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2. Elongate cavities and skin-core structure in Nephila spider silk observed by electron microscopy

Author

Sebastian Frische, Maunsbach, Ab, and Vollrath, F.

Subjects
MAJOR AMPULLATE SILK, DRAGLINE SILK, biopolymer, fungi, microstructure, technology, industry, and agriculture, biomaterial, macromolecular substances, equipment and supplies, fibrous protein, CLAVIPES, Nephila madagascariensis
Abstract

Major ampullate silk fibres from the orb-weaving spider Nephila madagascariensis were analysed by transmission electron microscopy. The fibres have a thin outer layer surrounding a column of apparently homogeneous material which contains elongate cavities orientated parallel to the silk fibre axis. The cavities appear similar to 'elongate vacuolar droplets' observed in the silk of Antheraea silkmoth larvae. The overall skin-core structure is probably the result of a rheological pattern originating in the two secreting regions recognized in Nephila silk glands; the cavities indicate material inhomogeneities.

Published
1998

5. Probing of the membrane topology of sarcoplasmic reticulum Ca2+-ATPase with sequence-specific antibodies. Evidence for plasticity of the c-terminal domain

Author

Moller, Jv, Ning, G., Maunsbach, Ab, Fujimoto, K., Asai, K., Juul, B., Lee, Yj, Gomezdegracia, A., Falson, P., Lemaire, M., Institut de biologie et chimie des protéines [Lyon] (IBCP), Université Claude Bernard Lyon 1 (UCBL), Université de Lyon-Université de Lyon-Centre National de la Recherche Scientifique (CNRS), and Deleage, Gilbert

Subjects
Protein Folding, Hydrolysis, Immune Sera, Detergents, Membrane Proteins, Enzyme-Linked Immunosorbent Assay, Calcium-Transporting ATPases, Antibodies, Sarcoplasmic Reticulum, Mutagenesis, Molecular Probes, [SDV.BBM] Life Sciences [q-bio]/Biochemistry, Molecular Biology, Animals, Freeze Fracturing, [SDV.BBM]Life Sciences [q-bio]/Biochemistry, Molecular Biology, Rabbits, Microscopy, Immunoelectron
Abstract

International audience; The topology of Ca2+-ATPase in sarcoplasmic reticulum (SR) vesicles was investigated with the aid of sequence-specific antibodies, produced against oligopeptides corresponding to sequences close to the membranous portions of the protein. The antisera in competitive enzyme-linked immunosorbent assays only reacted with intact SR vesicles to a limited extent, but most epitopic regions were exposed by low concentrations of nondenaturing detergent, octaethylene glycol dodecyl ether (C12E8) or after removal of cytosolic regions by proteinase K. In particular, these treatments exposed the loop regions in the C-terminal domain, including L7-8, the loop region located between transmembrane segments M7 and M8, with a putative intravesicular position, which had immunochemical properties very similar to those of the C terminus with a documented cytosolic exposure. In contrast to this, the reactivity of the N-terminal intravesicular loop regions L1-2 and L3-4 was only increased by C12E8 treatment but not by proteinase K proteolysis. Complexation of Ca2+-ATPase with beta,gamma-CrATP stabilized the C-terminal domain of Ca2+-ATPase against proteinase K proteolysis and reaction with most of the antisera, but immunoreactivity was maintained by the L6-7 and L7-8 loops. Immunoelectron microscopic analyses of vesicles following negative staining, thin sectioning, and the SDS-digested freeze-fracture labeling method suggested that the L7-8 epitope, in contrast to L6-7 and the C terminus, can be exposed on either the intravesicular or cytosolic side of the membrane. A preponderant intravesicular location of L7-8 in intact vesicles is suggested by the susceptibility of this region to proteolytic cleavage after disruption of the vesicular barrier with C12E8 and in symmetrically reconstituted Ca2+-ATPase proteoliposomes. In conclusion, our data suggest an adaptable membrane insertion of the C-terminal Ca2+-ATPase domain, which under some conditions permits sliding of M8 through the membrane with cytosolic exposure of L7-8, of possible functional significance in connection with Ca2+ translocation. On the technical side, our data emphasize that extreme caution is needed when using nondenaturing detergents or other treatments like EGTA at alkaline pH to open up vesicles for probing of intravesicular location with antibodies.The topology of Ca2+-ATPase in sarcoplasmic reticulum (SR) vesicles was investigated with the aid of sequence-specific antibodies, produced against oligopeptides corresponding to sequences close to the membranous portions of the protein. The antisera in competitive enzyme-linked immunosorbent assays only reacted with intact SR vesicles to a limited extent, but most epitopic regions were exposed by low concentrations of nondenaturing detergent, octaethylene glycol dodecyl ether (C12E8) or after removal of cytosolic regions by proteinase K. In particular, these treatments exposed the loop regions in the C-terminal domain, including L7-8, the loop region located between transmembrane segments M7 and M8, with a putative intravesicular position, which had immunochemical properties very similar to those of the C terminus with a documented cytosolic exposure. In contrast to this, the reactivity of the N-terminal intravesicular loop regions L1-2 and L3-4 was only increased by C12E8 treatment but not by proteinase K proteolysis. Complexation of Ca2+-ATPase with beta,gamma-CrATP stabilized the C-terminal domain of Ca2+-ATPase against proteinase K proteolysis and reaction with most of the antisera, but immunoreactivity was maintained by the L6-7 and L7-8 loops. Immunoelectron microscopic analyses of vesicles following negative staining, thin sectioning, and the SDS-digested freeze-fracture labeling method suggested that the L7-8 epitope, in contrast to L6-7 and the C terminus, can be exposed on either the intravesicular or cytosolic side of the membrane. A preponderant intravesicular location of L7-8 in intact vesicles is suggested by the susceptibility of this region to proteolytic cleavage after disruption of the vesicular barrier with C12E8 and in symmetrically reconstituted Ca2+-ATPase proteoliposomes. In conclusion, our data suggest an adaptable membrane insertion of the C-terminal Ca2+-ATPase domain, which under some conditions permits sliding of M8 through the membrane with cytosolic exposure of L7-8, of possible functional significance in connection with Ca2+ translocation. On the technical side, our data emphasize that extreme caution is needed when using nondenaturing detergents or other treatments like EGTA at alkaline pH to open up vesicles for probing of intravesicular location with antibodies.

Published
1997

7. Purposes and Organisation

Author

Maunsbach Ab and Hojer Ja

Subjects
General Medicine, General Dentistry
Abstract

(1953). Purposes and Organisation. Acta Odontologica Scandinavica: Vol. 11, No. 3-4, pp. 195-206.

Published
1953
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8. Ultrastructure of the sodium pump: Comparison of thin sectioning, negative staining, and freeze-fracture of purified, membrane-bound (Na+, K+)-ATPase

Author

Deguchi, N, Jorgensen, PL, and Maunsbach, AB

Abstract

Purified (Na+, K+)-ATPase was studied by electron microscopy after thin sectioning, negative staining, and freeze-fracturing, particular emphasis being paid to the dimensions and frequencies of substructures in the membranes. Ultrathin sections show exclusively flat or cup-shaped membrane fragments which are triple-layered along much of their length and have diameters of 0.1-0.6 μm. Negative staining revealed a distinct substructure of particles with diameters between 30 and 50 A and with a frequency of 12,500 +/- 2,400 (SD) per μm(2). Comparisons with sizes of the protein components suggest that each surface particle contains as its major component one large catalytic chain with mol wt close to 100,000 and that two surface particles unite to form the unit of (Na+,K+)-ATPase which binds one molecule of ATP or ouabain. The further observations that the surface particles protrude from the membrane surface and are observed on both membrane surfaces in different patterns and degrees of clustering suggest that protein units span the membrane and are capable of lateral mobility. Freeze-fracturing shows intramembranous particles with diameters of 90-110 A and distributed on both concave and convex fracture faces with a frequency of 3,410 +/- 370 per μm(2) and 390 +/- 170 per μm(2), respectively. The larger diameters and three to fourfold smaller frequency of the intramembranous particles as compared to the surface particles seen after negative staining may reflect technical differences between methods, but it is more likely that the intramembranous particle is an oliogomer composed of two or even more of the protein units which form the surface particles.

Published
1977
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9. MICROAUTORADIOGRAPHIC LOCALIZATION OF WATER-SOLUBLE CADMIUM IN MOUSE KIDNEY

Author

Berlin M, Hammarstroem L, and Maunsbach Ab

Subjects
Radioisotopes, Cadmium, Kidney, Microscopy, Research, chemistry.chemical_element, Water, General Medicine, Mice, Water soluble, medicine.anatomical_structure, chemistry, Biochemistry, Mouse Kidney, medicine, Animals, Autoradiography, Microscopy, Phase-Contrast, Physiological Phenomena
Published
1964

11. Sodium transport is modulated by p38 kinase-dependent cross-talk between ENaC and Na,K-ATPase in collecting duct principal cells.

Author

Wang YB, Leroy V, Maunsbach AB, Doucet A, Hasler U, Dizin E, Ernandez T, de Seigneux S, Martin PY, and Féraille E

Subjects
AMP-Activated Protein Kinases physiology, Aldosterone physiology, Animals, Basement Membrane metabolism, Biological Transport, Active physiology, Cell Line, Transformed, Cell Membrane metabolism, Cell Polarity, Endocytosis physiology, Enzyme Induction, Epithelial Sodium Channels biosynthesis, Epithelial Sodium Channels genetics, Homeostasis physiology, Intracellular Fluid metabolism, Ion Transport physiology, Kidney Tubules, Collecting cytology, Lysosomes metabolism, MAP Kinase Signaling System drug effects, Male, Mice, Rats, Rats, Sprague-Dawley, Sodium-Potassium-Exchanging ATPase biosynthesis, Sodium-Potassium-Exchanging ATPase genetics, Sodium-Potassium-Exchanging ATPase metabolism, p38 Mitogen-Activated Protein Kinases antagonists & inhibitors, Epithelial Sodium Channels physiology, Kidney Tubules, Collecting metabolism, MAP Kinase Signaling System physiology, Sodium metabolism, Sodium-Potassium-Exchanging ATPase physiology, p38 Mitogen-Activated Protein Kinases physiology
Abstract

In relation to dietary Na(+) intake and aldosterone levels, collecting duct principal cells are exposed to large variations in Na(+) transport. In these cells, Na(+) crosses the apical membrane via epithelial Na(+) channels (ENaC) and is extruded into the interstitium by Na,K-ATPase. The activity of ENaC and Na,K-ATPase must be highly coordinated to accommodate variations in Na(+) transport and minimize fluctuations in intracellular Na(+) concentration. We hypothesized that, independent of hormonal stimulus, cross-talk between ENaC and Na,K-ATPase coordinates Na(+) transport across apical and basolateral membranes. By varying Na(+) intake in aldosterone-clamped rats and overexpressing γ-ENaC or modulating apical Na(+) availability in cultured mouse collecting duct cells, enhanced apical Na(+) entry invariably led to increased basolateral Na,K-ATPase expression and activity. In cultured collecting duct cells, enhanced apical Na(+) entry increased the basolateral cell surface expression of Na,K-ATPase by inhibiting p38 kinase-mediated endocytosis of Na,K-ATPase. Our results reveal a new role for p38 kinase in mediating cross-talk between apical Na(+) entry via ENaC and its basolateral exit via Na,K-ATPase, which may allow principal cells to maintain intracellular Na(+) concentrations within narrow limits.

Published
2014
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12. Effects of ACE inhibition and ANG II stimulation on renal Na-Cl cotransporter distribution, phosphorylation, and membrane complex properties.

Author

Lee DH, Maunsbach AB, Riquier-Brison AD, Nguyen MT, Fenton RA, Bachmann S, Yu AS, and McDonough AA

Subjects
Animals, Calmodulin-Binding Proteins analysis, Captopril pharmacology, Kidney Tubules, Distal cytology, Kidney Tubules, Distal drug effects, Male, Phosphorylation, Rats, Rats, Sprague-Dawley, Sodium Chloride Symporter Inhibitors pharmacology, Angiotensin II pharmacology, Angiotensin-Converting Enzyme Inhibitors pharmacology, Kidney Tubules, Distal metabolism, Sodium Chloride Symporters metabolism
Abstract

The renal distal tubule Na-Cl cotransporter (NCC) reabsorbs <10% of the filtered Na(+) but is a key control point for blood pressure regulation by angiotensin II (ANG II), angiotensin-converting enzyme inhibitors (ACEI), and thiazide diuretics. This study aimed to determine whether NCC phosphorylation (NCCp) was regulated by acute (20-30 min) treatment with the ACEI captopril (12 μg/min × 20 min) or by a sub-pressor dose of ANG II (20 ng·kg(-1)·min(-1)) in Inactin-anesthetized rats. By immuno-EM, NCCp was detected exclusively in or adjacent to apical plama membranes (APM) in controls and after ACEI or ANG II treatment, while NCC total was detected in both APM and subapical cytoplasmic vesicles (SCV) in all conditions. In renal homogenates, neither ACEI nor ANG II treatment altered NCCp abundance, assayed by immunoblot. However, by density gradient fractionation we identified a pool of low-density APM in which NCCp decreased 50% in response to captopril and was restored during ANG II infusion, and another pool of higher-density APM that responded reciprocally, indicative of regulated redistribution between two APM pools. In both pools, NCCp was preferentially localized to Triton-soluble membranes. Blue Native gel electrophoresis established that APM NCCp localized to ~700 kDa complexes (containing γ-adducin) while unphosphorylated NCC in intracellular membranes primarily localized to ~400 kDa complexes: there was no evidence for native monomeric or dimeric NCC or NCCp. In summary, this study demonstrates that phosphorylated NCC, localized to multimeric complexes in the APM, redistributes in a regulated manner within the APM in response to ACEI and ANG II.

Published
2013
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13. Response of IMCD3 cells to hypertonic challenges as analyzed by electron microscopy.

Author

Pihakaski-Maunsbach K, Nonaka S, Vorum H, and Maunsbach AB

Subjects
Adaptation, Physiological, Animals, Apoptosis, Caspase 3 metabolism, Cell Line, Kidney Medulla cytology, Kidney Medulla metabolism, Kidney Tubules, Collecting cytology, Kidney Tubules, Collecting metabolism, Mice, Microscopy, Immunoelectron, Osmolar Concentration, Sodium Chloride pharmacology, Kidney Medulla ultrastructure, Kidney Tubules, Collecting ultrastructure, Saline Solution, Hypertonic pharmacology
Abstract

This work defines the ultrastructural responses of immortalized cells from the inner medullary collecting duct cells (IMCD3 cells) to hypertonic challenges. The cultured cells were either acutely exposed to hypertonic medium (550 mOsm/kgH₂O) for 24-72 h or gradually adapted to 600 or 900 mOsm/kgH₂O media with sodium chloride. After short (24 h) hypertonic challenges, there was an expansion of the Golgi apparatus with distinct expression of the γ subunit of Na,K-ATPase. The frequency of active caspase-3-positive cells was unchanged as was also the measured activity of caspase-3. Immunoelectron microscopy showed that active caspase-3 in the positive cells was localized in cytoplasmic bodies 0.5-1 μm in diameter but not in other structures. Apoptotic bodies with the nuclei were only rarely observed following acute hypertonicity for 24 to 72 h. Following prolonged hypertonic challenges, some cells showed condensation of the chromatin but still few apoptotic bodies. Gradual hypertonicity to 900 mOsm/kgH₂O led to a decrease of microvilli, dilated cisternae of the endoplasmic reticulum (ER), increased abundance of free ribosomes and longitudinal mitochondrial cristae. Virus particles were present inside and outside the cells in all experimental conditions and appeared unrelated to the apoptotic process. The results suggest that cultured IMCD3 cells are resistant to short hypertonic challenge or gradual adaptation to moderate hypertonicity and only rarely exhibit more ultrastructural apoptotic changes than control cells. The presence of caspase-3-containing bodies is a novel finding, and we suggest that they arise from the ER and are involved in the apoptotic signaling system.

Published
2010
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14. Identification and characterization of novel ERC-55 interacting proteins: evidence for the existence of several ERC-55 splicing variants; including the cytosolic ERC-55-C.

Author

Ludvigsen M, Jacobsen C, Maunsbach AB, and Honoré B

Subjects
Amino Acid Sequence, Calcium-Binding Proteins genetics, Calcium-Binding Proteins isolation & purification, Cell Cycle Proteins analysis, Cell Cycle Proteins metabolism, Cell Line, Female, Gene Expression, Humans, Kininogens analysis, Kininogens metabolism, Lactoferrin analysis, Lactoferrin metabolism, Molecular Sequence Data, Muramidase analysis, Muramidase metabolism, Peptides analysis, Peptides metabolism, Peroxiredoxin VI analysis, Peroxiredoxin VI metabolism, Placenta chemistry, Pregnancy, Protein Binding, S100 Calcium Binding Protein A6, S100 Proteins analysis, S100 Proteins metabolism, Calcium-Binding Proteins analysis, Calcium-Binding Proteins metabolism, Cytosol metabolism, Protein Splicing
Abstract

ERC-55, encoded from RCN2, is localized in the ER and belongs to the CREC protein family. ERC-55 is involved in various diseases and abnormal cell behavior, however, the function is not well defined and it has controversially been reported to interact with a cytosolic protein, the vitamin D receptor. We have used a number of proteomic techniques to further our functional understanding of ERC-55. By affinity purification, we observed interaction with a large variety of proteins, including those secreted and localized outside of the secretory pathway, in the cytosol and also in various organelles. We confirm the existence of several ERC-55 splicing variants including ERC-55-C localized in the cytosol in association with the cytoskeleton. Localization was verified by immunoelectron microscopy and sub-cellular fractionation. Interaction of lactoferrin, S100P, calcyclin (S100A6), peroxiredoxin-6, kininogen and lysozyme with ERC-55 was further studied in vitro by SPR experiments. Interaction of S100P requires [Ca(2+)] of approximately 10(-7) M or greater, while calcyclin interaction requires [Ca(2+)] of >10(-5) M. Interaction with peroxiredoxin-6 is independent of Ca(2+). Co-localization of lactoferrin, S100P and calcyclin with ERC-55 in the perinuclear area was analyzed by fluorescence confocal microscopy. The functional variety of the interacting proteins indicates a broad spectrum of ERC-55 activities such as immunity, redox homeostasis, cell cycle regulation and coagulation.

Published
2009
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15. Acute hypertension provokes acute trafficking of distal tubule Na-Cl cotransporter (NCC) to subapical cytoplasmic vesicles.

Author

Lee DH, Riquier AD, Yang LE, Leong PK, Maunsbach AB, and McDonough AA

Subjects
Acute Disease, Angiotensin II administration & dosage, Angiotensin-Converting Enzyme Inhibitors administration & dosage, Animals, Captopril administration & dosage, Cell Fractionation, Cell Membrane drug effects, Cell Membrane ultrastructure, Cytoplasmic Vesicles drug effects, Cytoplasmic Vesicles ultrastructure, Disease Models, Animal, Hypertension physiopathology, Infusions, Intravenous, Kidney Tubules, Distal drug effects, Kidney Tubules, Distal ultrastructure, Male, Microscopy, Immunoelectron, Protein Transport, Rats, Rats, Sprague-Dawley, Solute Carrier Family 12, Member 3, Time Factors, Blood Pressure drug effects, Cell Membrane metabolism, Cytoplasmic Vesicles metabolism, Diuresis drug effects, Hypertension metabolism, Kidney Tubules, Distal metabolism, Receptors, Drug metabolism, Sodium Chloride Symporters metabolism, Symporters metabolism
Abstract

When blood pressure (BP) is elevated above baseline, a pressure natriuresis-diuresis response ensues, critical to volume and BP homeostasis. Distal convoluted tubule Na(+)-Cl(-) cotransporter (NCC) is regulated by trafficking between the apical plasma membrane (APM) and subapical cytoplasmic vesicles (SCV). We aimed to determine whether NCC trafficking contributes to pressure diuresis by decreasing APM NCC or compensates for increased volume flow to the DCT by increasing APM NCC. BP was raised 50 mmHg (high BP) in rats by arterial constriction for 5 or 20-30 min, provoking a 10-fold diuresis at both times. Kidneys were excised, and NCC subcellular distribution was analyzed by 1) sorbitol density gradient fractionation and immunoblotting and 2) immunoelectron microscopy (immuno-EM). NCC distribution did not change after 5-min high BP. After 20-30 min of high BP, 20% of NCC redistributed from low-density, APM-enriched fractions to higher density, endosome-enriched fractions, and, by quantitative immuno-EM, pool size of APM NCC decreased 14% and SCV pool size increased. Because of the time lag of the response, we tested the hypothesis that internalization of NCC was secondary to the decrease in ANG II that accompanies high BP. Clamping ANG II at a nonpressor level by coinfusion of captopril (12 microg/min) and ANG II (20 ng.kg(-1).min(-1)) during 30-min high BP reduced diuresis to eightfold and prevented redistribution of NCC from APM- to SCV-enriched fractions. We conclude that DCT NCC may participate in pressure natriuresis-diuresis by retraction out of apical plasma membranes and that the retraction is, at least in part, driven by the fall in ANG II that accompanies acute hypertension.

Published
2009
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16. A profile of Fritiof S. Sjöstrand--the founding editor.

Author

Maunsbach AB

Subjects
History, 20th Century, History, 21st Century, Publishing history, Microscopy, Electron history, Periodicals as Topic history
Abstract

The Journal of Ultrastructure Research was founded in 1957 by Fritiof S. Sjöstrand, who served as Editor-in-Chief until 1990, when the journal changed the name to the Journal of Structural Biology. This profile summarizes the developments that led to the start of the journal and aspects of Fritiof Sjöstrand's scientific and personal carrier.

Published
2008
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17. Expression and trafficking of the gamma subunit of Na,K-ATPase in hypertonically challenged IMCD3 cells.

Author

Pihakaski-Maunsbach K, Nonaka S, and Maunsbach AB

Abstract

The gamma subunit (FXYD2) of Na,K-ATPase is an important regulator of the sodium pump. In this investigation we have analysed the trafficking of gamma to the plasma membrane in cultures of inner medullary collecting duct cells (IMCD3) following acute hypertonic challenge and brefeldin A (BFA) treatment. Following hypertonic challenging for 24 hr immunofluorescence labeling revealed initial co-localization of the gamma subunit and 58K Golgi protein in the cytoplasm, but no co-localization of alpha1 and Golgi protein. Exposure of the challenged cells to BFA prevented the subsequent incorporation of gamma into the basolateral plasma membrane. The gamma subunit instead remained in cytoplasmic vesicles while cell proliferation and cell viability decreased simultaneously. Following removal of BFA from the hypertonic medium the IMCD3 cells recovered with distinct expression of gamma in the basolateral membrane. The alpha1 subunit was only marginally influenced by BFA. The results demonstrate that the gamma subunit trafficks to the plasma membrane via the Golgi apparatus, despite the absence of a signal sequence. The results also suggest that the gamma and alpha subunits do not traffic together to the plasma membrane, and that the gamma and alpha subunit have different turnover rates during these experimental conditions.

Published
2008
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18. Localization of electrogenic Na/bicarbonate cotransporter NBCe1 variants in rat brain.

Author

Majumdar D, Maunsbach AB, Shacka JJ, Williams JB, Berger UV, Schultz KP, Harkins LE, Boron WF, Roth KA, and Bevensee MO

Subjects
Animals, Brain cytology, Microscopy, Immunoelectron methods, Nerve Tissue Proteins genetics, Nerve Tissue Proteins metabolism, Neurons metabolism, Neurons ultrastructure, Protein Isoforms genetics, Rats, Sodium-Bicarbonate Symporters genetics, Brain metabolism, Protein Isoforms metabolism, Sodium-Bicarbonate Symporters metabolism
Abstract

The activity of HCO(3)(-) transporters contributes to the acid-base environment of the nervous system. In the present study, we used in situ hybridization, immunoblotting, immunohistochemistry, and immunogold electron microscopy to localize electrogenic Na/bicarbonate cotransporter NBCe1 splice variants (-A, -B, and -C) in rat brain. The in situ hybridization data are consistent with NBCe1-B and -C, but not -A, being the predominant NBCe1 variants in brain, particularly in the cerebellum, hippocampus, piriform cortex, and olfactory bulb. An antisense probe to the B and C variants strongly labeled granule neurons in the dentate gyrus of the hippocampus, and cells in the granule layer and Purkinje layer (e.g. Bergmann glia) of the cerebellum. Weaker labeling was observed in the pyramidal layer of the hippocampus and in astrocytes throughout the brain. Similar, but weaker labeling was obtained with an antisense probe to the A and B variants. In immunoblot studies, antibodies to the A and B variants (alphaA/B) and C variant (alphaC) labeled approximately 130-kDa proteins in various brain regions. From immunohistochemistry data, both alphaA/B and alphaC exhibited diffuse labeling throughout brain, but alphaA/B labeling was more intracellular and punctate. Based on co-localization studies with antibodies to neuronal or astrocytic markers, alphaA/B labeled neurons in the pyramidal layer and dentate gyrus of the hippocampus, as well as cortex. alphaC labeled glia surrounding neurons (and possibly neurons) in the neuropil of the Purkinje cell layer of the cerebellum, the pyramidal cell layer and dentate gyrus of the hippocampus, and the cortex. According to electron microscopy data from the cerebellum, alphaA/B primarily labeled neurons intracellularly and alphaC labeled astrocytes at the plasma membrane. In summary, the B and C variants are the predominant NBCe1 variants in rat brain and exhibit different localization profiles.

Published
2008
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19. A metabonomic and proteomic analysis of changes in IMCD3 cells chronically adapted to hypertonicity.

Author

Klawitter J, Rivard CJ, Brown LM, Capasso JM, Almeida NE, Maunsbach AB, Pihakaski-Maunsbach K, Berl T, Leibfritz D, Christians U, and Chan L

Subjects
Adaptation, Physiological, Amino Acids metabolism, Animals, Blotting, Western, Cell Line, Cell Proliferation, Electrophoresis, Gel, Two-Dimensional, Enzymes genetics, Glucose metabolism, Kidney Medulla enzymology, Kidney Medulla ultrastructure, Kidney Tubules, Collecting enzymology, Kidney Tubules, Collecting ultrastructure, Mice, Microscopy, Electron, Transmission, Mitochondria metabolism, Nuclear Magnetic Resonance, Biomolecular, Osmotic Pressure, Phenotype, Phosphates metabolism, Polymers metabolism, Reverse Transcriptase Polymerase Chain Reaction, Saline Solution, Hypertonic, Energy Metabolism, Enzymes metabolism, Kidney Medulla metabolism, Kidney Tubules, Collecting metabolism, Proteomics methods
Abstract

Background: The genomic response to adaptation of IMCD3 cells to hypertonicity results in both upregulation and downregulation of a variety of genes., Method: The present study was undertaken to assess the metabonomic and proteomic response of IMCD3 cells that have been chronically adapted to hypertonicity (600 and 900 mosm/kg H(2)O) as compared to cells under isotonic conditions., Results: Adaptation of IMCD3 cells to hypertonic conditions resulted in a change of a wide range of organic osmolytes, including sorbitol (+8,291%), betaine (+1,099%), myo-inositol (+669%), taurine (+113%) and glycerophosphorylcholine (+61%). Evaluation of the polyol pathway for sorbitol production revealed a reduction in sorbitol dehydrogenase and an increase in aldose reductase mRNA in adapted cells. Proteome analysis revealed increased expression of six glycolytic proteins, including malic enzyme and pyruvate carboxylase, indicating the activation of the pyruvate shunt and changes in glucose metabolism. This study showed that the observed reduction in cell replication could possibly reflect a redirection of cellular energy from cell growth and replication to maintenance of intracellular ion levels in chronically adapted cells., Conclusion: The combined metabonomic and proteomic analysis was shown to be a very helpful tool for the analysis of the effects caused by chronic adaptation to hypertonicity. It made it possible to better evaluate the importance of certain changes that occur in the process of adaptation., (Copyright 2008 S. Karger AG, Basel.)

Published
2008
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20. Controversies in nephrology: renal albumin handling, facts, and artifacts!

Author

Christensen EI, Birn H, Rippe B, and Maunsbach AB

Subjects
Albumins ultrastructure, Animals, Autoradiography, Biological Transport, Endocytosis, Glomerular Filtration Rate, Iodine Radioisotopes metabolism, Kidney Tubules, Proximal physiology, Kidney Tubules, Proximal ultrastructure, Rats, Rats, Sprague-Dawley, Albumins metabolism, Artifacts, Kidney chemistry, Kidney physiology
Abstract

In this article, we discuss and contradict a recent publication by Russo et al., which suggests that the filtration of large amounts of albumin followed by transtubular transport of intact albumin is a physiological phenomenon.

Published
2007
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21. ANG II provokes acute trafficking of distal tubule Na+-Cl(-) cotransporter to apical membrane.

Author

Sandberg MB, Riquier AD, Pihakaski-Maunsbach K, McDonough AA, and Maunsbach AB

Subjects
Angiotensin-Converting Enzyme Inhibitors pharmacology, Animals, Captopril pharmacology, Gene Expression Regulation, Kidney Tubules, Distal cytology, Kidney Tubules, Distal drug effects, Microscopy, Immunoelectron, Protein Transport, Rats, Rats, Sprague-Dawley, Receptors, Drug genetics, Sodium Chloride Symporters genetics, Angiotensin II metabolism, Kidney Tubules, Distal metabolism, Receptors, Drug metabolism, Sodium Chloride Symporters metabolism
Abstract

The distal convoluted tubule (DCT) Na+-Cl(-) cotransporter (NCC), the target of thiazide diuretics, is responsible for the reabsorption of 5-10% of filtered NaCl. The aim of this study was to test the hypothesis that acute infusion of the angiotensin-converting enzyme (ACE) inhibitor captopril (at 12 microg/min) for 20 min provokes trafficking of NCC from apical plasma membranes (APM) to subapical cytoplasmic vesicles (SCV), which is reversed by acute ANG II infusion (ANG II at 20 ng.kg(-1).min(-1) along with 12 microg/min captopril) for 20 min in male Sprague-Dawley rats (250-350 g). By immuno-electron microscopy using an anti-NCC (D. Ellison) 71.5 +/- SD 4.9% of the NCC gold labeling was associated with the APM in control, sham operated, and infused rats, while captopril infusion reduced NCC in APM to 54.9 +/- 6.9% (P < 0.001) and markedly increased immunogold labeling of SCV. Subsequent infusion of ANG II with captopril restored NCC immunogold labeling of APM to 72.4 +/- 4.2%, that is, 20% of the total NCC trafficked between APM and SCV. Likewise, on density gradients of cortex, captopril provoked redistribution of 27.3% of total NCC from low-density APM-enriched membranes to higher-density membranes and ANG II+captopril restored 20.3% of the NCC to APM-enriched fractions. Redistribution occurred independent of a change in NCC total abundance. In conclusion, this study demonstrates that ACE inhibition provokes acute trafficking of NCC out of the plasma membrane, which likely decreases DCT Na+ reabsorption, while ANG II provokes rapid trafficking of NCC from stores in subapical vesicles to the plasma membrane, which likely increases DCT Na+ reabsorption.

Published
2007
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22. Expression of the calcium-binding protein S100A4 is markedly up-regulated by osmotic stress and is involved in the renal osmoadaptive response.

Author

Rivard CJ, Brown LM, Almeida NE, Maunsbach AB, Pihakaski-Maunsbach K, Andres-Hernando A, Capasso JM, and Berl T

Subjects
Adaptation, Physiological, Animals, Calcium-Binding Proteins, Cell Line, Chromatography, High Pressure Liquid, Gene Expression Regulation, Humans, Kidney cytology, Mass Spectrometry, Mice, Proteomics, S100 Calcium-Binding Protein A4, S100 Proteins analysis, Kidney physiology, Osmotic Pressure, S100 Proteins genetics, S100 Proteins physiology, Up-Regulation genetics
Abstract

Proteomic analysis of Inner Medullary Collecting Duct (IMCD3) cells adapted to increasing levels of tonicity (300, 600, and 900 mosmol/kg H(2)O) by two-dimensional difference gel electrophoresis and mass spectrometry revealed several proteins as yet unknown to be up-regulated in response to hypertonic stress. Of these proteins, one of the most robustly up-regulated (22-fold) was S100A4. The identity of the protein was verified by high pressure liquid chromatography-mass spectrometry. Western blot analysis confirmed increased expression with increased tonicity, both acute and chronic. S100A4 protein expression was further confirmed by immunocytochemical analysis. Cells grown in isotonic conditions showed complete absence of immunostaining, whereas chronically adapted IMCD3 cells had uniform cytoplasmic localization. The protein is also regulated in vivo as in mouse kidney tissues S100A4 expression was many -fold greater in the papilla as compared with the cortex and increased further in the papilla upon 36 h of thirsting. Increased expression of S100A4 was also observed in the medulla and papilla, but not the cortex of a human kidney. Data from Affymetrix gene chip analysis and quantitative PCR also revealed increased S100A4 message in IMCD3 cells adapted to hypertonicity. The initial expression of message increased at 8-10 h following exposure to acute sublethal hypertonic stress (550 mosmol/kg H(2)O). Protein and message half-life in IMCD3 cells were 85.5 and 6.8 h, respectively. Increasing medium tonicity with NaCl, sucrose, mannitol, and choline chloride stimulated S100A4 expression, whereas urea did not. Silencing of S100A4 expression using a stable siRNA vector (pSM2; Open Biosystems) resulted in a 48-h delay in adaptation of IMCD3 cells under sublethal osmotic stress, suggesting S100A4 is involved in the osmoadaptive response. In summary, we describe the heretofore unrecognized up-regulation of a small calcium-binding protein, both in vitro and in vivo, whose absence profoundly delays osmoadaptation and slows cellular growth under hypertonic conditions.

Published
2007
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23. Locations, abundances, and possible functions of FXYD ion transport regulators in rat renal medulla.

Author

Pihakaski-Maunsbach K, Vorum H, Honoré B, Tokonabe S, Frøkiaer J, Garty H, Karlish SJ, and Maunsbach AB

Subjects
Animals, Diet, Sodium-Restricted, Fluorescent Antibody Technique, Kidney Medulla ultrastructure, Male, Microscopy, Immunoelectron, Rats, Rats, Wistar, Sodium Chloride metabolism, Sodium Chloride pharmacology, Intracellular Signaling Peptides and Proteins metabolism, Kidney Medulla metabolism, Potassium Channels metabolism, Sodium-Potassium-Exchanging ATPase metabolism
Abstract

The gamma-subunit of Na-K-ATPase (FXYD2) and corticosteroid hormone-induced factor (CHIF; FXYD4) are considered pump regulators in kidney tubules. The aim of this study was to expand the information about their locations in the kidney medulla and to evaluate their importance for electrolyte excretion in an animal model. The cellular and subcellular locations and abundances of gamma and CHIF in the medulla of control and sodium-depleted rats were analyzed by immunofluorescence and immunoelectron microscopy and semiquantitative Western blotting. The results showed that antibodies against the gamma-subunit COOH terminus and splice variant gamma(a), but not splice variant gamma(b), labeled intercalated cells, but not principal cells, in the initial part of the inner medullary collecting duct (IMCD1). In subsequent segments (IMCD2 and IMCD3), all principal cells exhibited distinct basolateral labeling for both the gamma-subunit COOH terminus, splice variant gamma(a), and CHIF. Splice variant gamma(b) was abundant in the inner stripe of the outer medulla but absent in the inner medulla (IM). Double labeling by high-resolution immunoelectron microscopy showed close structural association between CHIF and the Na-K-ATPase alpha(1)-subunit in basolateral membranes. The present observations provide new information about the cellular and subcellular locations of gamma and CHIF in the renal medulla and show a new gamma variant in the IM. Extensive NaCl depletion did not induce significant changes in the locations or abundances of the gamma-subunit COOH terminus and CHIF in different kidney zones. We conclude that the unchanged levels of these two FXYD proteins suggest that they are not primary determinants for urine electrolyte composition during NaCl depletion.

Published
2006
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24. Redistribution of distal tubule Na+-Cl- cotransporter (NCC) in response to a high-salt diet.

Author

Sandberg MB, Maunsbach AB, and McDonough AA

Subjects
Absorption, Animals, Animals, Newborn physiology, Cell Membrane chemistry, Cell Membrane physiology, Centrifugation, Density Gradient, Homeostasis physiology, Immunohistochemistry, Kidney Tubules, Distal physiology, Microscopy, Immunoelectron, Rats, Rats, Sprague-Dawley, Sodium Chloride metabolism, Sodium Chloride Symporters physiology, Kidney Tubules, Distal chemistry, Kidney Tubules, Distal drug effects, Sodium Chloride Symporters analysis, Sodium Chloride, Dietary pharmacology
Abstract

The distal convoluted tubule (DCT) apical Na(+)-Cl(-) cotransporter (NCC) is responsible for the reabsorption of 5-10% of filtered NaCl and is the target for thiazide diuretics. NCC abundance is increased during dietary NaCl restriction and by aldosterone and decreased during a high-salt (HS) diet and mineralocorticoid blockade. This study tested the hypothesis that subcellular distribution of NCC is also regulated in response to changes in dietary salt. Six-week-old Sprague-Dawley rats were fed a normal-salt diet (NS; 0.4% NaCl) for 3 wk, then switched to a HS diet (4% NaCl) for 3 wk or a low-salt diet (LS; 0.07% NaCl) for 1 wk. Under anesthesia, kidneys were excised, renal cortex was dissected, and NCC was analyzed with specific antibodies after either 1) density gradient centrifugation followed by immunoblotting or 2) fixation followed by immunoelectron microscopy. The HS diet decreased NCC abundance to 0.50 +/- 0.10 of levels in LS diet (1.00 +/- 0.23). The HS diet also caused a redistribution of NCC from low to higher density membranes. Immunoelectron microscopy revealed that NCC resides predominantly in the apical membrane in rats fed the LS diet and increases in subapical vesicles in rats fed the HS diet. In conclusion, a HS diet provokes a rapid and persistent redistribution of NCC from apical to subapical membranes, a mechanism that would facilitate a homeostatic decrease in NaCl reabsorption in the DCT to compensate for increased dietary salt.

Published
2006
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25. Structural characterization of Na,K-ATPase from shark rectal glands by extensive trypsinization.

Author

Esmann M, Arora A, Maunsbach AB, and Marsh D

Subjects
Amino Acid Sequence, Animals, Ion Channels, Models, Molecular, Molecular Sequence Data, Peptide Fragments, Protein Conformation, Salt Gland enzymology, Sharks, Sodium-Potassium-Exchanging ATPase chemistry, Sodium-Potassium-Exchanging ATPase metabolism, Trypsin metabolism
Abstract

Extensive trypsinization of Na,K-ATPase from the salt gland of Squalus acanthias removes about half of the extramembranous protein mass of the alpha-subunit, while leaving the beta-subunit intact. Sequence analysis and epitope recognition of the remaining alpha-peptides show that transmembrane segments M1/M2 and M3/M4 are present when trypsinization is performed in either NaCl or RbCl. The M5/M6 segment and the intact 19-kDa peptide (M7-M10) are detected in Rb-trypsinized membranes but not in Na-trypsinized membranes. The L7/L8 loop is associated with Na-trypsinized membranes, indicating the presence of an M7/M8 or M8/M9 fragment. Freeze-fracture electron microscopy of both Rb- and Na-trypsinized membranes reveals intramembranous particles that indicate a retained cluster of peptides, even in the absence of an intact 19-kDa fragment. The rotational diffusion of covalently spin-labeled trypsinized complexes is studied in the presence of poly(ethylene glycol) or glycerol by using saturation transfer electron spin resonance. Rotational correlation times in aqueous poly(ethylene glycol) are longer than in glycerol solutions of the same viscosity and increase nonlinearly with the viscosity of the suspending medium, indicating that poly(ethylene glycol) induces aggregation of the tryptic peptides (and beta-subunit) within the membrane. The aggregates of enzyme trypsinized in the presence of NaCl are larger than those for enzyme trypsinized in RbCl, at both low and high aqueous viscosities. Similarities in mobility for native and Rb-trypsinized enzymes suggest either a change in average orientation of the spin-label upon trypsinization or that trypsinization leads to a reorganized protein structure that is more prone to aggregation.

Published
2006
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26. Association of renal Na,K-ATPase alpha-subunit with the beta- and gamma-subunits based on cryoelectron microscopy.

Author

Purhonen P, Thomsen K, Maunsbach AB, and Hebert H

Subjects
Animals, Cryoelectron Microscopy, Protein Structure, Quaternary, Swine, Kidney chemistry, Models, Molecular, Multiprotein Complexes chemistry, Multiprotein Complexes ultrastructure, Protein Subunits chemistry, Sodium-Potassium-Exchanging ATPase chemistry
Abstract

Na,K-ATPase transports Na(+) and K(+) across cell membranes and consists of alpha- and beta-subunits. Na,K-ATPase also associates with small FXYD proteins that regulate the activity of the pump. We have used cryoelectron microscopy of two-dimensional crystals including data to 8 A resolution to determine the three-dimensional (3-D) structure of renal Na,K-ATPase containing FXYD2, the gamma-subunit. A homology model for the alpha-subunit was calculated from a Ca(2+)-ATPase structure and used to locate the additional beta- and gamma-subunits present in the 3-D map of Na,K-ATPase. Based on the 3-D map, the beta-subunit is located close to transmembrane helices M8 and M10 and the gamma-subunit is adjacent to helices M2 and M9 of the alpha-subunit.

Published
2006
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27. Interaction with the Na,K-ATPase and tissue distribution of FXYD5 (related to ion channel).

Author

Lubarski I, Pihakaski-Maunsbach K, Karlish SJ, Maunsbach AB, and Garty H

Subjects
Animals, Gene Expression Regulation, Enzymologic, Ion Channels, Kidney enzymology, Kidney metabolism, Kidney ultrastructure, Membrane Proteins genetics, Mice, Mice, Inbred ICR, Microfilament Proteins, Oocytes metabolism, Organ Specificity, Protein Binding, Rats, Sodium-Potassium-Exchanging ATPase genetics, Swine, Xenopus laevis, Membrane Proteins metabolism, Sodium-Potassium-Exchanging ATPase metabolism
Abstract

FXYD5 (related to ion channel, dysadherin) is a member of the FXYD family of single span type I membrane proteins. Five members of this group have been shown to interact with the Na,K-ATPase and to modulate its properties. However, FXYD5 is structurally different from other family members and has been suggested to play a role in regulating E-cadherin and promoting metastasis (Ino, Y., Gotoh, M., Sakamoto, M., Tsukagoshi, K., and Hirohashi, S. (2002) Proc. Natl. Acad. Sci. U. S. A. 99, 365-370). The goal of this study was to determine whether FXYD5 can modulate the Na,K-ATPase activity, establish its cellular and tissue distribution, and characterize its biochemical properties. Anti-FXYD5 antibodies detected a 24-kDa polypeptide that was preferentially expressed in kidney, intestine, spleen, and lung. In kidney, FXYD5 resides in the basolateral membrane of the connecting tubule, the collecting tubule, and the intercalated cells of the collecting duct. However, there is also labeling of the apical membrane in long thin limb of Henle's loop. FXYD5 was effectively immunoprecipitated by antibodies to the alpha subunit of Na,K-ATPase and the anti-FXYD5 antibody immunoprecipitates alpha. Co-expressing FXYD5 with the alpha1 and beta1 subunits of the Na,K-ATPase in Xenopus oocytes elicited a more than 2-fold increase in pump activity, measured either as ouabain-blockable outward current or as ouabain-sensitive (86)Rb(+) uptake. Thus, as found with other FXYD proteins, FXYD5 interacts with the Na,K-ATPase and modulates its properties.

Published
2005
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28. Redistribution of myosin VI from top to base of proximal tubule microvilli during acute hypertension.

Author

Yang LE, Maunsbach AB, Leong PK, and McDonough AA

Subjects
Acute Disease, Animals, Male, Microvilli, Protein Transport, Rats, Rats, Sprague-Dawley, Sodium-Hydrogen Exchanger 3, Sodium-Hydrogen Exchangers metabolism, Hypertension metabolism, Kidney Tubules, Proximal metabolism, Kidney Tubules, Proximal ultrastructure, Myosin Heavy Chains metabolism
Abstract

During acute hypertension, Na(+)/H(+) exchangers (NHE3) retract from top to base of proximal tubule microvilli (MV) and Na(+) reabsorption decreases in proximal tubule. This study aimed to determine whether the actin-based motor myosin VI coordinately retracts with NHE3 in response to acute hypertension. BP was raised approximately 50 mmHg in rats for 20 to 30 min or sham treated, and kidneys were analyzed by subcellular fractionation or microscopy. During acute hypertension, myosin VI redistributed from low density apical MV-enriched membranes (from 23 +/- 2.4 to 11.4 +/- 2.2%) into higher density membranes (from 23.2 +/- 0.7 to 36.9 +/- 2.6%). By confocal microscopy, myosin VI was detected over the whole length of the MV in controls, then became completely focused at the base of MV during acute hypertension. For electron microscopic analysis using immunogold labeling, MV were divided into five zones from top (z1) to base (z5). In controls, myosin VI was evenly distributed through the five MV zones. In acute hypertension, myosin VI decreased in z1 (from 20.6 +/- 1.9 to 10.5 +/- 2.3%) and z2 (from 21.0 +/- 2.0 to 13.2 +/- 1.4%) and increased in z5 (from 21.1 +/- 3.3 to 38.6 +/- 3.0%). These results provide the first observation that acute hypertension causes myosin VI redistribution and support the idea that myosin VI may serve as the molecular motor for NHE3 retraction from top to base of MV during acute hypertension.

Published
2005
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29. The gamma-subunit of Na-K-ATPase is incorporated into plasma membranes of mouse IMCD3 cells in response to hypertonicity.

Author

Pihakaski-Maunsbach K, Tokonabe S, Vorum H, Rivard CJ, Capasso JM, Berl T, and Maunsbach AB

Subjects
Adaptation, Physiological, Animals, Blotting, Western, Cell Polarity, Cells, Cultured, Hypertonic Solutions, Immunohistochemistry, Kidney Medulla cytology, Mice, Osmotic Pressure, Cell Membrane metabolism, Kidney Medulla enzymology, Sodium-Potassium-Exchanging ATPase metabolism, Water-Electrolyte Balance physiology
Abstract

Hypertonicity mediated by chloride upregulates the expression of the gamma-subunit of Na-K-ATPase in cultured cells derived from the murine inner medullary collecting duct (IMCD3; Capasso JM, Rivard CJ, Enomoto LM, and Berl T. Proc Natl Acad Sci USA 100: 6428-6433, 2003). The purpose of this study was to examine the cellular locations and the time course of gamma-subunit expression after long-term adaptation and acute hypertonic challenges induced with different salts. Cells were analyzed by confocal immunofluorescence and immunoelectron microscopy with antibodies against the COOH terminus of the Na-K-ATPase gamma-subunit or the gamma(b) splice variant. Cells grown in 300 mosmol/kgH(2)O showed no immunoreactivity for the gamma-subunit, whereas cells adapted to 600 or 900 mosmol/kgH(2)O demonstrated distinct reactivity located at the plasma membrane of all cells. IMCD3 cell cultures acutely challenged to 550 mosmol/kgH(2)O with sodium chloride or choline chloride showed incorporation of gamma into plasma membrane 12 h after osmotic challenge and distinct membrane staining in approximately 40% of the cells 48 h after osmotic shock. In contrast, challenging the IMCD3 cells to 550 mosmol/kgH(2)O by addition of sodium acetate did not result in expression of the gamma-subunit in the membranes of surviving cells after 48 h. The present results demonstrate that the Na-K-ATPase gamma-subunit becomes incorporated into the basolateral membrane of IMCD3 cells after both acute hyperosmotic challenge and hyperosmotic adaptation. We conclude that the gamma-subunit has an important role in the function of Na-K-ATPase to sustain the cellular cation balance over the plasma membrane in a hypertonic environment.

Published
2005
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30. Differential traffic of proximal tubule Na+ transporters during hypertension or PTH: NHE3 to base of microvilli vs. NaPi2 to endosomes.

Author

Yang LE, Maunsbach AB, Leong PK, and McDonough AA

Subjects
Animals, Blotting, Western, Fluorescent Antibody Technique, Indirect, Kidney Cortex cytology, Kidney Cortex drug effects, Kidney Cortex metabolism, Lysosomes metabolism, Male, Microscopy, Confocal, Microscopy, Immunoelectron, Phosphates metabolism, Rats, Rats, Sprague-Dawley, Sodium-Hydrogen Exchanger 3, Subcellular Fractions metabolism, Endosomes metabolism, Hypertension, Renal metabolism, Kidney Tubules, Proximal metabolism, Microvilli metabolism, Parathyroid Hormone pharmacology, Sodium metabolism, Sodium-Hydrogen Exchangers metabolism
Abstract

We previously reported that Na(+)/H(+) exchanger type 3 (NHE3) and NaPi2 are acutely retracted from the proximal tubule (PT) microvilli (MV) during acute hypertension [high blood pressure (BP)] or parathyroid hormone (PTH) treatment. By subcellular membrane fractionation, NHE3 and NaPi2 show indistinguishable redistribution patterns out of light-density into heavy-density membranes in response to either treatment consistent with a retraction from the apical MV to the intermicrovillar cleft region. This study aimed to examine the redistribution of PT NHE3 vs. NaPi2 by confocal and electron microscopy during high BP and during PTH treatment to determine whether their respective destinations overlap or are distinct. High-BP protocol: systolic BP was increased 50-60 mmHg by increasing peripheral resistance for 20 min; PTH protocol: rats were infused with 6.6 microg/kg iv of PTH followed by 0.1 microg.kg(-1).min(-1) infusion for 1 h. For light microscopy, rats were infused with 25 mg of horseradish peroxidase (HRP) 10 min before kidney fixation. Kidney slices were dual labeled with either NHE3 or NaPi2 and either clathrin-coated vesicle adaptor protein AP2 or endosome marker HRP. The results demonstrate retraction of NHE3 from the MV to the base of MV during either high-BP or PTH treatment: NHE3 staining did not retract below the AP2-stained domain or to HRP-labeled endosomes in either model. In comparison, NaPi2 was retracted from MV to below the AP2-stained region in both models, a little colocalizing with HRP staining. At the electron microscopic level with immunogold labeling, during high BP NHE3 was concentrated in a distinct domain in the base of the MV while NaPi2 moved to endosomes. The results demonstrate that there are divergent routes of retraction of PT NHE3 and NaPi2 from the MV during acute hypertension or PTH treatment: NHE3 is not internalized but remains at the base of the MV while NaPi2 is internalized.

Published
2004
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31. [Status report on the research of Na,K-ATPase, Ca-ATPase and other P-type cation pumps].

Author

Jørgensen PL, Karlish SJ, and Maunsbach AB

Subjects
Humans, Research, Calcium-Transporting ATPases chemistry, Calcium-Transporting ATPases genetics, Calcium-Transporting ATPases physiology, Cation Transport Proteins chemistry, Cation Transport Proteins genetics, Cation Transport Proteins physiology, Sodium-Potassium-Exchanging ATPase chemistry, Sodium-Potassium-Exchanging ATPase genetics, Sodium-Potassium-Exchanging ATPase physiology
Published
2004

32. Biological ultrastructure research; the first 50 years.

Author

Afzelius BA and Maunsbach AB

Subjects
Cell Biology history, History, 20th Century, Imaging, Three-Dimensional trends, Microscopy, Electron methods, Microscopy, Electron history, Microscopy, Electron trends
Abstract

The second half of the 20th century has witnessed the birth and growth of biological ultrastructure research--a branch of cell biology in which electron microscopy plays an important role. After a humble start in around 1950, when only a limited arsenal of instrumentation was available, a wealth of auxiliary methodologies were developed and gradually put in use. Here we review these techniques: ultramicrotomy of "optimally" fixed and prepared samples, histochemical methods such as immuno-electron microscopy and electron microscope autoradiography, negative staining techniques, freeze-fracturing and other techniques. Closer to the millennium shift, various cryotechniques have gradually developed. Together with computer-based reconstruction methods they are likely to play increasingly more important roles in the future.

Published
2004
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33. Changes of rat kidney AQP2 and Na,K-ATPase mRNA expression in lithium-induced nephrogenic diabetes insipidus.

Author

Laursen UH, Pihakaski-Maunsbach K, Kwon TH, Østergaard Jensen E, Nielsen S, and Maunsbach AB

Subjects
Animals, Aquaporin 2, Aquaporins genetics, Diabetes Insipidus, Nephrogenic genetics, Down-Regulation, Gene Expression drug effects, Kidney metabolism, Kidney Tubules, Collecting ultrastructure, Male, RNA, Messenger metabolism, Rats, Rats, Wistar, Sodium-Potassium-Exchanging ATPase genetics, Aquaporins metabolism, Diabetes Insipidus, Nephrogenic chemically induced, Diabetes Insipidus, Nephrogenic metabolism, Lithium toxicity, Sodium-Potassium-Exchanging ATPase metabolism
Abstract

Background/aim: In a rat model, lithium treatment is associated with polyuria and severe downregulation of aquaporin-2 (AQP2) protein in the inner medulla (IM) or in the whole kidney. However, it is not known (1) to what extent this downregulation occurs at the mRNA level; (2) whether the main sodium transporter of the nephron, Na,K-ATPase, is regulated in parallel at the mRNA level, and (3) whether lithium treatment induces zonal or segmental differences in AQP2 and Na,K-ATPase mRNA levels., Method: We examined the changes in mRNA expression levels for AQP2 and Na,K-ATPase in kidney cortex, inner stripe of the outer medulla (ISOM), and IM of rats treated with lithium orally using semiquantitative Northern blot analyses and in situ hybridization at the light and electron microscopic levels., Results: The AQP2 mRNA levels decreased significantly (p < 0.01) in lithium-treated rats to 37 +/- 4% in the cortex, to 17 +/- 4% in the ISOM, and to 23 +/- 5% in the IM, while the Na,K-ATPase mRNA levels were not altered in the cortex, but were significantly (p < 0.05) altered in the ISOM (144 +/- 15% after 10 days, but 68 +/- 4% after 4 weeks) and in the IM (63 +/- 8% after 10 days, but normalized after 4 weeks). In situ hybridization showed reduced levels of AQP2 mRNA in all zones of the kidney, but the Na,K-ATPase mRNA expressions were slightly decreased only in IM collecting ducts. At the ultrastructural level, principal cells in the IM collecting ducts showed slight hypertrophy, but no cell damage after 4 weeks of lithium treatment. The results demonstrate substantial downregulation of AQP2 at the mRNA level throughout the collecting duct in experimental lithium-induced nephrogenic dabetes insipidus and moderately decreased Na,K-ATPase mRNA levels in the ISOM and in the IM., Conclusion: The results suggest that decreased mRNA expressions of AQP2 and Na,K-ATPase contribute to the development of lithium-induced nephrogenic diabetes insipidus., (Copyright 2004 S. Karger AG, Basel)

Published
2004
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34. Regulation of Na,K-ATPase by PLMS, the phospholemman-like protein from shark: molecular cloning, sequence, expression, cellular distribution, and functional effects of PLMS.

Author

Mahmmoud YA, Cramb G, Maunsbach AB, Cutler CP, Meischke L, and Cornelius F

Subjects
Adenosine Triphosphate metabolism, Amino Acid Sequence, Animals, Base Sequence, Chloride Channels, Cloning, Molecular, Fish Proteins analysis, Fish Proteins genetics, Immunohistochemistry, Molecular Sequence Data, Phosphoproteins analysis, Phosphoproteins genetics, Phosphorylation, Potassium metabolism, Protein Subunits, Sharks, Sodium-Potassium-Exchanging ATPase chemistry, Trypsin pharmacology, Fish Proteins physiology, Phosphoproteins physiology, Sodium-Potassium-Exchanging ATPase metabolism
Abstract

In Na,K-ATPase membrane preparations from shark rectal glands, we have previously identified an FXYD domain-containing protein, phospholemman-like protein from shark, PLMS. This protein was shown to associate and modulate shark Na,K-ATPase activity in vitro. Here we describe the complete coding sequence, expression, and cellular localization of PLMS in the rectal gland of the shark Squalus acanthias. The mature protein contained 74 amino acids, including the N-terminal FXYD motif and a C-terminal protein kinase multisite phosphorylation motif. The sequence is preceded by a 20 amino acid candidate cleavable signal sequence. Immunogold labeling of the Na,K-ATPase alpha-subunit and PLMS showed the presence of alpha and PLMS in the basolateral membranes of the rectal gland cells and suggested their partial colocalization. Furthermore, through controlled proteolysis, the C terminus of PLMS containing the protein kinase phosphorylation domain can be specifically cleaved. Removal of this domain resulted in stimulation of maximal Na,K-ATPase activity, as well as several partial reactions. Both the E1 approximately P --> E2-P reaction, which is partially rate-limiting in shark, and the K+ deocclusion reaction, E2(K) --> E1, are accelerated. The latter may explain the finding that the apparent Na+ affinity was increased by the specific C-terminal PLMS truncation. Thus, these data are consistent with a model where interaction of the phosphorylation domain of PLMS with the Na,K-ATPase alpha-subunit is important for the modulation of shark Na,K-ATPase activity.

Published
2003
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36. Immunocytochemical localization of Na,K-ATPase gamma subunit and CHIF in inner medulla of rat kidney.

Author

Pihakaski-Maunsbach K, Vorum H, Løcke EM, Garty H, Karlish SJ, and Maunsbach AB

Subjects
Animals, Blotting, Western, Immunohistochemistry, Membrane Proteins analysis, Microscopy, Immunoelectron, Rats, Rats, Wistar, Sodium-Potassium-Exchanging ATPase analysis, Kidney Medulla enzymology, Membrane Proteins metabolism, Sodium-Potassium-Exchanging ATPase metabolism
Abstract

The gamma subunit of Na,K-ATPase and CHIF both belong to the FXYD single-membrane-spanning protein family and have been suggested to have regulatory functions in kidney tubules. CHIF is known to be present in the collecting duct, and gamma has been demonstrated in several segments of the rat kidney tubule, but never clearly in the inner medullary collecting duct (IMCD). Here, we demonstrate the cellular and subcellular localization of the gamma subunit and CHIF in the IMCD in inner medulla by using Western blotting, laser-scanning confocal immunofluorescence, and immunoelectron microscopy. In the initial quarter of the IMCD (next to the outer medulla), antibodies against the C-terminal of gamma as well as splice variant gammaa labeled the basolateral surface of intercalated cells (ICs), while principal cells (PCs) remained unlabeled. In the middle segment of the IMCD, all PCs exhibited distinct basolateral staining for the gammaC-terminal as well as gammaa and CHIF. Immunoelectron microscopy showed that the gammaC-terminal and CHIF were associated with the inner leaflet of the basolateral plasma membrane in the labeled cells. Immunoblotting demonstrated the presence of both the gammaC-terminal and gammaa in inner medullary tissue. However, splice variant gammab was not detected in inner medulla by immunocytochemistry or immunoblotting. The present observations demonstrate that the Na,K-ATPase gamma subunit and CHIF are strategically located in the inner medulla to participate in the fine-tuning of urine ion composition through the regulation of the Na,K-ATPase activity in the IMCD.

Published
2003
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37. Renal Na,K-ATPase structure from cryo-electron microscopy of two-dimensional crystals.

Author

Hebert H, Purhonen P, Thomsen K, Vorum H, and Maunsbach AB

Subjects
Animals, Cryoelectron Microscopy, Crystallography, X-Ray, Models, Molecular, Protein Structure, Secondary, Protein Subunits, Sodium-Potassium-Exchanging ATPase isolation & purification, Swine, Kidney Medulla enzymology, Sodium-Potassium-Exchanging ATPase chemistry, Sodium-Potassium-Exchanging ATPase ultrastructure
Abstract

The molecular structure of Na,K-ATPase was determined by electron crystallography from two-dimensional crystals induced in purified membranes isolated from the outer medulla of pig kidney. The P2 type unit cell contains two protomers in the E(2) conformation, each of them with a size of 65 x 75 x 150 A(3). The alpha, beta, and gamma subunits in the membrane crystals were demonstrated in the crystals with Western blotting and related to distinct domains in the density map. The alpha subunit corresponds to most of the density in the transmembrane region as well as to the large hydrophilic headpiece on the cytoplasmic side of the membrane. The headpiece is divided into three separated domains. One of these gives rise to an elongated projection onto the membrane plane, while the putative nucleotide binding and phosphorylation domains form compact densities in the rest of the cytoplasmic part of the structure. Density on the extracellular face corresponds to the protein part of the beta subunit. Ten helices from the catalytic a subunit correspond to two groups of distinct densities in the transmembrane region. The structure of the lipid bilayer spanning part also suggests positions for the transmembrane helices from the beta and gamma subunits. The overall structure of the alpha subunit of Na,K-ATPase as determined here by cryo-electron microscopy is similar to the X-ray structure of Ca-ATPase. However, conformational changes between the E(1) and E(2) forms are suggested by different relative positions of cytoplasmic domains.

Published
2003
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38. Three-dimensional structure of renal Na,K-ATPase from cryo-electron microscopy of two-dimensional crystals.

Author

Hebert H, Purhonen P, Vorum H, Thomsen K, and Maunsbach AB

Subjects
Animals, Blotting, Western, Crystallization, Models, Molecular, Protein Structure, Quaternary, Protein Structure, Secondary, Protein Structure, Tertiary, Protein Subunits, Reproducibility of Results, Sodium-Potassium-Exchanging ATPase metabolism, Cryoelectron Microscopy, Kidney Medulla enzymology, Sodium-Potassium-Exchanging ATPase chemistry, Sodium-Potassium-Exchanging ATPase ultrastructure, Swine
Abstract

The structure of Na, K-ATPase was determined by electron crystallography at 9.5 A from multiple small 2-D crystals induced in purified membranes isolated from the outer medulla of pig kidney. The density map shows a protomer stabilized in the E(2) conformation which extends approximately 65 A x 75 A x 150 A in the asymmetric unit of the P2 type unit cell. The alpha, beta, and gamma subunits were demonstrated in the membrane crystals with Western blotting and related to distinct domains in the density map. The alpha subunit corresponds to most of the density in the transmembrane region as well as the large hydrophilic headpiece on the cytoplasmic side of the membrane. The headpiece is divided into three separated domains, which are similar in overall shape to the domains of the calcium pump of the sarcoplasmic reticulum. One of these domains gives rise to a characteristic elongated projection onto the membrane plane while the putative nucleotide binding and phosphorylation domains form comparatively compact densities in the rest of the cytoplasmic part of the structure. Density on the extracellular face corresponds to the protein part of the beta subunit and is located as an extension of the transmembrane region perpendicular to the membrane plane. The structure of the lipid bilayer spanning part suggests the positions for the transmembrane helix from the beta subunit as well as the small gamma subunit present in this Na,K-ATPase. Two groups of ten helices from the catalytic alpha subunit corresponds to the remaining density in the transmembrane region. The present results demonstrate distinct similarities between the structure of the alpha subunit of Na,K-ATPase as determined here by cryo-electron microscopy and the reported X-ray structure of Ca-ATPase. However, conformational changes between the E(1) and E(2) forms are suggested by different relative positions of cytoplasmatic domains., (Copyright 2001 Academic Press.)

Published
2001
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39. Genes encoding chitinase-antifreeze proteins are regulated by cold and expressed by all cell types in winter rye shoots.

Author

Pihakaski-Maunsbach K, Moffatt B, Testillano P, Risueño M, Yeh S, Griffith M, and Maunsbach AB

Abstract

One group of antifreeze proteins (AFPs) is composed of two chitinases that accumulate in the apoplast of winter rye leaves during cold acclimation. In this study, the 28- and 35-kDa chitinase-AFPs were localized in nonacclimated and cold-acclimated rye leaves by immunoelectron microscopy with an antiserum produced against the purified winter rye 35-kDa chitinase-AFP. In cold-acclimated winter rye leaves, labelled chitinase-AFPs were abundant in the walls of epidermal, parenchymal sheath and mesophyll cells and xylem vessels, while less label was present in walls of vascular parenchyma cells. In contrast, chitinase labelling was essentially absent in the nonacclimated cells except in xylem vessels. As shown by RNA blotting, the transcripts of chitinase-AFPs accumulated to a high level in rye leaves during cold acclimation, to a lesser extent in crowns and were not detectable in roots. mRNA transcripts of the 28-kDa chitinase-AFP were localized in rye leaves by in situ hybridization. The chitinase-AFP transcripts were found in the same cell types as the protein itself. We conclude that all metabolically active cell types in cold-acclimated winter rye leaves and crowns are able to synthesize chitinase-AFPs and secrete them into adjacent cell walls, where they may interact with ice to delay its propagation through the plant and modify its growth.

Published
2001
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40. Cyclooxygenase-1 and cyclooxygenase-2 expression in rat kidney and adrenal gland after stimulation with systemic lipopolysaccharide: in situ hybridization and immunocytochemical studies.

Author

Ichitani Y, Holmberg K, Maunsbach AB, Haeggström JZ, Samuelsson B, De Witt D, and Hökfelt T

Subjects
Adrenal Glands ultrastructure, Animals, Antibodies, Cyclooxygenase 1, Cyclooxygenase 2, Fluorescent Antibody Technique, Indirect, Gene Expression Regulation, Enzymologic drug effects, Gene Expression Regulation, Enzymologic physiology, Immunohistochemistry, In Situ Hybridization, Isoenzymes analysis, Isoenzymes immunology, Kidney ultrastructure, Male, Membrane Proteins, Microscopy, Immunoelectron, Nitric Oxide Synthase analysis, Nitric Oxide Synthase immunology, Prostaglandin-Endoperoxide Synthases analysis, Prostaglandin-Endoperoxide Synthases immunology, RNA, Messenger analysis, Rats, Rats, Sprague-Dawley, Adrenal Glands enzymology, Isoenzymes genetics, Kidney enzymology, Lipopolysaccharides pharmacology, Prostaglandin-Endoperoxide Synthases genetics
Abstract

Cyclooxygenase-2 (COX-2) is a recently discovered isoform of cyclooxygenase that is inducible by various types of inflammatory stimuli. Although this enzyme is considered to play a major role in inflammation processes by catalyzing the production of prostaglandins, the precise location, distribution, and regulation of prostaglandin synthesis remains unclear in several tissues. Using in situ hybridization histochemistry, we investigated the induction of COX-1 and COX-2 mRNA expression after systemic administration of a pyrogen, lipopolysaccharide (LPS), in kidney and adrenal gland in the rat. The COX-2 mRNA signals dramatically increased 1 h after LPS treatment in the kidney outer medulla and adrenal cortex, where almost no or little expression was observed in nontreated animals, and returned to control levels within 24 h. COX-2 mRNA levels increased in the kidney inner medulla 6 h after treatment. There was also a significant increase in mRNA levels in the kidney cortex and adrenal medulla. On the other hand, COX-1 mRNA levels did not show any detectable changes except in the kidney inner medulla, where a significant downregulation of mRNA expression was observed after LPS treatment. Light and electron immunocytochemistry using COX-2 antibodies showed that strong COX-2 immunoreactivity was localized to certain cortical cells of the thick ascending limb of Henle. In addition, based on double-staining with antiserum to nitric oxide synthase (NOS) four further cell populations could be identified in kidney cortex, including weakly COX-2-positive, NOS-positive macula densa cells. After LPS treatment, changes in COX-2 immunoreactivity could be observed in interstitial cells in the kidney medulla and in inner cortical cells in the adrenal gland. These results show that COX-2 is a highly induced enzyme that can be up-regulated in specific cell populations in kidney and adrenal gland in response to inflammation, leading to the elevated levels of prostaglandins seen during fever. In contrast COX-1 mRNA levels remained unchanged in this experimental situation, except for a decrease in kidney inner medulla.

Published
2001
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41. Immunoelectron microscopic localization of the electrogenic Na/HCO(3) cotransporter in rat and ambystoma kidney.

Author

Maunsbach AB, Vorum H, Kwon TH, Nielsen S, Simonsen B, Choi I, Schmitt BM, Boron WF, and AALKJæR C

Subjects
Animals, Immunoblotting, Immunohistochemistry, Microscopy, Immunoelectron, Rabbits, Sodium-Bicarbonate Symporters, Tissue Distribution, Ambystoma metabolism, Carrier Proteins metabolism, Rats metabolism
Abstract

Immunofluorescence analysis has revealed that electrogenic Na(+)/HCO(3)(-) (NBC1) is expressed in the proximal tubule of rat kidney and in the proximal and distal tubules of the salamander AMBYSTOMA: tigrinum kidney. The present study was undertaken to define the detailed subcellular localization of the NBC1 in rat and AMBYSTOMA: kidney using high-resolution immunoelectron microscopy. For this purpose, two rabbit polyclonal antibodies raised against amino acids 928 to 1035 and amino acids 1021 to 1035 of the C-terminus of rat kidney (rkNBC1) were developed. The affinity-purified antibodies revealed a strong band of approximately 140 kD in immunoblots of membranes from rat kidney cortex but no signal in membranes isolated from outer and inner medulla. Deglycosylation reduced the apparent molecular weight to approximately 120 kD, corresponding to the predicted molecular weight. A similar but weaker band was also present in membranes isolated from the lateral part of Ambystoma: kidney. In rat kidney, immunohistochemistry confirmed the presence of rkNBC1 in convoluted segments of the proximal tubules. In ultrathin cryosections or Lowicryl HM20 sections from rat kidney cortex, distinct immunogold labeling was associated with the basolateral plasma membrane of segments S1 and S2 of proximal tubules, whereas in S3 no labeling was observed. The labeling density was similar at the basal and lateral plasma membrane and was specifically associated with the inner surface of the membrane consistent with the internal position of the C-terminus of the transporter. In contrast, rkNBC1 was absent from the apical plasma membrane and not observed in intracellular vesicles, including those closely associated with basolateral plasma membrane. In Ambystoma: kidney, a weak labeling was present in the basolateral membrane of the proximal tubule and stronger labeling was observed in the late distal segment. The results demonstrate that rkNBC1 is expressed only in segment S1 and segment S2 of rat proximal tubule as well as Ambystoma: proximal and late distal tubule and that rkNBC1 is present in both basal and lateral plasma membranes and absent in intracellular vesicles of the apical plasma membrane.

Published
2000
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42. Immunolocalization of electroneutral Na-HCO(3)(-) cotransporter in rat kidney.

Author

Vorum H, Kwon TH, Fulton C, Simonsen B, Choi I, Boron W, Maunsbach AB, Nielsen S, and Aalkjaer C

Subjects
4,4'-Diisothiocyanostilbene-2,2'-Disulfonic Acid pharmacology, Animals, Antibody Specificity, Bicarbonates metabolism, Cell Membrane chemistry, Cell Membrane ultrastructure, Glycosylation, Hydrogen-Ion Concentration, Immunoblotting, Immunohistochemistry, Ion Transport drug effects, Kidney ultrastructure, Male, Microscopy, Immunoelectron, Rats, Rats, Wistar, Sodium-Bicarbonate Symporters, Subcellular Fractions metabolism, Subcellular Fractions ultrastructure, Carrier Proteins metabolism, Kidney metabolism
Abstract

An electroneutral Na-HCO(3)(-) cotransporter (NBC(N)1) was recently cloned, and Northern blot analyses indicated its expression in rat kidney. In this study, we determined the cellular and subcellular localization of NBC(N)1 in the rat kidney at the light and electron microscopic level. A peptide-derived antibody was raised against the COOH-terminal amino acids of NBC(N)1. The affinity-purified antibody specifically recognized one band, approximately 180 kDa, in rat kidney membranes. Peptide-N-glycosidase F deglycosylation reduced the band to approximately 140 kDa. Immunoblotting of membrane fractions from different kidney regions demonstrated strong signals in the inner stripe of the outer medulla (ISOM), weaker signals in the outer stripe of the outer medulla and inner medulla, and no labeling in cortex. Immunocytochemistry demonstrated that NBC(N)1 immunolabeling was exclusively observed in the basolateral domains of thick ascending limb (TAL) cells in the outer medulla (strongest in ISOM) but not in the cortex. In addition, collecting duct intercalated cells in the ISOM and in the inner medulla also exhibited NBC(N)1 immunolabeling. Immunoelectron microscopy demonstrated that NBC(N)1 labeling was confined to the basolateral plasma membranes of TAL and collecting duct type A intercalated cells. Immunolabeling controls were negative. By using 2, 7-bis-carboxyethyl-5,6-caboxyfluorescein, intracellular pH transients were measured in kidney slices from ISOM and from mid-inner medulla. The results revealed DIDS-sensitive, Na- and HCO(3)(-)-dependent net acid extrusion only in the ISOM but not in mid-inner medulla, which is consistent with the immunolocalization of NBC(N)1. The localization of NBC(N)1 in medullary TAL cells and medullary collecting duct intercalated cells suggests that NBC(N)1 may be important for electroneutral basolateral HCO(3)(-) transport in these cells.

Published
2000
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43. Protonation-dependent inactivation of Na,K-ATPase by hydrostatic pressure developed at high-speed centrifugation.

Author

Esmann M, Fedosova NU, and Maunsbach AB

Subjects
Animals, Calcium-Transporting ATPases chemistry, Dogfish, Enzyme Activation, Enzyme Stability, Glycerol, H(+)-K(+)-Exchanging ATPase chemistry, Hydrogen-Ion Concentration, Kidney enzymology, Potassium Chloride, Protein Conformation, Salt Gland enzymology, Sodium Chloride, Sodium-Potassium-Exchanging ATPase isolation & purification, Sucrose, Swine, Time Factors, Ultracentrifugation, Hydrostatic Pressure, Protons, Sodium-Potassium-Exchanging ATPase chemistry
Abstract

Irreversible inactivation of membranous Na,K-ATPase by high-speed centrifugation in dilute aqueous solutions depends markedly on the protonation state of the protein. Pig kidney Na,K-ATPase is irreversibly inactivated at pH 5 but is fully protected at pH 7 and above. Shark rectal gland Na,K-ATPase is irreversibly inactivated at neutral or acidic pH and partially protected at an alkaline pH. The overall Na,K-ATPase activity and the K-dependent pNPPase activity were denatured in parallel. Cryoprotectants such as glycerol or sucrose at concentrations of 25-30% fully protect both enzymes against inactivation. The specific ligands NaCl and KCl protect the Na,K-ATPase activity partially and the pNPPase activity fully at concentrations of 0.2-0.3 M. Electron microscope analysis of the centrifuged Na,K-ATPase membranes revealed that the ultrastructure of the native membranes is preserved upon inactivation. It was also observed that the sarcoplasmic reticulum Ca-ATPase and hog gastric H, K-ATPase are susceptible to inactivation by high-speed centrifugation in a pH-dependent fashion. H,K-ATPase is protected at alkaline pH, whereas Ca-ATPase is protected only in the neutral pH range.

Published
2000
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44. Altered expression of renal AQPs and Na(+) transporters in rats with lithium-induced NDI.

Author

Kwon TH, Laursen UH, Marples D, Maunsbach AB, Knepper MA, Frokiaer J, and Nielsen S

Subjects
Animals, Aquaporin 1, Aquaporin 2, Aquaporin 3, Aquaporin 6, Aquaporins metabolism, Blotting, Western, Carrier Proteins metabolism, Diabetes Insipidus chemically induced, Diabetic Nephropathies chemically induced, Diuresis physiology, Kidney drug effects, Kidney metabolism, Kidney Concentrating Ability drug effects, Kidney Concentrating Ability physiology, Kidney Medulla metabolism, Kidney Medulla ultrastructure, Kidney Tubules, Collecting metabolism, Kidney Tubules, Collecting ultrastructure, Male, Microscopy, Immunoelectron, Rats, Rats, Wistar, Receptors, Drug biosynthesis, Receptors, Drug metabolism, Sodium metabolism, Sodium Chloride Symporters, Sodium-Hydrogen Exchanger 3, Sodium-Hydrogen Exchangers biosynthesis, Sodium-Hydrogen Exchangers metabolism, Sodium-Phosphate Cotransporter Proteins, Sodium-Phosphate Cotransporter Proteins, Type I, Sodium-Phosphate Cotransporter Proteins, Type II, Sodium-Potassium-Chloride Symporters, Sodium-Potassium-Exchanging ATPase biosynthesis, Sodium-Potassium-Exchanging ATPase metabolism, Solute Carrier Family 12, Member 3, Water metabolism, Aquaporins biosynthesis, Carrier Proteins biosynthesis, Diabetes Insipidus metabolism, Diabetic Nephropathies metabolism, Lithium adverse effects, Symporters
Abstract

Lithium (Li) treatment is often associated with nephrogenic diabetes insipidus (NDI). The changes in whole kidney expression of aquaporin-1 (AQP1), -2, and -3 as well as Na-K-ATPase, type 3 Na/H exchanger (NHE3), type 2 Na-Pi cotransporter (NaPi-2), type 1 bumetanide-sensitive Na-K-2Cl cotransporter (BSC-1), and thiazide-sensitive Na-Cl cotransporter (TSC) were examined in rats treated with Li orally for 4 wk: protocol 1, high doses of Li (high Na(+) intake), and protocol 2, low doses of Li (identical food and normal Na(+) intake in Li-treated and control rats). Both protocols resulted in severe polyuria. Semiquantitative immunoblotting revealed that whole kidney abundance of AQP2 was dramatically reduced to 6% (protocol 1) and 27% (protocol 2) of control levels. In contrast, the abundance of AQP1 was not decreased. Immunoelectron microscopy confirmed the dramatic downregulation of AQP2 and AQP3, whereas AQP4 labeling was not reduced. Li-treated rats had a marked increase in urinary Na(+) excretion in both protocols. However, the expression of several major Na(+) transporters in the proximal tubule, loop of Henle, and distal convoluted tubule was unchanged in protocol 2, whereas in protocol 1 significantly increased NHE3 and BSC-1 expression or reduced NaPi-2 expression was associated with chronic Li treatment. In conclusion, severe downregulation of AQP2 and AQP3 appears to be important for the development of Li-induced polyuria. In contrast, the increased or unchanged expression of NHE3, BSC-1, Na-K-ATPase, and TSC indicates that these Na(+) transporters do not participate in the development of Li-induced polyuria.

Published
2000
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45. Altered expression of Na transporters NHE-3, NaPi-II, Na-K-ATPase, BSC-1, and TSC in CRF rat kidneys.

Author

Kwon TH, Frøkiaer J, Fernández-Llama P, Maunsbach AB, Knepper MA, and Nielsen S

Subjects
Animals, Diuresis, Kidney Concentrating Ability, Kidney Failure, Chronic physiopathology, Mucoproteins metabolism, Natriuresis, Nephrectomy methods, Rats, Rats, Inbred Strains, Receptors, Drug metabolism, Sodium Chloride Symporters, Sodium-Hydrogen Exchanger 3, Sodium-Hydrogen Exchangers metabolism, Sodium-Phosphate Cotransporter Proteins, Sodium-Potassium-Chloride Symporters, Sodium-Potassium-Exchanging ATPase metabolism, Solute Carrier Family 12, Member 3, Uromodulin, Carrier Proteins metabolism, Kidney metabolism, Kidney Failure, Chronic metabolism, Sodium metabolism, Symporters
Abstract

In chronic renal failure (CRF), reduction in renal mass leads to an increase in the filtration rates of the remaining nephrons and increased excretion of sodium per nephron. To address the mechanisms involved in the increased sodium excretion, we determined the total kidney levels and the densities per nephron of the major renal NaCl transporters in rats with experimental CRF. Two weeks after 5/6 nephrectomy (reducing the total number of nephrons to approximately 24 +/- 8%), the rats were azotemic and displayed increased Na excretion. Semiquantitative immunoblotting revealed significant reduction in the total kidney levels of the proximal tubule Na transporters NHE-3 (48% of control), NaPi-II (13%), and Na-K-ATPase (30%). However, the densities per nephron of NHE-3, NaPi-II, and Na-K-ATPase were not significantly altered in remnant kidneys, despite the extensive hypertrophy of remaining nephrons. Immunocytochemistry confirmed the reduction in NHE-3 and Na-K-ATPase labeling densities in the proximal tubule. In contrast, there was no significant reduction in the total kidney levels of the thick ascending limb and distal convoluted tubule NaCl transporters BSC-1 and TSC, respectively. This corresponded to a 3.6 and 2.5-fold increase in densities per nephron, respectively (confirmed by immunocytochemistry). In conclusion, in this rat CRF model: 1) increased fractional sodium excretion is associated with altered expression of proximal tubule Na transporter expression (NHE-3, NaPi-II, and Na-K-ATPase), consistent with glomerulotubular imbalance in the face of increased single-nephron glomerular filtration rate; and 2) compensatory increases in BSC-1 and TSC expression per nephron occur in distal segments.

Published
1999
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46. Ultrastructural localization of Na-K-2Cl cotransporter in thick ascending limb and macula densa of rat kidney.

Author

Nielsen S, Maunsbach AB, Ecelbarger CA, and Knepper MA

Subjects
Animals, Carrier Proteins drug effects, Carrier Proteins ultrastructure, Immunoblotting, Immunohistochemistry, Kidney Tubules, Distal cytology, Kidney Tubules, Distal ultrastructure, Loop of Henle ultrastructure, Microscopy, Immunoelectron, Rats, Sodium-Potassium-Chloride Symporters, Tissue Distribution, Carrier Proteins metabolism, Kidney Tubules, Distal metabolism, Loop of Henle metabolism
Abstract

A bumetanide-sensitive Na-K-2Cl cotransporter, BSC-1, is believed to mediate the apical component of transcellular NaCl absorption in the thick ascending limb (TAL) of Henle's loop. To study its ultrastructural localization in kidney, we used an affinity-purified, peptide-derived polyclonal antibody against rat BSC-1. Immunoblots from rat kidney cortex and outer medulla revealed a solitary 161-kDa band in membrane fractions. Immunocytochemistry of 1-micrometer cryosections demonstrated strong BSC-1 labeling of the apical and subapical regions of medullary and cortical TAL cells. Notably, macula densa cells also exhibited distinct labeling. Distal convoluted tubules and other renal tubule segments were unlabeled. Immunoelectron microscopy demonstrated that BSC-1 labeling was associated with the apical plasma membrane and with subapical intracellular vesicles in medullary and cortical TAL and in macula densa cells. Smooth-surfaced TAL cells, in particular, had extensive BSC-1 labeling of intracellular vesicles. These results support the view that BSC-1 provides the apical pathway for NaCl transport across the TAL and that an extensive intracellular reservoir of BSC-1 is present in a subpopulation of TAL cells. Furthermore, the BSC-1 localization in the apical plasma membrane of macula densa cells is consistent with its proposed role in tubuloglomerular feedback.

Published
1998
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47. Biochemical and ultrastructural characterization of fluid transporting LLC-PK1 microspheres.

Author

Andersen KJ, Maunsbach AB, and Christensen EI

Subjects
Animals, Biological Transport drug effects, Biological Transport physiology, Cell Division drug effects, Cell Division physiology, Cell Membrane ultrastructure, Endocytosis, Epithelial Cells, Ferritins pharmacokinetics, Humans, Immunohistochemistry, Kidney Tubules, Proximal drug effects, LLC-PK1 Cells, Lysosomes enzymology, Mercuric Chloride pharmacology, Microscopy, Electron, Microspheres, Microvilli metabolism, Organelles ultrastructure, Ouabain pharmacology, Renal Agents pharmacology, Spheroids, Cellular drug effects, Spheroids, Cellular metabolism, Swine, Vasopressins pharmacology, Body Fluids metabolism, Kidney Tubules, Proximal metabolism, Kidney Tubules, Proximal ultrastructure, Spheroids, Cellular ultrastructure
Abstract

The established renal epithelial cell line LLC-PK1 (proximal tubule) started to form multicellular spheroids within 24 h when grown in agar overlay culture. The spheroids, average diameter 100 to 350 microns, were free-floating with a butterfly-like structure due to the formation of several hollow microspheres. The microspheres were lined with polarized epithelial cells that had an abundance of microvilli protruding into the external medium and a well developed vacuolar apparatus, including coated pits, endocytotic vacuoles, and lysosomes. The microspheres were sealed between lumen and the surrounding medium by tight junctions and fluctuated in size due to fluid being transported in an apical-to-basal direction. Vasopressin was found to stimulate this transport, whereas the addition of ouabain or HgCl2 inhibited both spheroid growth and fluctuation in size with time. Biochemical assays of brush-border and lysosomal marker enzymes demonstrated an increase in enzyme activity during spheroid formation and growth. The most dramatic changes were observed for dipeptidyl peptidase IV (two- to threefold after 1 d and 53.5-fold after 15 d), reflecting the cellular polarization and brush-border formation during spheroid formation. When the typical lysosomal enzymes were compared, the activity of peptide bond splitting enzymes increased earlier than others. In conclusion, LLC-PK1 spheroids capable of forming microspheres represent an in vitro manifestation of specialized epithelial properties maintained in cell culture, thus providing a tool for studying renal physiologic mechanisms at a cellular level.

Published
1998
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48. Ultrastructure of the vacuolar apparatus in the renal proximal tubule microinfused in vivo with the cytological stain light green.

Author

Cui S, Mata L, Maunsbach AB, and Christensen EI

Subjects
Animals, Endocytosis physiology, Kidney Tubules, Proximal physiology, Male, Methyl Green, Rats, Rats, Wistar, Rosaniline Dyes, Kidney Tubules, Proximal ultrastructure, Vacuoles ultrastructure
Abstract

To obtain insight into the basic mechanisms controlling endocytosis, we tested the effects of different perfusates containing the cytological stain light green on endocytosis and ultrastructure of the vacuolar apparatus in renal proximal tubule cells. Rat proximal tubules were microinfused in vivo for 2 min in the presence or absence of light green with the following solutions: (A) perfusates containing inorganic salts and (B) perfusates with organic components or protein. In other experiments, the tubules were first microinfused for 2 min with 0.9% NaCl in the presence or absence of light green, then 15 min later further microinfused with or without light green using either group A or B solutions in order to either aggravate or reverse possible changes. All infused tubules were fixed after 5 min with 1% glutaraldehyde and examined by electron microscopy. In tubules microinfused without light green, the endocytic vacuolar apparatus in the apical cytoplasm showed a normal ultrastructure. However, microinfusion of solutions containing light green in either inorganic salts or a low concentration of protein caused significant changes in the apical endocytic apparatus. Large endocytic vacuoles were absent, and invaginations and small endocytic vacuoles were decreased in frequency. On the other hand, the amount of dense apical tubules was significantly increased, and in some cells dense apical tubules had transformed into a cisternalike network. These changes were aggravated in tubules which received a second microinfusion of NaCl and reversed in tubules that received a second infusion of protein. Furthermore, in the tubules microinfused with light green using perfusates containing organic components or protein, the apical cytoplasm of proximal tubule cells showed an essentially normal endocytic apparatus. The present study demonstrates that microinfusion of renal proximal tubules with light green disrupted normal endocytic membrane trafficking and recycling. These changes could be prevented or reversed by microinfusion of solutions containing protein or organic components.

Published
1998
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49. Resorption of hydroxyapatite and fluorapatite ceramic coatings on weight-bearing implants: a quantitative and morphological study in dogs.

Author

Overgaard S, Lind M, Josephsen K, Maunsbach AB, Bünger C, and Søballe K

Subjects
Animals, Bone and Bones pathology, Dogs, Osteoclasts pathology, Apatites, Biocompatible Materials, Bioprosthesis, Bone Substitutes, Bone and Bones surgery, Durapatite
Abstract

Resorption (defined as loss of ceramic coating because of cellular activity or dissolution) of ceramic coatings is a matter of concern for the long-term performance of ceramic-coated implants. A new fluorine-containing coating, fluorapatite (FA), has been shown to be more stable than hydroxyapatite (HA) in unloaded models. In a weight-bearing model in trabecular bone, we evaluated loss (defined as reduction of coating irrespective of type of mechanism) of HA and FA coatings during 25 weeks of implantation. Eight mature dogs had HA- or FA-coated implants inserted bilaterally into the weight-bearing region of the medial femoral condyle. Quantified loss of ceramic coating was estimated at the light microscopic level using stereological methods. The experiment showed significant loss of both types of coatings. However, no statistical difference in loss of ceramic coating was found regarding surface area implant coverage, volume, and thickness (p = 0.77, p = 0.13, p = 0.56, p = 0.23, respectively). Completely resorbed HA coating was replaced by 36 +/- 6.0% (range: 26-42) bone in direct contact with the implant surface compared with 29 +/- 16.0% (range: 12-59) for FA (p = 0.40), suggesting that the implant was firmly fixed despite loss of the ceramic coating. Transmission electron microscopy in combination with electron energy spectroscopy and electron spectroscopic imaging showed that osteclast-like cells, osteocytes, macrophage-like cells, and fibroblasts had phagocytosed calcium-containing fragments, indicating cell-mediated resorption of the ceramic coating.

Published
1998
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50. Three-dimensional organization and segmental ultrastructure of rat proximal tubules.

Author

Dørup J and Maunsbach AB

Subjects
Animals, Cell Membrane ultrastructure, Endocytosis, Epithelium ultrastructure, Kidney Cortex anatomy & histology, Kidney Cortex ultrastructure, Kidney Medulla anatomy & histology, Kidney Medulla ultrastructure, Kidney Tubules, Proximal cytology, Male, Microvilli ultrastructure, Mitochondria ultrastructure, Rats, Rats, Sprague-Dawley, Vacuoles ultrastructure, Computer Simulation, Kidney Tubules, Proximal ultrastructure, Models, Structural
Abstract

Aims: To provide a 3-D description and basic morphometric data along the course of subcapsular proximal tubules., Methods: Proximal convoluted (PCT) and straight (PST) tubules were analyzed in series of up to one thousand 4-micron sections of perfusion-fixed rat renal cortex. Nine proximal tubules were traced through the sections by computer-assisted 3-D reconstruction. Selected sections were reembedded and resectioned for ultrastructural morphometry., Results: Subcapsular PCTs (n = 3) had a total length of 12.0 +/- 0.2 mm (SEM), formed tight clusters and contacted the renal surface from 5 to 10 times. In contrast, mid-cortical tubules (total PT length 11.6 +/- 0.1 mm) and in particular deep cortical tubules (total PT length 12.1 +/- 0.9 mm) extended laterally and intermingled considerably with neighboring tubules. Epithelial height gradually decreased from around 11 microns in the PCT to 7.5 microns in the end of the PST. Brush-border height was around 4 microns in the first PT segment (S1), 2.3 microns in the second segment (S2) and 4.5 microns in the end of the proximal tubule. Tubular wall volume, excluding microvilli, decreased from around 1,450 micron3/microns tubule length in early PCT to 825 micron3/microns in terminal PST., Conclusions: The results provide, at precisely defined nephron levels, quantitative ultrastructural data relevant to transport physiology.

Published
1997

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