (TG) secretion from liver contributes to atherogenic dyslipidemia that is associated with obesity, diabetes, and the metabolic syndrome. Numerous models of obesity are characterized by increased central nervous system (CNS) neuropeptide Y (NPY) tone which contributes to positive energy balance and obesity. In fact, an acute, single intracerebroventricular (ICV) administration of NPY in lean fasted rats elevates hepatic VLDL-TG secretion. Thus, our overarching hypothesis is that elevated CNS NPY action contributes to dyslipidemia by activating central circuits that modulate liver lipid metabolism. Our studies focused on identifying molecular determinants in the hypothalamus and the liver by which increased CNS NPY signaling modulates hepatic lipoprotein metabolism. First, we sought to determine if the effects of NPY on feeding and/or obesity are dissociable from effects on hepatic VLDL-TG secretion. ICV NPY-treated chow-fed rats pair-fed to vehicle-treated controls develop hypertriglyceridemia in the absence of increased food intake and body fat accumulation. Acute ICV injection of selective Y1, Y2, Y4, and Y5 receptor agonists all induced hyperphagia in lean ad-libitum fed rats with the Y2 receptor agonist having the most pronounced effect. The NPY Y1 receptor agonist robustly stimulated hepatic VLDL-TG secretion, while a Y2 receptor agonist had a modest effect on VLDL-TGs, and no effect was observed for Y4 and Y5 receptor agonists in lean fasted rats. These findings raise the possibility that NPY regulates feeding and lipoprotein metabolism partially via separate NPY receptor systems and/or mechanisms. Lastly, we sought to identify novel regulatory mechanisms in the liver engaged by CNS NPY signaling. We observed, in ICV NPY- and Y1 agonist-treated lean fasted rats, that oleic and linoleic acid were enriched in the liver phospholipid (PL) pool and secreted into plasma TGs. Furthermore, CNS NPY signaling via the Y1 receptor robustly activated key hepatic regulatory enzymes, ADP-ribosylation factor-1 and lipin-1, involved in remodeling liver PL into TG for VLDL maturation and secretion. Altogether, this body of work has overarching implications in further understanding how obesity-related CNS dysfunction contributes to the pathophysiology of atherogenic dyslipidemia associated with obesity, diabetes, and the metabolic syndrome.

Molecular Physiology and Biophysics

GENETIC AND PHENOTYPIC DISSECTION OF AUTISM SUSCEPTIBILITY

McCauley, Jacob Lee

09 March 2005

Autism is a severe neurodevelopmental disorder characterized by deficits in language and social interaction, and patterns of repetitive and stereotyped behaviors, interests and activities. Evidence indicates that autism has a predominantly genetic etiology, and that as many as fifteen genes may contribute to disease susceptibility. One model suggests autism may result from oligogenic inheritance, with locus heterogeneity, such that different families or individuals possess a different mix of susceptibility alleles. In this dissertation, I present genome-wide linkage studies of autism and traits comprising the aspects of the broader phenotype to identify autism susceptibility loci. I further document detailed molecular and genetic analyses of candidate genes in regions detected by linkage, and in the case of 15q11-q13, as chromosomal duplications found in 1-3% of autism cases. A unifying theme to my dissertation is the focus of genetic studies on genes acting within candidate neurobiological systems suspected of involvement in autism. Genetic analyses include linkage, linkage refinement, construction of detailed linkage disequilibrium (LD) and corresponding haplotype maps across candidate loci, and tests for transmission disequilibrium of single markers and haplotypes. Molecular studies of select candidates aim to identify functional variation on associated alleles; in the absence of association they seek to identify potential rare disease-related variants considering for example evolutionarily conserved sequence. I hypothesize that there are allelic variants, which underlie genetic linkage and/or association to autism and related traits, and these contribute to autism susceptibility through both direct and interactive effects. The goal of this study is to dissect the genetic etiology of autism by leveraging trait-based phenotypic subsets of autism using the approaches and tools I have outlined here.

Molecular Physiology and Biophysics

THE IMPACT OF INTERLEUKIN-6 ON THE METABOLIC RESPONSE TO ENDOTOXIN in vivo

Tweedell, Andrea Donielle

29 July 2005

Inflammation and insulin resistance are characteristics of endotoxemia. While the role of interleukin-6 (IL-6) in insulin resistant states has been characterized, little is known of its role in the metabolic response to inflammation. To study the role of IL-6, conscious chronically catheterized mice were used. Five days prior to being studied, catheters were implanted in the carotid artery and jugular vein. After a 5 h fast, E.coli (250 microgram/mouse) LPS was injected in IL6-/- (KO; n=13), IL6+/- (HET; n=9), and IL-6+/+ (WT; n=10) littermates. The IL-6 response to LPS was simulated in an additional group of KO mice (KO+IL6; n=10). Glucose turnover (Ra) was assessed using 3-[3H]-D-glucose. IL-6 increased similarly in WT and HET (15±0.7 and 14±0.5 ng/ml) 4h after LPS and was undetectable in KO. IL-6 replacement in KO restored circulating IL-6 to levels observed in the WT group (14±0.3 ng/ml). WT was the only group to experience an early rise in tumor necrosis factor-alpha (TNF-alpha). Interleukin-1beta (IL-1beta) was similar in all groups. KO exhibited a more profound hyperglycemia 30 min after LPS injection and no apparent hypoglycemia at 4h (95±5 mg/dl). Glucose levels in KO+IL6, while decreased (93±4 mg/dl) at 4h, remained higher than WT. Ra was not altered. In summary, the absence of IL-6 protected against LPS induced hypoglycemia. Acute restoration of the IL-6 response to LPS did not potentiate hypoglycemia. Thus, while IL-6 promotes glucose intolerance in insulin resistant states, IL-6 promotes hypoglycemia during inflammation.

Molecular Physiology and Biophysics

The Regulation of Net Hepatic Glucose Uptake in vivo

DiCostanzo, Catherine Anne

02 November 2005

It is well known that the arterial plasma insulin/glucagon level, the hepatic glucose load, and the route of glucose delivery (the portal glucose signal) are the three major determinants of NHGU. Recent studies have reported that the ability of insulin and glucose to stimulate splanchnic glucose uptake is impaired in individuals with type 2 diabetes. Thus, in specific aim I of this thesis we explored the ability of first phase insulin release to control the glycemic excursion on the background of basal insulin and a duodenal glucose infusion. It was determined that the pulse of insulin acutely affected net hepatic glucose production and increased NHGU while it still had significant effects on plasma glucose levels 4.5 hours later due to its ability to affect non hepatic glucose clearance. Although it has been demonstrated that the portal glucose signal is an important regulator of NHGU, the mechanism of action by which it exerts its effects is not completely understood. The relative importance of the sympathetic and parasympathetic nerves was not known. Other investigators had suggested that the portal signal may exert its effects through an intrahepatic reflex involving other mediators and neurotransmitters. Thus the remaining portion of this thesis was to further elucidate the potential regulators of the portal glucose signal and NHGU. Our attention first turned towards the role of the sympathetic nerves in the regulation of NHGU. The data from specific aim II suggest that the sympathetic nerves exert a tonic inhibition on NHGU in the presence of hyperglycemia, and that removal of these nerves, results in an increase in NHGU. Our conclusions from specific aim II led us to further investigate the vagus nerve and the role of the vagal afferents in mediating the portal glucose signal. The data from specific aim III suggested that the vagus nerve does not play a role in the regulation of NHGU suggesting that the afferent nerves found in the vagus are not the transmitters of the portal glucose signal. The data from specific aims II and III suggested that the sympathetic nerves exerted a dominant effect on NHGU while the input from the vagus nerve is not essential for the regulation of the portal glucose signal. Thus, the possibility exists that a local effect of the portal signal might be occurring via an intrahepatic reflex. Thus we hypothesized that nitric oxide may be involved in the regulation of NHGU. It is clear that the intraportal administration of the nitric oxide donor SIN-1 significantly decreased NHGU in the presence of the portal signal. This effect may be due to either a direct or an indirect mechanism.

Molecular Physiology and Biophysics

METABOTROPIC GLUTAMATE RECEPTOR MEDIATED SYNAPTIC PLASTICITY IN THE BED NUCLEUS OF THE STRIA TERMINALIS AS A TARGET FOR STRESS, ANXIETY AND ADDICTION DISORDERS

Grueter, Brad Alan

20 January 2006

The importance of integration of information from neurocircuits innervating the reward circuitry is becoming increasingly recognized. For instance, the roles of stress/anxiety pathways in modulating specific effects of the reward system are becoming more apparent. Behavioral data suggest the bed nucleus of the stria terminalis (BNST) is involved in integrating stress information and relaying this information to the stress and reward pathways. Moreover, behavioral data suggest glutamatergic transmission in the BNST as well as other regions in the stress/reward pathways plays an integral role in regulating stress and drug addiction behaviors. Changes in synaptic physiology in the BNST could in part underlie the persistent behavioral alterations in generalized anxiety, addiction and post-traumatic stress disorder. Metabotropic glutamate receptors (mGluRs) have been implicated in stress, addiction and synaptic plasticity, but their roles in the BNST are currently unknown. Field recordings and whole-cell patch clamp analysis in an in vitro slice preparation of C57/Bl6j adult male mouse dorsolateral BNST were utilized. Activation of either group I, group II or group III mGluRs in the dBNST causes a depression of excitatory synaptic transmission. Further characterization of mGluR5-dependent long-term depression (LTD) of excitatory synaptic transmission indicates this LTD is associated with a decrease in miniature EPSC frequency but not a change in paired pulse ratios of evoked responses. This suggests a novel maintenance mechanism for this form of LTD. Potential downstream effectors of group I mGluRs that have also been implicated in stress, addiction and synaptic plasticity are the cannabinoid system and extracellular signal regulated kinase (ERK). mGluR5-mediated LTD in the BNST is G-protein dependent, and persists in the cannabinoid receptor 1 knockout mouse. Further, converging pharmacological and genetic approaches suggest the mGluR5-mediated LTD in the BNST is ERK dependent. Consistent with an emerging role for group I mGluRs in drug addiction, mGluR5-mediated LTD in the BNST is attenuated in mice trained to self-administer cocaine.

Molecular Physiology and Biophysics