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5. Haploinsufficiency of RanBP2 is neuroprotective against light-elicited and age-dependent degeneration of photoreceptor neurons.

Author

Cho, K.-in, Yi, H., Yeh, A., Tserentsoodol, N., Cuadrado, L., Searle, K., Hao, Y., and Ferreira, P. A.

Subjects
PHOTORECEPTORS, NEURODEGENERATION, APOPTOSIS, CELL death, LABORATORY mice
Abstract

Prolonged light exposure is a determinant factor in inducing neurodegeneration of photoreceptors by apoptosis. Yet, the molecular bases of the pathways and components triggering this cell death event are elusive. Here, we reveal a prominent age-dependent increase in the susceptibility of photoreceptor neurons to undergo apoptosis under light in a mouse model. This is accompanied by light-induced subcellular changes of photoreceptors, such as dilation of the disks at the tip of the outer segments, prominent vesiculation of nascent disks, and autophagy of mitochondria into large multilamellar bodies. Notably, haploinsufficiency of Ran-binding protein-2 (RanBP2) suppresses apoptosis and most facets of membrane dysgenesis observed with age upon light-elicited stress. RanBP2 haploinsufficiency promotes decreased levels of free fatty acids in the retina independent of light exposure and turns the mice refractory to weight gain on a high-fat diet, whereas light promotes an increase in hydrogen peroxide regardless of the genotype. These studies demonstrate the presence of age-dependent and RanBP2-mediated pathways modulating membrane biogenesis of the outer segments and light-elicited neurodegeneration of photoreceptors. Furthermore, the findings support a mechanism whereby the RanBP2-dependent production of free fatty acids, metabolites thereof or the modulation of a cofactor dependent on any of these, promote apoptosis of photoreceptors in concert with the light-stimulated production of reactive oxygen species.Cell Death and Differentiation (2009) 16, 287–297; doi:10.1038/cdd.2008.153; published online 24 October 2008 [ABSTRACT FROM AUTHOR]

Published
2009
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8. Aldosterone Exposure Causes Increased Retinal Edema and Severe Retinopathy Following Laser-Induced Retinal Vein Occlusion in Mice.

Author

Allingham MJ, Tserentsoodol N, Saloupis P, Mettu PS, and Cousins SW

Subjects
Aldosterone administration & dosage, Animals, Biomarkers metabolism, Blotting, Western, Drug Implants, Female, Fluorescent Dyes, Macular Edema metabolism, Macular Edema physiopathology, Male, Mice, Mice, Inbred C57BL, Microscopy, Fluorescence, Retinal Hemorrhage metabolism, Retinal Hemorrhage physiopathology, Retinal Vein Occlusion metabolism, Retinal Vein Occlusion physiopathology, Rose Bengal, Tomography, Optical Coherence, Aldosterone adverse effects, Disease Models, Animal, Laser Coagulation adverse effects, Macular Edema chemically induced, Retinal Hemorrhage chemically induced, Retinal Vein Occlusion etiology
Abstract

Purpose: To determine the effects of aldosterone exposure on retinal edema and retinopathy in a mouse model of retinal vein occlusion (RVO)., Methods: RVO was induced immediately following intravenous injection of Rose bengal (66 mg/kg) using a 532-nm wavelength laser to place three to seven applications at 80 mW and 50-μm spot size directed at the superior retinal vein one disc diameter away from the nerve. Negative control consisted of placing an equal number of laser spots without targeting the vein. Male and female C57BL/6J mice aged 7 to 9 months with confirmed absence of Crb1rd8 were used. Aldosterone pellets releasing a daily dose of 0.83 μg/day were implanted subcutaneously 4 weeks prior to RVO. Retinal imaging by optical coherence tomography (OCT) was performed using a Micron IV rodent imaging system. Retinas were analyzed by immunohistochemistry using standard techniques. Retinal imaging and tissue analysis were performed 2, 4, and 7 days following RVO. Comparisons were made using Student's t-test, ANOVA, and Pearson's χ2., Results: RVO caused retinal edema in the form of cystic spaces and retinal thickening detectable by both OCT and histology. RVO also caused Müller glia (MG) dysfunction manifest as upregulated glial fibrillary acidic protein (GFAP) and altered localization of aquaporin 4 (AQP4) and Kir4.1. Treatment with aldosterone caused a significant increase in retinal edema and more severe retinopathy manifest as retinal whitening and extensive intraretinal hemorrhage. MG dysfunction was more severe and persistent in aldosterone-treated mice. Finally, aldosterone greatly increased the number of infiltrating mononuclear phagocytes following RVO., Conclusions: Systemic aldosterone exposure causes a more severe RVO phenotype manifest as increased severity and duration of retinal edema and more severe retinopathy. The effects of aldosterone may be mediated by MG dysfunction and increased infiltration of mononuclear phagocytes. This suggests that small increases in aldosterone levels may be a risk factor for severe RVO.

Published
2018
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9. Phosphorylation of G protein-coupled receptor kinase 1 (GRK1) is regulated by light but independent of phototransduction in rod photoreceptors.

Author

Osawa S, Jo R, Xiong Y, Reidel B, Tserentsoodol N, Arshavsky VY, Iuvone PM, and Weiss ER

Subjects
Adenylyl Cyclases genetics, Adenylyl Cyclases metabolism, Animals, Cyclic AMP genetics, Cyclic AMP metabolism, Cyclic AMP-Dependent Protein Kinases genetics, Dark Adaptation radiation effects, G-Protein-Coupled Receptor Kinase 1 genetics, Light Signal Transduction radiation effects, Mice, Mice, Knockout, Phosphorylation radiation effects, Transducin genetics, Transducin metabolism, Cyclic AMP-Dependent Protein Kinases metabolism, Dark Adaptation physiology, G-Protein-Coupled Receptor Kinase 1 metabolism, Light, Light Signal Transduction physiology, Retinal Rod Photoreceptor Cells metabolism
Abstract

Phosphorylation of rhodopsin by G protein-coupled receptor kinase 1 (GRK1, or rhodopsin kinase) is critical for the deactivation of the phototransduction cascade in vertebrate photoreceptors. Based on our previous studies in vitro, we predicted that Ser(21) in GRK1 would be phosphorylated by cAMP-dependent protein kinase (PKA) in vivo. Here, we report that dark-adapted, wild-type mice demonstrate significantly elevated levels of phosphorylated GRK1 compared with light-adapted animals. Based on comparatively slow half-times for phosphorylation and dephosphorylation, phosphorylation of GRK1 by PKA is likely to be involved in light and dark adaptation. In mice missing the gene for adenylyl cyclase type 1, levels of phosphorylated GRK1 were low in retinas from both dark- and light-adapted animals. These data are consistent with reports that cAMP levels are high in the dark and low in the light and also indicate that cAMP generated by adenylyl cyclase type 1 is required for phosphorylation of GRK1 on Ser(21). Surprisingly, dephosphorylation was induced by light in mice missing the rod transducin α-subunit. This result indicates that phototransduction does not play a direct role in the light-dependent dephosphorylation of GRK1.

Published
2011
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10. Neuroprotection resulting from insufficiency of RANBP2 is associated with the modulation of protein and lipid homeostasis of functionally diverse but linked pathways in response to oxidative stress.

Author

Cho KI, Yi H, Tserentsoodol N, Searle K, and Ferreira PA

Subjects
Animals, COUP Transcription Factor I metabolism, Cholesterol metabolism, Fatty Acids metabolism, Haploinsufficiency radiation effects, Light, Mice, Models, Biological, Molecular Chaperones genetics, Nuclear Pore Complex Proteins genetics, Protein Binding radiation effects, Protein Isoforms metabolism, Retinal Neurons metabolism, Retinal Neurons radiation effects, Retinal Pigment Epithelium metabolism, Retinal Pigment Epithelium pathology, Retinal Pigment Epithelium radiation effects, Signal Transduction radiation effects, Ubiquitin-Conjugating Enzymes, Ubiquitinated Proteins metabolism, Ubiquitin-Conjugating Enzyme UBC9, Cytoprotection radiation effects, Haploinsufficiency genetics, Homeostasis radiation effects, Lipid Metabolism radiation effects, Molecular Chaperones metabolism, Nuclear Pore Complex Proteins metabolism, Oxidative Stress radiation effects, Retinal Neurons pathology
Abstract

Oxidative stress is a deleterious stressor associated with a plethora of disease and aging manifestations, including neurodegenerative disorders, yet very few factors and mechanisms promoting the neuroprotection of photoreceptor and other neurons against oxidative stress are known. Insufficiency of RAN-binding protein-2 (RANBP2), a large, mosaic protein with pleiotropic functions, suppresses apoptosis of photoreceptor neurons upon aging and light-elicited oxidative stress, and promotes age-dependent tumorigenesis by mechanisms that are not well understood. Here we show that, by downregulating selective partners of RANBP2, such as RAN GTPase, UBC9 and ErbB-2 (HER2; Neu), and blunting the upregulation of a set of orphan nuclear receptors and the light-dependent accumulation of ubiquitylated substrates, light-elicited oxidative stress and Ranbp2 haploinsufficiency have a selective effect on protein homeostasis in the retina. Among the nuclear orphan receptors affected by insufficiency of RANBP2, we identified an isoform of COUP-TFI (Nr2f1) as the only receptor stably co-associating in vivo with RANBP2 and distinct isoforms of UBC9. Strikingly, most changes in proteostasis caused by insufficiency of RANBP2 in the retina are not observed in the supporting tissue, the retinal pigment epithelium (RPE). Instead, insufficiency of RANBP2 in the RPE prominently suppresses the light-dependent accumulation of lipophilic deposits, and it has divergent effects on the accumulation of free cholesterol and free fatty acids despite the genotype-independent increase of light-elicited oxidative stress in this tissue. Thus, the data indicate that insufficiency of RANBP2 results in the cell-type-dependent downregulation of protein and lipid homeostasis, acting on functionally interconnected pathways in response to oxidative stress. These results provide a rationale for the neuroprotection from light damage of photosensory neurons by RANBP2 insufficiency and for the identification of novel therapeutic targets and approaches promoting neuroprotection.

Published
2010
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11. Gene and protein expression pilot profiling and biomarkers in an experimental mouse model of hypertensive glaucoma.

Author

Walsh MM, Yi H, Friedman J, Cho KI, Tserentsoodol N, McKinnon S, Searle K, Yeh A, and Ferreira PA

Subjects
Animals, Disease Models, Animal, Gene Expression Regulation, Glaucoma physiopathology, Hydrogen Peroxide metabolism, Immunohistochemistry, Intraocular Pressure physiology, Mice, Microglia metabolism, Microglia pathology, Neurons metabolism, Neurons pathology, Ocular Hypertension physiopathology, Retina metabolism, Retina pathology, Retina physiopathology, Gene Expression Profiling, Glaucoma complications, Glaucoma genetics, Ocular Hypertension complications, Ocular Hypertension genetics
Abstract

Glaucoma is a group of genetically heterogeneous neurodegenerative disorders causing the degeneration of the ganglion neurons of the retina. Increased intraocular pressure (IOP) is a hallmark risk factor promoting the death of ganglion neurons of the retina in glaucoma. Yet, the molecular processes underlying the degeneration of these neurons by increased IOP are not understood. To gain insight into the early molecular events and discover biomarkers induced by IOP, we performed gene and protein expression profiling to compare retinas of eyes with and without high IOP in a rodent model of experimental glaucoma. This pilot study found that the IOP-mediated changes in the transcription levels of a restricted set of genes implicated in peroxisomal and mitochondrial function, modulation of neuron survival and inflammatory processes, were also accompanied by changes in the levels of proteins encoded by the same genes. With the exception of the inflammatory markers, serum amyloid-A1 (SAA1) and serum amyloid-A2 (SAA2), the IOP-induced changes in protein expression were restricted to ganglion neurons of the retina and they were detected also in the vitreous, thus suggesting an early IOP-mediated loss of ganglion cell integrity. Interestingly, SAA1 and SAA2 were induced in retinal microglia cells, whereas they were reduced in sera of IOP-responsive mice. Hence, this study defines novel IOP-induced molecular processes, biomarkers and sources thereof, and it further validates the extension of the analyses herein reported to other genes modulated by IOP.

Published
2009
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12. Uptake of cholesterol by the retina occurs primarily via a low density lipoprotein receptor-mediated process.

Author

Tserentsoodol N, Sztein J, Campos M, Gordiyenko NV, Fariss RN, Lee JW, Fliesler SJ, and Rodriguez IR

Subjects
Animals, Apolipoproteins B pharmacokinetics, Cell Line, Cholestenes pharmacokinetics, Cholesterol pharmacokinetics, Humans, Immunohistochemistry, Injections, Intravenous, Lipoproteins, LDL administration & dosage, Lipoproteins, LDL pharmacokinetics, Macaca mulatta, Rats, Rats, Sprague-Dawley, Tissue Distribution, Cholesterol metabolism, Receptors, LDL metabolism, Retina metabolism
Abstract

Purpose: In this study we examined the uptake of circulating lipoproteins into the retina, using a naturally fluorescent cholesterol analog for imaging and deuterated cholesterol for quantification by mass spectroscopy. The purpose of this study was to better understand cholesterol uptake, transport and homeostasis in the retina., Methods: Human low density lipoprotein (LDL) and high density lipoprotein (HDL) were labeled with the fluorescent cholesterol analog cholesta-5,7,9(11)-trien-3beta-ol (CTL) and deuterated cholesterol (25,26,26,26,27,27,27-[2H]cholesterol, D7Ch). Rats were injected intravenously with CTL-LDL, CTL-HDL and D7Ch-LDL. Fluorescent confocal microscopy was used to image the uptake of CTL and mass spectroscopy was used to quantify D7Ch. Immunohistochemistry and fluorescent confocal microscopy were used to localize apoB (an LDL marker protein) and LDL receptor (LDLR) protein in rat and monkey retinas., Results: CTL-specific fluorescence was imaged by confocal microscopy in the retinal pigment epithelium (RPE), choriocapillaris and parts of the neural retina within 2 h post-injection and was visualized in the photoreceptor outer segments by 4 h. Replacing LDL with HDL as the CTL carrier gave a less robust and more delayed labeling of retinal layers. Human apolipoprotein B (apoB) was also localized in the rat choriocapillaris and RPE by 4 h post-injection. Human apoB was detected by immunoblot analysis in the rat retina primarily as a about 70 kDa protein, suggesting proteolytic degradation. LDL-mediated uptake of cholesterol was quantified by mass spectroscopy using deuterated cholesterol in place of CTL. In addition, apoB and LDLR were localized in monkey retina by immunohistochemistry., Conclusions: The retina is capable of rapid uptake of circulating LDL via an LDLR-mediated process primarily occurring in the RPE and also possibly Müller cells. Despite the dominance of HDL over LDL in rat serum, LDL appears to be the preferred carrier for cholesterol transport to and uptake by the retina. The results also suggest that blood-borne LDL represents a significant contributor to the steady-state levels of cholesterol and possibly other lipids in the retina.

Published
2006

13. Intraretinal lipid transport is dependent on high density lipoprotein-like particles and class B scavenger receptors.

Author

Tserentsoodol N, Gordiyenko NV, Pascual I, Lee JW, Fliesler SJ, and Rodriguez IR

Subjects
ATP Binding Cassette Transporter 1, ATP-Binding Cassette Transporters metabolism, Animals, Apolipoprotein A-I metabolism, Biological Transport, Carrier Proteins metabolism, Cholesterol Ester Transfer Proteins metabolism, Haplorhini, Humans, Lipoproteins metabolism, Phosphatidylcholine-Sterol O-Acyltransferase metabolism, Receptors, Lipoprotein metabolism, Receptors, Scavenger, Tissue Distribution, CD36 Antigens metabolism, Lipid Metabolism physiology, Lipoproteins, HDL metabolism, Lysosomal Membrane Proteins metabolism, Retina metabolism, Sialoglycoproteins metabolism
Abstract

Purpose: In our companion paper we demonstrated that circulating lipoproteins enter the retina via the retinal pigment epithelium (RPE) and possibly Müller cells. In order to understand how these lipids are transported within the retina, expression and localization of the main proteins known to be involved in systemic lipid transport was determined., Methods: Expression of ABCA1, apoA1 (the major HDL protein), SR-BI, SR-BII, CD36, lecithin:cholesterol acyltransferase (LCAT), and cholesteryl ester transfer protein (CETP) was determined by reverse transcriptase polymerase chain reaction (RT-PCR) and immunoblots. Localization was determined by immunohistochemistry using fresh monkey vibrotome sections and imaged by confocal microscopy., Results: ABCA1 and apoA1 were localized to the ganglion cell layer, retinal pigment epithelium (RPE), and rod photoreceptor inner segments. ApoA1 was also observed associated with rod photoreceptor outer segments, presumably localized to the interphotoreceptor matrix (IPM). The scavenger receptors SR-BI and SR-BII localized mainly to the ganglion cell layer and photoreceptor outer segments; in the latter they appear to be associated with microtubules. LCAT and CETP localized mainly to the IPM., Conclusions: The presence and specific localization of these well-known lipid transport proteins suggest that the retina employs an internal lipid transport mechanism that involves processing and maturation of HDL-like particles.

Published
2006

14. The glucose transporter GLUT1 and the tight junction protein occludin in nasal olfactory mucosa.

Author

Hussar P, Tserentsoodol N, Koyama H, Yokoo-Sugawara M, Matsuzaki T, Takami S, and Takata K

Subjects
Animals, Endothelium, Vascular chemistry, Glucose Transporter Type 1, Immunohistochemistry, Male, Membrane Proteins physiology, Monosaccharide Transport Proteins physiology, Occludin, Olfactory Mucosa blood supply, Olfactory Nerve chemistry, Olfactory Receptor Neurons chemistry, Rats, Rats, Wistar, Tight Junctions chemistry, Membrane Proteins analysis, Monosaccharide Transport Proteins analysis, Olfactory Mucosa chemistry
Abstract

The nervous cells in the brain and the peripheral nerves are isolated from the external environment by the blood-brain, blood-cerebrospinal fluid and blood-nerve barriers. The glucose transporter GLUT1 mediates the specific transfer of glucose across these barriers. The olfactory system is unique in that its sensory cells, olfactory receptor neurons, are embedded in the nasal olfactory epithelium and send their axons directly to the olfactory bulb of the brain. Only the apical parts of the olfactory receptor neurons are exposed to the lumen, and these serve as sensors for smell. Immunohistochemical examination showed that the tight junction protein occludin was present in the junctions of the olfactory epithelium. Endothelial cells in the blood vessels in the lamina propria of the olfactory mucosa were also positive for occludin. These observations suggest that the olfactory system is guarded from both the external environment and the blood. GLUT1 was abundant in these occludin-positive endothelial cells, suggesting that GLUT1 may serve in nourishing the cells of the olfactory system. Taken together, GLUT1 and occludin may serve as part of the machinery for the specific transfer of glucose in the olfactory system while preventing the non-specific entry of substances.

Published
2002
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15. Immunolocalization of tight junction proteins, occludin and ZO-1, and glucose transporter GLUT1 in the cells of the blood-nerve barrier.

Author

Tserentsoodol N, Shin BC, Koyama H, Suzuki T, and Takata K

Subjects
Animals, Capillaries chemistry, Capillaries ultrastructure, Capillary Permeability physiology, Fluorescent Antibody Technique, Glucose Transporter Type 1, Guinea Pigs, Male, Microscopy, Immunoelectron, Occludin, Peripheral Nerves blood supply, Peripheral Nerves chemistry, Peripheral Nerves ultrastructure, Rabbits, Rats, Rats, Wistar, Sciatic Nerve blood supply, Sciatic Nerve chemistry, Tight Junctions ultrastructure, Zonula Occludens-1 Protein, Membrane Proteins analysis, Monosaccharide Transport Proteins analysis, Phosphoproteins analysis, Sciatic Nerve ultrastructure, Tight Junctions chemistry
Abstract

Facilitated-diffusion glucose transporter GLUT1 is abundant in the blood-nerve barrier. To observe the relationship between glucose transfer across the barrier and the molecular architecture of the barrier, we examined the localization of GLUT1 and tight junction proteins, occludin and zonula occludens-1 (ZO-1), by immunofluorescence microscopy and immunogold electron microscopy in the rat sciatic nerve. GLUT1 was enriched at the whole aspects of the plasma membranes of the cells of the barrier: perineurial cells, and endothelial cells of the blood vessels in the endoneurium. These GLUT1-positive cells were also positive for occludin and ZO-1, both of which were localized at tight junctions. ZO-1 additionally was present in the GLUT1-negative cells not serving as the blood-nerve barrier. These observations suggest that occludin in the tight junctions and GLUT1 at the plasma membranes in the cells of the barrier may constitute a mechanism for the selective transfer of glucose across the barrier while preventing the non-specific flow of blood constituents.

Published
1999
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16. Colocalization of tight junction proteins, occludin and ZO-1, and glucose transporter GLUT1 in cells of the blood-ocular barrier in the mouse eye.

Author

Tserentsoodol N, Shin BC, Suzuki T, and Takata K

Subjects
Animals, Ciliary Body ultrastructure, Fluorescent Antibody Technique, Indirect, Glucose Transporter Type 1, Iris ultrastructure, Male, Mice, Mice, Inbred BALB C, Microscopy, Immunoelectron, Occludin, Retina ultrastructure, Tight Junctions chemistry, Tight Junctions ultrastructure, Zonula Occludens-1 Protein, Blood-Aqueous Barrier, Blood-Retinal Barrier, Ciliary Body chemistry, Iris chemistry, Membrane Proteins analysis, Monosaccharide Transport Proteins analysis, Phosphoproteins analysis, Retina chemistry
Abstract

The facilitative glucose transporter GLUT1 is abundant in cells of the blood-ocular barrier and serves as a glucose transport mechanism in the barrier. To see the relationship between the glucose transfer function and junctional proteins in the barrier, we examined the localization of GLUT1 and the tight junction proteins, occludin and ZO-1, in the mouse eye. Their localization in the retina, ciliary body, and iris was visualized by double-immunofluorescence microscopy and immunogold electron microscopy. Occludin and ZO-1 were colocalized at tight junctions of the cells of the barrier: retinal pigment epithelial cells, non-pigmented epithelial cells of the ciliary body, and endothelial cells of GLUT1-positive blood vessels. Occludin was restricted to these cells of the barrier. ZO-1 was found, in addition, in sites not functioning as a barrier: the outer limiting membrane in the retina, in the cell border between pigmented and non-pigmented epithelial cells in the ciliary body, and GLUT1-negative blood vessels. These observations show that localization of occludin is restricted to tight junctions of cells of the barrier, whereas ZO-1 is more widely distributed.

Published
1998
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