Your search keyword '"Brunk, U T"' showing total 173 results

51. Sphingosine-induced apoptosis is dependent on lysosomal proteases.

Author

Kågedal K, Zhao M, Svensson I, and Brunk UT

Subjects

Animals, Aspartic Acid Endopeptidases antagonists & inhibitors, Caspases metabolism, Cell Line, Cell Membrane drug effects, Cysteine Proteinase Inhibitors pharmacology, Dose-Response Relationship, Drug, Enzyme Activation drug effects, Humans, Jurkat Cells, Membrane Potentials drug effects, Mice, Mitochondria drug effects, Necrosis, Phosphatidylserines metabolism, Sphingosine administration & dosage, Sphingosine physiology, Apoptosis drug effects, Apoptosis physiology, Endopeptidases physiology, Lysosomes drug effects, Lysosomes enzymology, Sphingosine pharmacology

Abstract

We propose a new mechanism for sphingosine-induced apoptosis, involving relocation of lysosomal hydrolases to the cytosol. Owing to its lysosomotropic properties, sphingosine, which is also a detergent, especially when protonated, accumulates by proton trapping within the acidic vacuolar apparatus, where most of its action as a detergent would be exerted. When sphingosine was added in low-to-moderate concentrations to Jurkat and J774 cells, partial lysosomal rupture occurred dose-dependently, starting within a few minutes. This phenomenon preceded caspase activation, as well as changes of mitochondrial membrane potential. High sphingosine doses rapidly caused extensive lysosomal rupture and ensuing necrosis, without antecedent apoptosis or caspase activation. The sphingosine effect was prevented by pre-treatment with another, non-toxic, lysosomotropic base, ammonium chloride, at 10 mM. The lysosomal protease inhibitors, pepstatin A and epoxysuccinyl-L-leucylamido-3-methyl-butane ethyl ester ('E-64d'), inhibited markedly sphingosine-induced caspase activity to almost the same degree as the general caspase inhibitor benzyloxycarbonyl-Val-Ala-DL-Asp-fluoromethylketone ('Z-VAD-FMK'), although they did not by themselves inhibit caspases. We conclude that cathepsin D and one or more cysteine proteases, such as cathepsins B or L, are important mediators of sphingosine-induced apoptosis, working upstream of the caspase cascade and mitochondrial membrane-potential changes.

Published

2001

52. Apoptosis induced by exposure to a low steady-state concentration of H2O2 is a consequence of lysosomal rupture.

Author

Antunes F, Cadenas E, and Brunk UT

Subjects

Apoptosis physiology, Dose-Response Relationship, Drug, Humans, Hydrogen Peroxide administration & dosage, Jurkat Cells, Lysosomes metabolism, Mitochondria drug effects, Mitochondria metabolism, Models, Biological, Oxidative Stress drug effects, Time Factors, Apoptosis drug effects, Hydrogen Peroxide toxicity, Lysosomes drug effects

Abstract

We have re-examined the lysosomal hypothesis of oxidative-stress-induced apoptosis using a new technique for exposing cells in culture to a low steady-state concentration of H(2)O(2). This steady-state technique mimics the situation in vivo better than the bolus-administration method. A key aspect of H(2)O(2)-induced apoptosis is that the apoptosis is evident only after several hours, although cells may become committed within a few minutes of exposure to this particular reactive oxygen species. In the present work, we were able to show, for the first time, several correlative links between the triggering effect of H(2)O(2) and the later onset of apoptosis: (i) a short (15 min) exposure to H(2)O(2) caused almost immediate, albeit limited, lysosomal rupture; (ii) early lysosomal damage, and later apoptosis, showed a similar dose-related response to H(2)O(2); (iii) both events were inhibited by pre-treatment with iron chelators, including desferrioxamine. This compound is known to be taken up by endocytosis only and thus to become localized in the lysosomal compartment. After exposure to oxidative stress, when cells were again in standard culture conditions, a time-dependent continuous increase in lysosomal rupture was observed, resulting in a considerably lowered number of intact lysosomes in apoptotic cells, whereas non-apoptotic cells from the same batch of oxidative-stress-exposed cells showed mainly intact lysosomes. Taken together, our results reinforce earlier findings and strongly suggest that lysosomal rupture is an early upstream initiating event, and a consequence of intralysosomal iron-catalysed oxidative processes, when apoptosis is induced by oxidative stress.

Published

2001

53. Novel cellular defenses against iron and oxidation: ferritin and autophagocytosis preserve lysosomal stability in airway epithelium.

Author

Persson HL, Nilsson KJ, and Brunk UT

Subjects

Cell Membrane drug effects, Cell Membrane physiology, Cell Membrane ultrastructure, Enzyme-Linked Immunosorbent Assay, Humans, Intracellular Membranes drug effects, Intracellular Membranes physiology, Intracellular Membranes ultrastructure, Lung Neoplasms, Lysosomes drug effects, Lysosomes physiology, Lysosomes ultrastructure, Oxidation-Reduction, Respiratory Mucosa drug effects, Spectrophotometry, Atomic, Tumor Cells, Cultured, Ferritins physiology, Iron metabolism, Iron toxicity, Phagocytosis physiology, Respiratory Mucosa cytology, Respiratory Mucosa physiology

Abstract

Adsorbed to a variety of particles, iron may be carried to the lungs by inhalation thereby contributing to a number of inflammatory lung disorders. Redox-active iron is a potent catalyst of oxidative processes, but intracellularly it is bound primarily to ferritin in a non-reactive form and probably is catalytically active largely within the lysosomal compartment. Damage to the membranes of these organelles causes the release to the cytosol of a host of powerful hydrolytic enzymes, inducing apoptotic or necrotic cell death. The results of this study, using cultured BEAS-2B cells, which are adenovirus transformed human bronchial epithelial cells, and A549 cells, which have characteristics similar to type II alveolar epithelial cells, suggest that the varying abilities of different types of lung cells to resist oxidative stress may be due to differences in intralysosomal iron chelation. Cellular ferritin and iron were assayed by ELISA and atomic absorption, while plasma and lysosomal membrane stability were evaluated by the acridine orange uptake and trypan blue dye exclusion tests, respectively. Normally, and also after exposure to an iron complex, A549 cells contained significantly more ferritin (2.26 +/- 0.60 versus 0.63 +/- 0.33 ng/microg protein, P <0.001) and less iron (0.96 +/- 0.14 versus 1.48 +/- 0.21 ng/microg protein, P <0.05) than did BEAS-2B cells. Probably as a consequence, iron-exposed A549 cells displayed more stable lysosomes (P <0.05) and better survival (P <0.05) following oxidative stress. Following starvation-induced autophagocytosis, which also enhances resistance to oxidant stress, the A549 cells showed a significant reduction in ferritin, and the BEAS-2B cells did not. These results suggest that intralysosomal ferritin enhances lysosomal stability by iron-chelation, preventing Fenton-type chemistry. This notion was further supported by the finding that endocytosis of apoferritin, added to the medium, stabilized lysosomes (P <0.001 versus P <0.01) and increased survival (P <0.01 versus P <0.05) of iron-loaded A549 and BEAS-2B cells. Assuming that primary cell lines of the alveolar and bronchial epithelium behave in a similar manner as these respiratory cell lines, intrabronchial instillation of apoferritin-containing liposomes may in the future be a treatment for iron-dependent airway inflammatory processes.

Published

2001

54. Alpha-lipoic acid and alpha-lipoamide prevent oxidant-induced lysosomal rupture and apoptosis.

Author

Persson HL, Svensson AI, and Brunk UT

Subjects

Animals, Antioxidants pharmacology, Apoptosis physiology, Cells, Cultured, Deferoxamine pharmacology, Iron Chelating Agents pharmacology, Lysosomes metabolism, Oxidants pharmacology, Oxidative Stress drug effects, Apoptosis drug effects, Hydrogen Peroxide metabolism, Lysosomes drug effects, Thioctic Acid analogs & derivatives, Thioctic Acid pharmacology

Abstract

Alpha-lipoic acid (LA) and its corresponding derivative, alpha-lipoamide (LM), have been described as antioxidants, but the mechanisms of their putative antioxidant effects remain largely uncharacterised. The vicinal thiols present in the reduced forms of these compounds suggest that they might possess metal chelating properties. We have shown previously that cell death caused by oxidants may be initiated by lysosomal rupture and that this latter event may involve intralysosomal iron which catalyzes Fenton-type chemistry and resultant peroxidative damage to lysosomal membranes. Here, using cultured J774 cells as a model, we show that both LA and LM stabilize lysosomes against oxidative stress, probably by chelating intralysosomal iron and, consequently, preventing intralysosomal Fenton reactions. In preventing oxidant-mediated apoptosis, LM is significantly more effective than LA, as would be expected from their differing capacities to enter cells and concentrate within the acidic lysosomal compartment. As previously reported, the powerful iron-chelator, desferrioxamine (Des) (which also locates within the lysosomal compartment), also provides protection against oxidant-mediated cell death. Interestingly, although Des enhances the partial protection afforded by LA, it confers no additional protection when added with LM. Therefore, the antioxidant actions of LA and LM may arise from intralysosomal iron chelation, with LM being more effective in this regard.

Published

2001

55. Lysosomal involvement in apoptosis.

Author

Brunk UT, Neuzil J, and Eaton JW

Subjects

Acridine Orange analysis, Amides pharmacology, Animals, Caspases physiology, Cathepsins physiology, Detergents pharmacology, Fluorescent Dyes analysis, Iron analysis, Lysosomes drug effects, Lysosomes enzymology, Oxidation-Reduction, Oxidative Stress, Serine pharmacology, Signal Transduction, Sphingosine pharmacology, Vacuoles physiology, Apoptosis physiology, Lysosomes physiology, Serine analogs & derivatives

Published

2001

56. Vitamin E analogues as inducers of apoptosis: implications for their potential antineoplastic role.

Author

Neuzil J, Weber T, Terman A, Weber C, and Brunk UT

Subjects

Adenocarcinoma drug therapy, Animals, Antineoplastic Agents therapeutic use, Antioxidants therapeutic use, Cell Cycle drug effects, Colonic Neoplasms drug therapy, Drug Screening Assays, Antitumor, Free Radical Scavengers pharmacology, Free Radical Scavengers therapeutic use, Free Radicals, Gene Expression Regulation drug effects, Humans, Intestinal Mucosa drug effects, Intracellular Membranes drug effects, Lysosomes drug effects, Macrophages drug effects, Mice, Mice, Nude, Mitochondria drug effects, Molecular Structure, Neoplastic Stem Cells drug effects, Oxidation-Reduction, Protein Kinase C physiology, Reactive Oxygen Species, Signal Transduction drug effects, Stem Cells drug effects, Tocopherols, Tumor Cells, Cultured drug effects, Vitamin E therapeutic use, Xenograft Model Antitumor Assays, Antineoplastic Agents pharmacology, Antioxidants pharmacology, Apoptosis drug effects, Vitamin E analogs & derivatives, Vitamin E pharmacology

Abstract

Recent evidence suggests that vitamin E and its analogues, which have been used for many years as antioxidants, may not only protect cells from free radical damage but also induce apoptotic cell death in various cell types. While alpha-tocopherol (alpha-TOH) is mainly known as an anti-apoptotic agent, its redox-silent analogues either have no influence on cell survival (alpha-tocopheryl acetate, alpha-TOA), or induce apoptosis (alpha-tocopheryl succinate, alpha-TOS). Although precise mechanisms of apoptosis induction by alpha-TOS remain to be elucidated, there is evidence that this process involves both the antiproliferative and membrane destabilising activities of the agent. Alpha-TOS has been shown to induce apoptosis in malignant cell lines but not, in general, in normal cells, and to inhibit tumorigenesis in vivo. These features suggest that this semi-synthetic analogue of vitamin E could be a promising antineoplastic agent.

Published

2001

57. Lysosomotropic detergents induce time- and dose-dependent apoptosis/necrosis in cultured cells.

Author

Brunk UT

Subjects

Animals, Caspase 3, Caspases metabolism, Cell Line, Humans, Jurkat Cells, Kinetics, Lysosomes drug effects, Mice, Necrosis, U937 Cells, Apoptosis drug effects, Detergents pharmacology, Lysosomes physiology, Sphingosine pharmacology

Published

2000

58. Ceroid/lipofuscin-loaded human fibroblasts show decreased survival time and diminished autophagocytosis during amino acid starvation.

Author

Terman A, Dalen H, and Brunk UT

Subjects

Cell Survival physiology, Cells, Cultured, Fibroblasts metabolism, Fibroblasts ultrastructure, Humans, Microscopy, Confocal, Microscopy, Electron, Reference Values, Time Factors, Amino Acids deficiency, Autophagy physiology, Ceroid metabolism, Fibroblasts physiology, Lipofuscin metabolism

Abstract

To test whether heavy accumulation of ceroid/lipofuscin can disturb important functions of the lysosomal system, AG-1518 human fibroblasts, ceroid/lipofuscin-loaded (following prolonged culture at normobaric hyperoxia) or not, were exposed to amino acid starvation. Ceroid/lipofuscin-loading resulted in decreased cellular survival. Also, there was an inverse relationship between amounts of ceroid/lipofuscin and the survival time of individual cells within the same cultures. Ceroid/lipofuscin-loaded fibroblasts displayed diminished autophagocytotic capacity, as demonstrated by electron microscopy and by treatment of cell cultures with NH4Cl (which inhibits autophagocytotic degradation by increasing intralysosomal pH) for 1 week before ensuing starvation. The latter treatment increased survival of control cells (due to deposition of nondegraded autophagocytosed material before start of starvation), but not that of ceroid/lipofuscin-loaded cells. Moreover, when NH4Cl treatment was combined with starvation, both groups of cells showed approximately the same shortened survival times, testifying to the causal relationship between diminished autophagocytosis and decreased survival of starving ceroid/lipofuscin-loaded cells. We hypothesize that large amounts of undegradable ceroid/lipofuscin within the acidic vacuolar compartment may interfere with lysosomal function, resulting in poor renewal of long-lived proteins and worn-out/damaged organelles, decreased adaptability, and cell death.

Published

1999

59. Beta-cells, oxidative stress, lysosomal stability, and apoptotic/necrotic cell death.

Author

Olejnicka BT, Andersson A, Tyrberg B, Dalen H, and Brunk UT

Subjects

Animals, Autophagy drug effects, Cells, Cultured, Deferoxamine pharmacology, Glucose administration & dosage, Glucose pharmacology, Histocytochemistry, Hydrogen Peroxide pharmacology, Intracellular Membranes drug effects, Islets of Langerhans drug effects, Islets of Langerhans metabolism, Islets of Langerhans ultrastructure, Lysosomes drug effects, Lysosomes ultrastructure, Mice, Mice, Inbred Strains, Microscopy, Electron, Microscopy, Fluorescence, Necrosis, Secretory Vesicles drug effects, Secretory Vesicles metabolism, Apoptosis drug effects, Islets of Langerhans cytology, Lysosomes metabolism, Oxidative Stress drug effects

Abstract

Reactive oxygen intermediates (ROI) may be involved in the destruction of pancreatic beta-cells during the development of insulin-dependent diabetes mellitus (IDDM). To investigate the possible role of lysosomes in this process, normal mouse beta-cells were cultured as monolayers at D-glucose concentrations of 1.6 (pronounced crinophagy), 11 or 28 mM (minimal crinophagy), subjected to a low level of oxidative stress and returned to standard culture conditions. Some cultures were exposed to desferrioxamine (Des) before the oxidative stress. As a result of such stress, many of the cells' lysosomes ruptured with consequent apoptosis or necrosis. Cells kept at 1.6 mM glucose were rich in secretory granules, showed crinophagy/autophagy, were very sensitive to oxidative stress, and had the least stable lysosomes. Cells kept at 28 mM glucose did not show crinophagy, contained fewer secretory granules, were less sensitive to oxidative stress, and had more stable lysosomes. Des-treated cells behaved almost as cells not exposed to oxidative stress at all. The findings suggest that iron may occur together with zinc within the secretory granules and that it sensitizes crinophagic lysosomes to oxidative stress. The stress that was applied in this study may be comparable to what occurs within the vicinity of activated macrophages during autoimmune insulitis.

Published

1999

60. Ceroid/lipofuscin-loaded human fibroblasts show increased susceptibility to oxidative stress.

Author

Terman A, Abrahamsson N, and Brunk UT

Subjects

Acridine Orange metabolism, Cathepsin D metabolism, Cell Compartmentation, Cell Line, Fibroblasts cytology, Fibroblasts drug effects, Fibroblasts metabolism, Humans, Lysosomes metabolism, Lysosomes ultrastructure, Naphthoquinones pharmacology, Oxidants pharmacology, Ceroid metabolism, Lipofuscin metabolism, Oxidative Stress

Abstract

To test whether the possibly enhanced sensitivity of aged cells to oxidative stress may depend on their content of ceroid/lipofuscin, AG-1518 human fibroblasts with various amounts of the pigment accumulated due to prolonged cultivation under normobaric hyperoxia were exposed to acute oxidative stress (2.5 microM naphthazarin, 15 min) and then returned to standard culture conditions. Twenty-four hours after the naphthazarin treatment, 37% of the cells were still vital, whereas others had undergone oxidative stress-induced apoptosis with ensuing postapoptotic necrosis. The average amount of ceroid/lipofuscin within the surviving cells was only about half of that of the initial population of cells, as measured before the naphthazarin exposure. This finding suggests that ceroid/lipofuscin-rich cells have an increased sensitivity to oxidative stress. The ceroid/lipofuscin quantity strongly positively correlated with the size of the acidic compartment (as evaluated by uptake of the weakly basic lysosomotropic fluorochrome acridine orange) and with its content of the lysosomal protease cathepsin D, as assayed by immunocytochemistry. We hypothesize that the enhanced sensitivity of ceroid/lipofuscin-loaded cells to oxidative stress may be caused by the increased amounts of lysosomal enzymes, known as mediators of oxidative damage, and/or by catalysis of intralysosomal oxidative reactions by lipofuscin-associated iron.

Published

1999

61. Is lipofuscin eliminated from cells?

Author

Terman A and Brunk UT

Subjects

Fibroblasts drug effects, Fibroblasts metabolism, Heart drug effects, Humans, Inclusion Bodies metabolism, Leupeptins pharmacology, Myocardium metabolism, Lipofuscin metabolism, Pigment Epithelium of Eye metabolism

Published

1999

62. Minute oxidative stress is sufficient to induce apoptotic death of NIT-1 insulinoma cells.

Author

Olejnicka BT, Dalen H, and Brunk UT

Subjects

Adenosine Triphosphate metabolism, Caspase 3, Caspases metabolism, Cell Line, Transformed, Evaluation Studies as Topic, Humans, Hydrogen Peroxide pharmacology, Insulinoma, Intracellular Fluid metabolism, Intracellular Membranes drug effects, Intracellular Membranes physiology, Jurkat Cells, Lysosomes drug effects, Microscopy, Confocal, Microscopy, Electron, Tumor Cells, Cultured, Apoptosis, Oxidative Stress

Abstract

When cultured NIT-1 cells were subjected to a low level of oxidative stress (30 microM hydrogen peroxide for 15 min at 37 degrees C) several of their lysosomes ruptured, as demonstrated by intravital staining with the lysosomotropic weak base acridine orange. Such rupture is due to intralysosomal, iron-catalyzed oxidative reactions, since it was largely prevented by previous endocytotic uptake of desferrioxamine. The resultant limited leakage of lysosomal hydrolytic enzymes into the cytosol could be important for an apoptotic-type degradation/fragmentation process within initially intact plasma membranes. In contrast, extensive lysosomal rupture leads to necrosis. The development of the damage process was followed by light- and electron microscopy; and by the TUNEL-reaction. As a result of the applied oxidative stress, which is comparable to that expected to occur within the microenvironment surrounding activated macrophages under oxidative burst (e.g. during autoimmune insulitis), about 90% of the cells eventually died due to post-apoptotic secondary necrosis. The few surviving cells phagocytosed the debris from their fragmented neighbours and began to divide about 24 h after the insult. Thus the sensitivity to oxidative stress varies, perhaps as a consequence of varying amounts of intralysosomal redox-active iron, as we have found to be the case in several other cellular systems. Since the NIT-1 cells are highly differentiated, and in many ways like beta cells, we consider our result to be of value for the understanding of beta-cell death during the development of insulin-dependent (Type I) diabetes mellitus (IDDM).

Published

1999

63. alpha-tocopheryl succinate-induced apoptosis in Jurkat T cells involves caspase-3 activation, and both lysosomal and mitochondrial destabilisation.

Author

Neuzil J, Svensson I, Weber T, Weber C, and Brunk UT

Subjects

Caspase 3, Enzyme Activation, Humans, Jurkat Cells, Lysosomes, Mitochondria physiology, Tocopherols, Vitamin E metabolism, Vitamin E pharmacology, Apoptosis drug effects, Caspases metabolism, Vitamin E analogs & derivatives

Abstract

Alpha-Tocopheryl succinate (alpha-TOS), but not a-tocopherol, triggered apoptosis in Jurkat T cells. Apoptosis was induced by alpha-TOS in a time- and concentration-dependent mode, and signs of apoptosis were visible at concentrations of alpha-TOS as low as 30 microM, and within 3-5 h after addition of the ester. Employing a specific fluorogenic substrate, caspase-3 was found to be activated rapidly in response to alpha-TOS at 50 microM. We also found that Jurkat T cells challenged with alpha-TOS, when exposed to the lysosomotropic weak base acridine orange, showed decreased lysosomal uptake of the dye. This is suggestive of the involvement of lysosomal destabilisation in apoptosis of the cells. Apoptosis of Jurkat T cells induced with alpha-TOS also involved a drop in the mitochondrial membrane potential, although this phenomenon occurred after the initiation of lysosomal rupture. All apoptotic features observed with alpha-TOS were very similar to those found when cross-linking of the Fas receptor triggered apoptosis. These findings are consistent with the recent idea that vitamin E can contribute to elimination of malignant cells by the induction of apoptosis, and can be of (patho)physiological significance.

Published

1999

64. Oxidative stress, growth factor starvation and Fas activation may all cause apoptosis through lysosomal leak.

Author

Brunk UT and Svensson I

Subjects

DNA Fragmentation, Enzyme-Linked Immunosorbent Assay, Humans, Jurkat Cells, Apoptosis, Growth Substances physiology, Lysosomes metabolism, Oxidative Stress, fas Receptor physiology

Abstract

Oxidative stress, growth factor starvation, and activation of the Fas/APO-1/CD95 receptor all induce apoptosis in a variety of cell-types, including the established human Jurkat T-cell line. Oxidative stress, in the form of exposure of the cells to a bolus dose of hydrogen peroxide, results in intralysosomal, iron-catalyzed oxidative reactions. This is accompanied by a time- and dose-dependent lysosomal destabilization--as evaluated by a decreased lysosomal uptake of the metachromatic fluorochrome, and weak base, acridine orange--in combination with leakage to the cytosol of lysosomal contents, including hydrolytic enzymes. Moderate lysosomal rupture is followed by apoptosis within initially intact plasma membranes, while necrosis and cell lysis are associated with a more complete lysosomal breach. Prior endocytosis of the potent iron-chelator desferrioxamine, resulting in binding of intralysosomal low molecular weight iron in a non-redox active form, largely prevents not only oxidative stress-induced lysosomal labilization, but apoptosis as well. When apoptosis is induced by the use of a monoclonal IgM anti-human Fas/APO-1/CD95 receptor antibody, the apoptotic process is again found to be accompanied by lysosomal leak. It is, however, not prevented by a preceding endocytosis of desferrioxamine and, consequently, could not be a function of intralysosomal iron-catalyzed oxidative reactions, but must be due to other mechanisms. Growth factor starvation of Jurkat cultures for a few days results in a high proportion of apoptotic cells, which contain lysosomes many of which have lost their proton gradient and appear to have released their contents. Overall, our results indicate that lysosomal leakage/rupture precedes apoptosis in Jurkat cells regardless of the initiating agent, but that such rupture may occur through multiple mechanisms. Lysosomal enzymes, leaking out of their normal vacuolar compartment, may then induce apoptosis, perhaps by proteolytic activation of the caspase-family of enzymes. Regardless of the precise mechanism, these observations suggest that partial rupture of the acidic vacuolar compartment may be one of the final pathways in apoptosis.

Published

1999

65. Redox availability of lens iron and copper: implications for HO* generation in cataract.

Author

Garner B, Roberg K, Qian M, Brunk UT, Eaton JW, and Truscott RJ

Subjects

Humans, Oxidation-Reduction, Cataract metabolism, Copper metabolism, Hydroxyl Radical metabolism, Iron metabolism, Lens, Crystalline metabolism

Published

1999

66. OxLDL-induced macrophage cytotoxicity is mediated by lysosomal rupture and modified by intralysosomal redox-active iron.

Author

Li W, Yuan XM, and Brunk UT

Subjects

Animals, Cell Division drug effects, Cell Line, Cell Survival drug effects, DNA Fragmentation, Deferoxamine pharmacology, Iron Chelating Agents pharmacology, Mice, Oxidation-Reduction, Apoptosis drug effects, Iron pharmacology, Lipoproteins, LDL pharmacology, Lysosomes drug effects, Macrophages drug effects, Macrophages ultrastructure

Abstract

Oxidized low density lipoprotein (oxLDL) is believed to play a central role in atherogenesis. LDL is oxidized in the arterial intima by mechanisms that are still only partially understood. OxLDL is then taken up by macrophages through scavenger receptor-mediated endocytosis, which then leads to cellular damage, including apoptosis. The complex mechanisms by which oxLDL induces cell injury are mostly unknown. This study has demonstrated that oxLDL-induced damage of macrophages is associated with iron-mediated intralysosomal oxidative reactions, which cause partial lysosomal rupture and ensuing apoptosis. This series of events can be prevented by pre-exposing cells to the iron-chelator, desferrioxamine (DFO), whereas it is augmented by pretreating the cells with a low molecular weight iron complex. Since both DFO and the iron complex would be taken up by endocytosis, and thus directed to the lysosomal compartment, the results suggest that the normal contents of lysosomal low molecular weight iron may play an important role in oxLDL-induced cell damage, presumably by catalyzing intralysosomal fragmentation of lipid peroxides and the formation of toxic aldehydes and oxygen-centered radicals.

Published

1998

67. Congenital disorders sharing oxidative stress and cancer proneness as phenotypic hallmarks: prospects for joint research in pharmacology.

Author

Pagano G, Korkina LG, Brunk UT, Chessa L, Degan P, del Principe D, Kelly FJ, Malorni W, Pallardó F, Pasquier C, Scovassi I, Zatterale A, and Franceschi C

Subjects

Aging, Animals, Apoptosis, Humans, Neoplasms genetics, Phenotype, Disease Susceptibility, Genetic Diseases, Inborn genetics, Neoplasms etiology, Oxidative Stress genetics

Abstract

In spite of very distinct genotypic assets, a number of congenital conditions include oxidative stress as a phenotypic hallmark. These disorders include Fanconi's anaemia, ataxia telangiectasia, xeroderma pigmentosum and Bloom's syndrome, as well as two frequent congenital conditions: Down's syndrome and cystic fibrosis. Cancer proneness is a clinical feature shared by these disorders, while other manifestations include early ageing, neurological symptoms or congenital malformations. The onset of oxidative stress has been related to excess formation, or defective detoxification, of reactive oxygen species (ROS). This can arise from either the abnormal expression or inducibility of ROS-detoxifying enzymes, or by defective absorption of nutrient antioxidants. Resulting oxidative injury has been characterized through: (i) DNA, protein or lipid oxidative damage; (ii) excess ROS formation (in vitro and ex vivo); (iii) sensitivity to oxygen-related toxicity; (iv) improvement of cellular defects by either hypoxia or antioxidants; and (v) circumstantial evidence for in vivo oxidative stress (as e.g. clastogenic factors). Investigations conducted so far have been confined to individual disorders. Comparative studies of selected indicators for oxidative stress could provide further insights into the pathogenesis of each individual condition. Such a unified approach may have wide-ranging consequences for studies of ageing and cancer.

Published

1998

68. Lipofuscin accumulation in cultured retinal pigment epithelial cells reduces their phagocytic capacity.

Author

Sundelin S, Wihlmark U, Nilsson SE, and Brunk UT

Subjects

Animals, Animals, Newborn, Cattle, Cells, Cultured, Fluorescent Dyes, Microscopy, Confocal, Microspheres, Pigment Epithelium of Eye cytology, Pigment Epithelium of Eye ultrastructure, Rabbits, Rod Cell Outer Segment physiology, Xanthenes, Lipofuscin metabolism, Phagocytosis physiology, Pigment Epithelium of Eye physiology

Abstract

Purpose: Retinal pigment epithelial (RPE) cells slowly accumulate lipofuscin pigment within their acidic vacuolar apparatus as a result of extra- and/or intralysosomal oxidative alterations of phagocytosed photoreceptor outer segments (POS) with consequent imperfect degradation of these structures. In old age, lipofuscin accumulation may become quite substantial. It has been suggested that pronounced accumulation of lipofuscin is related to decreased RPE function and, possibly, to age-related macular degeneration. The aim of the present investigation was to study whether heavy loading with lipofuscin of RPE acidic lysosomes would affect the further phagocytic ability of the cells., Methods: In the first section of the investigation, cultures of rabbit RPE cells were exposed daily to bovine UV-irradiated POS (artificial lipofuscin) for 4 weeks, resulting in a pronounced lipofuscin accumulation of the cells. Fluorescent latex beads (labelled with a red fluorophore) were added to unloaded control cultures at O and 4 weeks after their establishment, and to lipofuscin loaded cells after 4 weeks of feeding with artificial lipofuscin. Cellular amounts of lipofuscin, and their phagocytotic activity, were quantified by static fluorometry measuring lipofuscin-specific and red bead-specific fluorescence, respectively. The intracellular location of the beads was verified by confocal laser scanning microscopy., Results: Unloaded, and thus almost lipofuscin-free, control cells exposed to latex beads showed numerous cytoplasmic particles emitting reddish fluorescence, while few particles were taken up by cells initially loaded with artificial, POS-derived, lipofuscin. Measurement of the latex bead-specific fluorescence showed significantly (p < 0.001) higher levels in unloaded control cells than in lipofuscin-loaded ones. In the second part of the investigation, unloaded control cultures and lipofuscin-loaded cultures were exposed to native bovine Texas Red-X-labelled POS 4 weeks after the establishment of the cultures. Unloaded control cells showed a large number of cytoplasmic POS emitting reddish fluorescence, while fewer POS were phagocytosed by cells loaded with artificial lipofuscin. Measurement of the Texas Red-X-specific fluorescence, thus quantifying the phagocytic ability of the cells, showed significantly (p < 0.001) higher levels in control cells than in lipofuscin-loaded ones., Conclusions: Severe lipofuscin accumulation of RPE cells appears to result in a greatly decreased phagocytic capacity. The resulting reduction in ability to cope with the needs of the overlying photoreceptor cells, in order to eliminate the obsolete tips of their POS, may well be of significance in the development of age-related macular degeneration.

Published

1998

69. Endogenous ferritin protects cells with iron-laden lysosomes against oxidative stress.

Author

Garner B, Roberg K, and Brunk UT

Subjects

Animals, Cell Survival, Fluorescent Antibody Technique, Histocytochemistry, Hydrogen Peroxide metabolism, Hydrogen Peroxide pharmacology, Intracellular Membranes drug effects, Intracellular Membranes ultrastructure, Lymphoma, Large B-Cell, Diffuse, Lysosomes ultrastructure, Macrophages ultrastructure, Mice, Microscopy, Electron, Oxidation-Reduction, Tumor Cells, Cultured, Ferritins metabolism, Iron metabolism, Lysosomes metabolism, Macrophages metabolism, Oxidative Stress

Abstract

Previous studies have shown that a variety of mammalian cell types, including macrophages, contain small amounts of redox-active iron in their lysosomes. Increases in the level of this iron pool predispose the cell to oxidative stress. Limiting the availability of intralysosomal redox-active iron could therefore represent potential cytoprotection for cells under oxidative stress. In the present study we have shown that an initial 6 h exposure of J774 macrophages to 30 microM iron, added to the culture medium as FeCl3, increased the lysosomal iron content and their sensitivity to H2O2-induced (0.25 mM for 30 min) oxidative stress. Over time (24-72 h), however, the cells were desensitized to the cytotoxic effects of H2O2; most likely as a consequence of both lysosomal iron exocytosis and of ferritin synthesis (demonstrated by atomic absorption spectrophotometry, autometallography, and immunohistochemistry). When the cells were exposed to a second dose of iron, their lysosomal content of iron increased again but the cells became no further sensitized to the cytotoxic effects of H2O2. Using the lysosomotropic weak base, acridine orange, we demonstrated that after the second exposure to iron and H2O2, lysosomes remained intact and were no different from control cells which were exposed to H2O2 but not iron. These data suggest that the initial induction of ferritin synthesis leads to enrichment of lysosomes with ferritin via autophagocytosis. This limits the redox-availability of intralysosomal iron and, in turn, decreases the cells' sensitivity to oxidative stress. These in vitro observations could also explain why cells under pathological conditions, such as haemochromatosis, are apparently able to withstand high iron concentrations for some time in vivo.

Published

1998

70. Uptake of oxidized LDL by macrophages results in partial lysosomal enzyme inactivation and relocation.

Author

Li W, Yuan XM, Olsson AG, and Brunk UT

Subjects

Acridine Orange, Animals, Biological Transport physiology, Cell Line, Electrophoresis, Agar Gel, Enzyme Activation physiology, Enzymes metabolism, Humans, Lipoproteins, HDL pharmacology, Lipoproteins, LDL antagonists & inhibitors, Lipoproteins, LDL pharmacology, Lysosomes drug effects, Mice, Tissue Distribution, Vitamin E pharmacology, Lipoproteins, LDL pharmacokinetics, Lysosomes enzymology, Macrophages metabolism

Abstract

The cytotoxicity of oxidized LDL (oxLDL) to several types of artery wall cells might contribute to atherosclerosis by causing cell death, presumably by both apoptosis and necrosis. After its uptake into macrophage lysosomes by receptor-mediated endocytosis, oxLDL is poorly degraded, resulting in ceroid-containing foam cells. We studied the influence ofoxLDL on lysosomal enzyme activity and, in particular, on lysosomal membrane stability and the modulation of these cellular characteristics by HDL and vitamin E (vit-E). Unexposed cells and cells exposed to acetylated LDL (AcLDL) were used as controls. The lysosomal marker enzymes cathepsin L and N-acetyl-beta-glucosaminidase (NAbetaGase) were biochemically assayed in J-774 cells after fractionation. Lysosomal integrity in living cells was assayed by the acridine orange (AO) relocation test. Cathepsin D was immunocytochemically demonstrated in J-774 cells and human monocyte-derived macrophages. We found that the total activities of NAbetaGase and cathepsin L were significantly decreased, whereas their relative cytosolic activities were enhanced, after oxLDL exposure. Labilization of the lysosomal membranes was further proven by decreased lysosomal AO uptake and relocation to the cytosol of cathepsin D, as estimated by light and electron microscopic immunocytochemistry. HDL and vit-E diminished the cytotoxicity of oxLDL by decreasing the lysosomal damage. The results indicate that endocytosed oxLDL not only partially inactivates lysosomal enzymes but also destabilizes the acidic vacuolar compartment, causing relocation of lysosomal enzymes to the cytosol. Exposure to AcLDL resulted in its uptake with enlargement of the lysosomal apparatus, but the stability of the lysosomal membranes was not changed.

Published

1998

71. Lipofuscin: mechanisms of formation and increase with age.

Author

Terman A and Brunk UT

Subjects

Animals, Humans, Lysosomes metabolism, Lysosomes physiology, Models, Biological, Aging metabolism, Aging physiology, Lipofuscin metabolism, Lipofuscin physiology

Abstract

Lipofuscin (age pigment) is a brown-yellow, electron-dense, autofluorescent material that accumulates progressively over time in lysosomes of postmitotic cells, such as neurons and cardiac myocytes. The exact mechanisms behind this accumulation are still unclear. This review outlines the present knowledge of age pigment formation, and considers possible mechanisms responsible for the increase of lipofuscin with age. Numerous studies indicate that the formation of lipofuscin is due to the oxidative alteration of macromolecules by oxygen-derived free radicals generated in reactions catalyzed by redox-active iron of low molecular weight. Two principal explanations for the increase of lipofuscin with age have been suggested. The first one is based on the notion that lipofuscin is not totally eliminated (either by degradation or exocytosis) even at young age, and, thus, accumulates in postmitotic cells as a function of time. Since oxidative reactions are obligatory for life, they would act as age-independent enhancers of lipofuscin accumulation, as well as of many other manifestations of senescence. The second explanation is that the increase of lipofuscin is an effect of aging, caused by an age-related enhancement of autophagocytosis, a decline in intralysosomal degradation, and/or a decrease in exocytosis.

Published

1998

72. On the cytoprotective role of ferritin in macrophages and its ability to enhance lysosomal stability.

Author

Garner B, Li W, Roberg K, and Brunk UT

Subjects

Animals, Apoferritins pharmacology, Cell Differentiation, Cell Line, Cells, Cultured, Deferoxamine pharmacology, Ferritins analysis, Humans, Hydrogen Peroxide toxicity, Intracellular Membranes drug effects, Lysosomes drug effects, Macrophages cytology, Macrophages drug effects, Mice, Monocytes cytology, Monocytes drug effects, Monocytes metabolism, Ferritins physiology, Lysosomes metabolism, Macrophages metabolism

Abstract

Macrophages have a great capacity to take up (e.g. by endocytosis and phagocytosis) exogenous sources of iron which could potentially become cytotoxic, particularly following the intralysosomal formation of low-molecular weight, redox active iron, and under conditions of oxidative stress. Following autophagocytosis of endogenous ferritin/apoferritin, these compounds may serve as chelators of such lysosomal iron and counteract the occurrence of iron-mediated intralysosomal oxidative reactions. Such redox-reactions have been shown to lead to destabilisation of lysosomal membranes and result in leakage of damaging lysosomal contents to the cytosol. In this study we have shown: (i) human monocyte-derived macrophages to accumulate ferritin in response to iron exposure; (ii) iron to destabilise macrophage secondary lysosomes when the cells are exposed to H2O2; and (iii) endocytosed apoferritin to act as a stabiliser of the acidic vacuolar compartment of iron-loaded macrophages. While the endogenous ferritin accumulation which was induced by iron exposure was not sufficient to protect cells from the damaging effects of H2O2, exogenously added apoferritin, as well as the potent iron chelator desferrioxamine, afforded significant protection. It is suggested that intralysosomal formation of haemosiderin, from partially degraded ferritin, is a protective strategy to suppress intralysosomal iron-catalysed redox reactions. However, under conditions of severe macrophage lysosomal iron-overload, induction of ferritin synthesis is not enough to completely prevent the enhanced cytotoxic effects of H2O2.

Published

1997

73. Lysosomal heterogeneity between and within cells with respect to resistance against oxidative stress.

Author

Nilsson E, Ghassemifar R, and Brunk UT

Subjects

Acridine Orange metabolism, Animals, Cell Membrane metabolism, Cells, Cultured, Cricetinae, Fibroblasts, Histocytochemistry, Humans, Hydrogen Peroxide metabolism, Iron analysis, Iron pharmacology, Lysosomes chemistry, Lysosomes ultrastructure, Mice, Oxidation-Reduction, Rats, Tumor Cells, Cultured, Cell Survival, Lysosomes physiology, Oxidative Stress

Abstract

The prevailing opinion on lysosomal endurance is that, as long as the cells are still alive, these organelles are generally quite stable and, thus, do not induce cell damage by leaking their numerous powerful hydrolytic enzymes to the cytosol. We suggest that this opinion is basically wrong and consider that many lysosomes are quite vulnerable, especially to oxidative stress. Moreover, we suggest that cellular degeneration, including apoptosis as well as necrosis, follows upon lysosomal disruption. We have found differing stability of lysosomal membranes to oxidative stress, not only among different cell types, but also between cells of the same type and between lysosomes of individual cells. We suggest that cellular resistance to oxidative stress is mainly a function of three parameters: (i) the capacity to degrade hydrogen peroxide before it reaches, and may diffuse into, the acidic vacuolar compartment; (ii) the resistance to reactive oxygen species of lysosomal membranes; and (iii) the intralysosomal amounts of redox-active, low molecular weight iron. Iron-catalysed intralysosomal reactions, if pronounced enough, result in peroxidation and destabilization of the lysosomal membrane. Owing to differences in the cellular synthesis of hydrogen peroxide-degrading enzymes, degree of autophagocytotic degradation of iron-containing metalloproteins, lysosomal localization within the cytoplasm and intralysosomal iron chelation, the above three parameters may vary between both different and similar cells and between lysosomes of individual cells as well, explaining their observed variability with respect to resistance against oxidative stress.

Published

1997

74. A short exposure to a high-glucose milieu stabilizes the acidic vacuolar apparatus of insulinoma cells in culture to ensuing oxidative stress.

Author

Olejnicka BT, Ollinger K, and Brunk UT

Subjects

Animals, Cell Survival drug effects, Cricetinae, Deferoxamine pharmacology, Hydrogen-Ion Concentration, Insulinoma, Mice, Microscopy, Confocal, Oxidation-Reduction, Time Factors, Tumor Cells, Cultured, Glucose pharmacology, Hydrogen Peroxide toxicity, Islets of Langerhans metabolism, Lysosomes metabolism, Oxidative Stress

Abstract

It was recently suggested that extracellular hydrogen peroxide, after diffusing into and throughout adjacent cells--which may be the case if they have only a weak capacity to degrade hydrogen peroxide--labilizes their lysosomal compartment due to its content of low-molecular-weight iron in redox-active form. The iron would be present as a consequence of normal autophagocytotic degradation of various iron-containing metalloproteins. Beta- and insulinoma cells are especially vulnerable to oxidative stress, since they possess only low capacity to degrade hydrogen peroxide, and, perhaps, since they normally have a certain degree of autophagocytotic degradation of secretory granules with some iron content--crinophagy. The toxicity to beta cells of oxidative stress, such as an exposure to alloxan, that results in extracellular formation of hydrogen peroxide, is considerably reduced if animals are initially given an intravenous bolus dose of glucose, temporarily bringing up the blood level to about 20 mM. In this study it was demonstrated that already as short an exposure as 30 min to 20 mM D-glucose reduces the sensitivity of HIT and NIT insulinoma cells in culture to a subsequent exposure to hydrogen peroxide. In parallel, exposure to such a high-glucose medium also reduces their desferrioxamine-available amount of iron and, moreover, stabilizes their lysosomal membranes against oxidative stress--thus preventing diffusion to the cytosol of damaging lysosomal contents following iron-catalyzed, Fenton-type, intralysosomal reactions. We suggest that both general autophagocytotic turnover and, in particular, crinophagy of secretory granules are decreased by an increased glucose concentration of the surrounding milieu, with attendant reduced amounts of intralysosomal low-molecular-weight iron and, thus, diminished sensitivity to oxidative stress.

Published

1997

75. Photo-oxidative disruption of lysosomal membranes causes apoptosis of cultured human fibroblasts.

Author

Brunk UT, Dalen H, Roberg K, and Hellquist HB

Subjects

Acridine Orange, Cathepsin D analysis, Cathepsin D metabolism, Cell Line, Humans, Male, Microscopy, Electron, Microscopy, Electron, Scanning, Oxidation-Reduction, Apoptosis, Fibroblasts ultrastructure, Intracellular Membranes chemistry, Intracellular Membranes physiology, Light, Lysosomes ultrastructure

Abstract

Acridine orange (AO) is a lysosomotropic weak base, a metachromatic fluorochrome, and a photosensitizer, as well. Living cells that are exposed for a short period of time to this compound at low concentration, and under ordinary culture conditions, accumulate the drug within their acidic vacuolar compartment, giving rise to a mainly red, granular fluoresence upon excitation with blue light. When AO-loaded cells are irradiated with intense blue light, AO soon starts to leak from late endosomes and lysosomes, partially shifting the fluorescence to a green, nuclear and diffuse cytosolic, one. This AO-relocalization is a consequence of photo-oxidation of the lysosomal membranes, which initially results in disruption of their proton-gradients and later, in leakage into the cytosol of a host of hydrolytic enzymes--as was here demonstrated by immunocytochemistry--which are capable of causing cellular damage. Most fibroblasts survived minor photo-oxidation, with a period of reparative autophagocytosis. Severe photo-oxidation, which resulted in severe lysosomal damage, caused cellular necrosis; whereas moderate stress, resulting in only partial lysosomal leakiness lead to apoptosis with TUNEL-positive nuclei and shrunken cytoplasm. The findings of the present study show that photo-oxidative damage to the membranes that surround the acidic vacuolar compartment, is an event that results in release of proteolytic and DNA-fragmenting enzymes into the cytosol, which may induce either necrosis, apoptosis, or reparable sublethal damage, depending on the magnitude of lysosomal rupture. Furthermore, the results strongly suggest that proteases and endonucleases of lysosomal origin may induce apoptosis if relocalized from the acidic vacuolar compartment into the cytosol.

Published

1997

76. Formation of lipofuscin in cultured retinal pigment epithelial cells exposed to pre-oxidized photoreceptor outer segments.

Author

Wihlmark U, Wrigstad A, Roberg K, Brunk UT, and Nilsson SE

Subjects

Animals, Cattle, Cells, Cultured, Eye Enucleation, Female, Male, Pigment Epithelium of Eye drug effects, Pigment Epithelium of Eye ultrastructure, Rabbits, Rod Cell Outer Segment drug effects, Rod Cell Outer Segment radiation effects, Thiobarbiturates, Ultraviolet Rays, Lipofuscin biosynthesis, Peroxides toxicity, Pigment Epithelium of Eye metabolism, Rod Cell Outer Segment physiology

Abstract

Accumulation of lipofuscin in the retinal pigment epithelium (RPE) with increasing age may affect essential supportive functions for the photoreceptors. Earlier, we described a model system for the study of lipofuscinogenesis in RPE cell cultures and showed that mild oxidative stress enhances lipofuscin formation from phagocytized photoreceptor outer segments (POS). In the present study, bovine POS were photo-oxidized, and turned into a lipofuscin-like material, by irradiation with UV light. Transmission electron microscopy of irradiated POS showed loss of the normal stacks of the disk membranes with conversion into an amorphous osmiophilic electron-dense mass. The formation of thiobarbituric acid reactive substances (TBARS), estimated during the irradiation process, indicated lipid peroxidation. Irradiated POS also showed a strong granular yellow autofluorescence. RPE cell cultures, kept at 21% ambient oxygen, were fed daily for 3, 5 or 7 days with either (i) UV-peroxidized POS, (ii) native POS or (iii) culture medium only. RPE cells fed irradiated POS showed significantly higher levels of lipofuscin-specific autofluorescence compared to cells exposed to native POS after 3 days (p = 0.0056), 5 days (p = 0.0037) and 7 days (p = 0.0020), and to the non-exposed control cells (3 days: p = 0.005, 5 days: p = 0.0037, 7 days: p = 0.0094). The lipofuscin content of cells exposed to irradiated POS increased significantly between days 3 and 7 (p = 0.0335). Ultrastructural studies showed much more numerous and larger lipofuscin-like inclusions in RPE cells fed irradiated POS compared to cells exposed to native POS. In the control cells, lipofuscin-like granules were small and sparse. It appears that exposing RPE cells to previously peroxidized POS, thus artificially converted to lipofuscin and obviously not digestible by the lysosomal enzymes, accelerates the formation of severely lipofuscin-loaded cells. The results will be useful for further studies of possible harmful effects of lipofuscin in heavily loaded RPE cells.

Published

1996

77. Lipofuscin formation in cultured retinal pigment epithelial cells exposed to photoreceptor outer segment material under different oxygen concentrations.

Author

Wihlmark U, Wrigstad A, Roberg K, Brunk UT, and Nilsson SE

Subjects

Animals, Cattle, Cells, Cultured, Dose-Response Relationship, Drug, Eye Enucleation, Female, Male, Pigment Epithelium of Eye drug effects, Pigment Epithelium of Eye ultrastructure, Rabbits, Rod Cell Outer Segment chemistry, Rod Cell Outer Segment ultrastructure, Lipofuscin biosynthesis, Oxygen toxicity, Pigment Epithelium of Eye metabolism, Rod Cell Outer Segment physiology

Abstract

Lipofuscin accumulates in the course of time in the acidic vacuolar apparatus of retinal pigment epithelial (RPE) cells and may influence their metabolic functions. In order to study the effect of oxidative stress on lipofuscin accumulation, rabbit RPE cell cultures were kept at an ambient oxygen concentration of either 8% or 40%. To simulate the normal phagocytic function of RPE cells, bovine photoreceptor outer segments (POS) were added daily. The lipofuscin-specific autofluorescence was measured after 1, 2 and 3 weeks. RPE cells cultured under normobaric hyperoxic conditions (40% oxygen) showed significantly higher levels of lipofuscin-like autofluorescence than those kept under normobaric and probably normoxic conditions (8% oxygen) after 1 (p = 0.0050), 2 (p = 0.0001) as well as 3 (p = 0.0077) weeks. At both oxygen concentrations, the lipofuscin accumulation level was increased after 2 weeks of POS exposure (40% p = 0.0001; 8% p = 0.0037) and even further after 3 weeks (40% p = 0.0541; 8% p = 0.0377). The results suggest an involvement of oxidative mechanisms in the formation of lipofuscin from phagocytized POS by RPE cells. The autofluorescence of control cells, not exposed to POS, was significantly (40%: 1 week p = 0.0011, 2 weeks p = < 0.0001, 3 weeks p = 0.0001; 8%: 1 week p = 0.0036, 2 weeks p = 0.0063, 3 weeks p = 0.0066) lower than that of the POS-fed cells. The autofluorescence increased significantly (40% p = 0.0059; 8% p = 0.0034) between week 1 and week 3 in the control cells. This finding may reflect a contribution to lipofuscin formation by autophagocytized intracellular material. The present model seems to be useful for further studies on the mechanisms behind lipofuscinogenesis of RPE cells as well as the possible effects of lipofuscin accumulation on cell functions and viability.

Published

1996

78. Cellular injury induced by oxidative stress is mediated through lysosomal damage.

Author

Ollinger K and Brunk UT

Subjects

Adenosine Triphosphate metabolism, Animals, Antineoplastic Agents antagonists & inhibitors, Antioxidants pharmacology, Calcium metabolism, Cell Survival drug effects, Cells, Cultured, Cytochalasin B pharmacology, Cytosol metabolism, Deferoxamine pharmacology, Endocytosis drug effects, Glutathione metabolism, Iron Chelating Agents pharmacology, Kinetics, Liver drug effects, Liver physiology, Lysosomes drug effects, Lysosomes physiology, Male, Monensin pharmacology, Naphthoquinones antagonists & inhibitors, Phenylenediamines pharmacology, Rats, Rats, Wistar, Time Factors, Antineoplastic Agents toxicity, Liver pathology, Lysosomes pathology, Naphthoquinones toxicity, Oxidative Stress

Abstract

Cultured primary hepatocytes pretreated (protected) with the iron chelator deferoxamine or the antioxidant N,N'-diphenyl-p-phenylenediamine (DPPD) were resistant to the toxicity of 5 microM naphthazarin (5,8-dihydroxy-1,4-naphthoquinone) during a 180-min exposure. Hepatocytes exposed to naphthazarin without any protection were abruptly depleted of intracellular reduced glutathione, and the level of cytosolic Ca2+ was rapidly increased. This was followed by lipid peroxidation, measured as accumulation of malondialdehyde (MDA) and 4-hydroxyalkenals (4-HNA) intra- and extracellularly; decrease in ATP levels; destabilization of lysosomes; and finally cell death. The stability of the lysosomal membranes was evaluated by determining retention of the lysosomotropic weak base acridine orange (AO). Naphthazarin exposure caused leakage of protons from the acidic compartment, as indicated by relocalization of AO to the cytosol. Protection of the cell cultures with deferoxamine or DPPD prevented destabilization of lysosomes and cell killing. It also reduced the loss of ATP but did not prevent the depletion of glutathione or the increase in Ca2+. In cells subjected to naphthazarin exposure, DPPD protection also completely inhibited lipid peroxidation, whereas deferoxamine pretreatment only slightly reduced the intracellular accumulation of MDA and 4-HNA but completely prevented cell rupture and the leakage of these lipid peroxidation products to the medium that took place in large amounts from unprotected cells exposed to naphthazarin. Deferoxamine is taken up by endocytosis and is thus transported to the acidic vacuolar apparatus, whereas the lipophilic DPPD is rapidly distributed throughout the cells. Inhibiting endocytosis during deferoxamine pretreatment, by incubating at +4 degrees C or by preexposure to a mixture of the endocytosis-inhibitors cytochalasin B and monensin, abolished the protective effect of deferoxamine. The findings suggest that naphthazarin-induced cell killing is not caused directly by either thiol oxidation or an increase in cytosolic free Ca2+, but rather is preceded by lysosomal destabilization, which may be prevented either by inhibition of cellular peroxidation in general or by prevention of iron-catalyzed oxidative reactions, and involves peroxidation of cellular membranes, energy depletion, and leakage of lysosomal content. DPPD would protect against cell killing by preventing lipid peroxidation of cellular membranes in general, whereas deferoxamine seems to allow a limited general cellular peroxidation but specifically prevents peroxidation and fragmentation of lysosomal membranes by chelating intralysosomal iron and, consequently, leakage of destructive lysosomal contents with ensuing cell rupture and death. Thus, a certain degree of cellular peroxidation does not appear to be lethal as long as lysosomal membranes are protected, placing lysosomes into a category of cellular loci minora resistentia.

Published

1995

79. Effects of iron- and hemoglobin-loaded human monocyte-derived macrophages on oxidation and uptake of LDL.

Author

Yuan XM, Brunk UT, and Olsson AG

Subjects

Cell Survival, Culture Media, Culture Media, Conditioned, Electrophoresis, Agar Gel, Exocytosis, Humans, Kinetics, Lipid Metabolism, Lipofuscin metabolism, Lysosomes metabolism, Oxidation-Reduction, Superoxides metabolism, Thiobarbituric Acid Reactive Substances metabolism, Hemoglobins metabolism, Iron metabolism, Lipoproteins, LDL metabolism, Macrophages metabolism

Abstract

It is generally accepted that transition metals are required for cellular LDL oxidation. LDL may also be oxidized by iron and reducing agents in cell-free systems. We hypothesized that lysosomal iron may be exocytosed from macrophages that have been iron loaded by phagocytosis and degradation of iron-rich structures, eg, erythrocytes, and that such released iron may promote LDL oxidation and uptake by macrophages. Human monocyte-derived macrophages (HMDMs) were isolated and cultured for 7 days and then exposed to FeCl3, Fe-ADP, or Fe-EDTA (100 mumol/L) or hemoglobin (25 or 50 micrograms/mL) for 24 hours. After rinsing, LDL (50 to 150 micrograms/mL) was added in fresh culture medium without serum. After another 24 hours the media concentrations of iron and thiobarbituric acid-reacting substances as well as the electrophoretic mobility of LDL were increased, while the cells showed only minimal signs of decreased viability. Lipofuscin, neutral lipids, and phospholipids accumulated in a granular, lysosome-like pattern, and the cells acquired a foam cell-like morphology. There was a strong correlation (r = .87, P = .005) between the amount of iron added during the pre-exposure period and lipofuscin accumulation during the ensuing exposure to LDL in fresh, serum-free medium. Our results support our hypothesis and indicate that lysosomal iron may be exocytosed from HMDMs and promote oxidation and uptake of LDL and thus induce foam cell formation.

Published

1995

80. Lipofuscin accumulation and ageing of fibroblasts.

Author

von Zglinicki T, Nilsson E, Döcke WD, and Brunk UT

Subjects

Cell Survival, Cells, Cultured, Fluorescence, Humans, Lipofuscin analysis, Lung cytology, Aging physiology, Fibroblasts metabolism, Lipofuscin metabolism

Abstract

Lipofuscin accumulates in postmitotic cells. In human fibroblasts, accumulation of lipofuscin as measured by cellular autofluorescence is exponential at first, but stops at a certain level. At the same time, cell death starts to decrease cell numbers significantly. Artificial lipofuscin-like material can be prepared by UV-crosslinking of mitochondrial preparations. This material is easily phagocytosed by human fibroblasts and results in an increased cellular lipofuscin accumulation. Such a forced lipofuscin accumulation is sufficient to block cellular proliferation within a short time and to induce cell death as soon as the cellular lipofuscin autofluorescence reaches the same upper limit as that observed in senescent cells. It is concluded that accumulation of lipofuscin in postmitotic cells is not just an innocent consequence of ageing, but rather one amongst the important causes of senescence.

Published

1995

81. Intracellular interactions under oxidative stress and aging: a hypothesis.

Author

von Zglinicki T and Brunk UT

Subjects

Aged, DNA Damage physiology, DNA, Mitochondrial physiology, Free Radicals, Humans, Lipid Peroxidation physiology, Lipofuscin metabolism, Lysosomes physiology, Cellular Senescence physiology, Mitochondria physiology, Reactive Oxygen Species metabolism

Abstract

Oxygen-derived free radicals may result from various reactions, both intra- and extracellularly, but generation of oxygen free radicals from electrons escaping from the electron transport chain in mitochondria is by far the predominant process during the lifetime of a "normal", healthy cell. There is clear evidence that mitochondria are also an important target for oxygen-derived free radicals, and the resulting mitochondrial malfunction has long been suggested as the intracellular basis of aging. Moreover, there is clear evidence that free radical-dependent reactions lead to lipofuscin formation and its accumulation in Lysosomes of post-mitotic cells. Lipofuscin accumulation was demonstrated to be dependent on the probability of iron-catalyzed Fenton reactions. A hypothesis is presented which assumes free radical dependent reactions in mitochondria and lysosomes to be interdependent. Production of hydrogen peroxide in mitochondria and its subsequent diffusion in the cytoplasm, and Fenton reactions in lysosomes, transferring hydrogen peroxide intra-lysosomally to the highly cytotoxic hydroxyl radical, are thought to be necessary intermediary steps in the generation of mitochondrial damage. On the other hand, damage to mitochondria increases both mitochondrial output of hydrogen peroxide and lipofuscin accumulation.

Published

1993

82. Mitochondrial production of pro-oxidants and cellular senescence.

Author

Sohal RS and Brunk UT

Subjects

Animals, Houseflies, Hydrogen Peroxide metabolism, Models, Biological, Oxygen Consumption, Superoxides metabolism, Aging physiology, Cellular Senescence physiology, Mitochondria metabolism, Oxidants metabolism

Abstract

Mitochondria are the major intracellular producers of O2- and H2O2. The level of oxidative stress in cells, as indicated by the in vivo exhalation of alkanes and the concentration of molecular products of oxy-radical reactions, increases during aging in mammals as well as insects. In this paper, we discuss the relationship between mitochondrial generation of O2- and H2O2, and the aging process. The rate of mitochondrial O2- and H2O2 generation increases with age in houseflies and the brain, heart and liver of rat. This rate has been found to correspond to the life expectancy of flies and to the maximum life span potential (MLSP) of six different mammalian species, namely, mouse, rat, guinea pig, rabbit, pig and cow. In contrast, the level of antioxidant defenses provided by activities of superoxide dismutase, catalase, glutathione peroxidase and glutathione concentration neither uniformly declines with age nor corresponds to variations in MLSP of different mammalian species. It is argued that the rate of mitochondrial O2- and H2O2 generation rather than the antioxidant level may act as a longevity determinant.

Published

1992

83. A novel hypothesis of lipofuscinogenesis and cellular aging based on interactions between oxidative stress and autophagocytosis.

Author

Brunk UT, Jones CB, and Sohal RS

Subjects

Animals, Cells, Cultured, Free Radicals metabolism, Hydrogen Peroxide metabolism, Hydroxides metabolism, Hydroxyl Radical, Models, Biological, Rats, Superoxides metabolism, Autophagy, Cellular Senescence physiology, Heart physiology, Lipofuscin biosynthesis, Mitochondria, Heart metabolism, Oxygen metabolism

Abstract

Based on a series of experiments, using cultured postmitotic neonatal rat cardiac myocytes as a model system, we present a novel hypothesis of lipofuscin formation. This hypothesis proposes that lipofuscin is formed within secondary lysosomes due to an interplay of two processes, the production of partially reduced oxygen species by mitochondria and the autophagocytotic degradation within secondary lysosomes. Specifically, it is proposed that H2O2 generated by mitochondria and other organelles permeates into the lumen of secondary lysosomes, which contain iron derived from cellular structures undergoing intralysosomal degradation. The interaction between reactive ferrous iron and H2O2 results, via Fenton-type mechanisms, in the generation of hydroxyl free radicals (OH), inducing lipid peroxidation and eventually leading to intermolecular cross-linking and lipofuscin formation. Additionally, mitochondria undergoing intralysosomal decomposition might continue for a certain period to produce superoxide anion radicals (O2-) and thus also H2O2. This model of lipofuscinogenesis could satisfactorily explain the variations observed in the rates of lipofuscinogenesis among different postmitotic cell types in various species. Such variations might arise from a variety of factors including differences in the efficiency of the 'anti-oxidative shield', rate of H2O2 generation, amount of chain-breaking antioxidants, mode of intralysosomal iron chelation, rate of autophagocytosis as well as degree of efficiency of the intralysosomal hydrolytic enzymes.

Published

1992

84. Alloxan cytotoxicity involves lysosomal damage.

Author

Zhang H, Zdolsek JM, and Brunk UT

Subjects

Animals, Cell Survival drug effects, Deferoxamine pharmacology, Free Radicals, Glutathione metabolism, In Vitro Techniques, Intracellular Membranes drug effects, Mice, Oxidation-Reduction, Oxygen Consumption drug effects, Tumor Cells, Cultured, Alloxan toxicity, Lysosomes drug effects

Abstract

The cytotoxic effects of alloxan are not understood in any great detail, although they are considered to involve reactions mediated by oxygen-derived free radicals. These reactive species may form extra-or intracellularly following alloxan reduction, and result in cell damage through a number of complex interactions with a variety of macromolecules. The purpose of the present study was to elucidate further the early intracellular effects of alloxan on a model system of macrophage-like cells in culture. Addition of alloxan (15 mM), without reducing agents, to the medium surrounding the cells (phosphate-buffered saline, PBS, 37 degrees C, pH 7.4) resulted in rapid lysosomal damage (disappearance of the proton gradient over the membrane) followed by severe cellular degeneration (swelling and blebbing) and 50% cell death (trypan blue dye exclusion test) within fifty min. Cells pretreated with the gamma-glutamyl cysteine synthetase-inhibiting agent BSO, to decrease levels of intracellular glutathione, showed enhanced sensitivity to alloxan. The results are interpreted as indicating the cytotoxicity to result from intracellular formation of superoxide radicals, hydrogen peroxide and hydroxyl radicals, the latter within secondary lysosomes containing trace amounts of reactive iron (inducing Fenton reactions). The ensuing lysosomal membrane damage may result in leakage of lysosomal hydrolases and further cellular degeneration.

Published

1992

85. Extracellular reduction of alloxan results in oxygen radical-mediated attack on plasma and lysosomal membranes.

Author

Zhang H, Gao G, and Brunk UT

Subjects

Acridine Orange, Alloxan metabolism, Animals, Catalase pharmacology, Cell Membrane Permeability drug effects, Cysteine pharmacology, Deferoxamine pharmacology, Free Radicals, In Vitro Techniques, Intracellular Membranes drug effects, Kinetics, Mice, Microscopy, Fluorescence, Mitochondria drug effects, Oxidation-Reduction, Oxygen Consumption, Superoxide Dismutase pharmacology, Tumor Cells, Cultured, Alloxan toxicity, Cell Membrane drug effects, Lysosomes drug effects, Oxygen toxicity

Abstract

Alloxan participation in extracellular redox processes results in the formation of the reactive oxygen species (ROS) superoxide anions (O2-), hydroxyl radical (OH.) and hydrogen peroxide (H2O2), causing cell damage through a number of complex interactions probably involving several different cellular structures. These involve the plasma membrane, and we have recently presented evidence for lysosomal interference. The present study elucidates the early (within 15 min) events in a model system of macrophage-like cells (J-774) in culture. Addition of 2 mM alloxan and 1 mM cysteine to the medium surrounding the cells (phosphate-buffered saline, PBS, 37 degrees C, pH 7.4) resulted in rapid lysosomal membrane damage with disappearance of the proton gradient as visualized by acridine orange relocalization, as well as plasma membrane alterations leading to increased leakage of fluorescein after fluorescein diacetate staining. These events were later (greater than 30 min) followed by cellular degeneration in the form of blebbing. Mitochondrial damage (rhodamine 123 relocalization) was a late event. Cells pretreated with desferrioxamine (Des) and superoxide dismutase (SOD) or Des, SOD and catalase (CAT) to induce partial (H2O2 formation only) or almost full protection (no ROS formation) showed about the same reactions as when cells were exposed to alloxan and cysteine without scavengers (O2-, H2O2 and OH. formation) or with PBS only, respectively. The results are interpreted as indicating that the cytotoxicity is a consequence mainly of H2O2 involvement and probably of lysosomal influx of H2O2 with ensuing OH.formation within secondary lysosomes containing trace amounts of reactive iron. It is suggested that the resultant lysosomal membrane damage is followed by leakage of lysosomal hydrolases and ensuing cellular degeneration.

Published

1992

86. Lipofuscinogenesis in a model system of cultured cardiac myocytes.

Author

Marzabadi MR, Yin D, and Brunk UT

Subjects

Aging metabolism, Animals, Cells, Cultured, Free Radicals metabolism, Humans, Lysosomes metabolism, Models, Biological, Neuroglia metabolism, Organelles metabolism, Organelles ultrastructure, Lipofuscin biosynthesis, Myocardium metabolism

Abstract

Lipofuscin, or age pigment, is a yellowish-brown, autofluorescent, protein, and lipid containing pigment that accumulates in the lysosomal vacuome of a variety of post-mitotic cells in man and animals during aging. Lipofuscin seems to be an end product of peroxidation, fragmentation and polymerization of proteins and lipids. Protein and lipid containing materials are regularly sequestered to the lysosomal system by means of endocytosis and autophagocytosis. Lysosomes and acidified endosomes constitute cellular compartments where iron for short periods of time may exist in reactive form allowing for peroxidative processes. The importance was demonstrated in model systems of cultured cells subjected to oxidative stress and augmented amounts of FeCl3 in the culture medium. This combination was considered to result in increased intracellular, mainly mitochondrial, production of hydrogen peroxide as well as increased intralysosomal concentration of iron. One of the results of this situation was dramatically increased lipofuscinogenesis.

Published

1992

87. Oxidized ascorbic acid and reaction products between ascorbic and amino acids might constitute part of age pigments.

Author

Yin DZ and Brunk UT

Subjects

Free Radicals, Hydrogen-Ion Concentration, In Vitro Techniques, Lipofuscin chemistry, Oxidation-Reduction, Oxygen chemistry, Pigments, Biological chemistry, Spectrometry, Fluorescence, Thiobarbiturates chemistry, Aging metabolism, Amino Acids chemistry, Ascorbic Acid chemistry

Abstract

Fluorescence and non-enzymatic browning were observed in reactions between ascorbic acid (AH2) and amino acids (AA) as well as in reactions involving AH2 autoxidation and/or polymerization in the presence of trace amounts of adventitious iron (less than or equal to 10 microM). These reaction products exhibited fluorescent spectra (400-490 nm) akin to those of extracts from lipofuscin-rich tissues. Lengthy incubation of AH2 at 37 degrees C in phosphate buffer (pH 7.0) caused a concentration- and time-dependent increase in absorbance at 412 nm, paralleling increase in 377/440 nm fluorescence, due to formation of autoxidation/polymerization products. The fluorescences of these substances were increased by acidity and quenched at alkaline conditions but restored by neutralization. The reactions between AH2 (0.1-2.0 mM) and a number of AA (1.0-4.0 mM) were also found to result in products with blue fluorescence. Following TBA test, the AH2 autoxidation/polymerization products and AH2/AA reaction products showed only moderate and slight absorbance at 535 nm, respectively, indicating a little or minute formation of aldehydes with MDA-like reactivity. The findings in this study, nevertheless, suggest possible misinterpretations of results in previous studies dealing with AH2-dependent, oxygen free radical induced, 'lipofuscin-related fluorescence'. Thus, similar to nonenzymatic glycosylation (Maillard) reactions, AH2 autoxidation as well as reactions between AH2 and AA may result in 'lipofuscin-like material', as judged from their fluorescence spectral patterns.

Published

1991

88. Effects of alloxan and reducing agents on macrophages in culture.

Author

Zhang H, Zdolsek JM, and Brunk UT

Subjects

Animals, Catalase pharmacology, Cell Death drug effects, Cell Line, Cell Survival drug effects, Deferoxamine pharmacology, Free Radicals, Macrophages cytology, Macrophages drug effects, Mice, Oxygen Consumption drug effects, Superoxide Dismutase pharmacology, Alloxan pharmacology, Ascorbic Acid pharmacology, Cysteine pharmacology, Macrophages metabolism

Abstract

The diabetogenic effect of the quinonoid compound alloxan is not understood in detail although it supposedly involves reactions mediated by alloxan and oxygen radicals. These reactive species may form extra- or intracellularly and cause cell damage through a variety of complex interactions with several macromolecules. The purpose of this study was to elucidate early (less than or equal to 60 min) effects of alloxan and reducing agents (cysteine and ascorbic acid) on cultured macrophages, as assayed by the trypan blue dye exclusion test and the sensitive fluorescein diacetate and propidium iodide (FDA/PI) double staining technique. During the reactions between alloxan and reducing agents, oxygen was consumed as a sign of superoxide anion radical formation. When alloxan alone was added to two different culture media without serum, oxygen was still consumed, indicating formation of oxygen radicals due to the occurrence of reducing substances in cell culture media. This finding demonstrated the necessity of performing further studies in solutions without reducing capacity, e.g. in phosphate-buffered saline. The experiments showed that exposure of normal and malignant macrophages to alloxan and reducing substances resulted in rapidly occurring plasma membrane damage and ensuing cell death. Separate addition of catalase, desferrioxamine or superoxide dismutase resulted in evident, slight and no protection, respectively. The combinations of (i) catalase and desferrioxamine, and (ii) catalase, desferrioxamine and superoxide dismutase, however, inhibited cell damage in a pronounced and complete way, respectively. The results are interpreted as indicating cell damage due to the extracellular formation of hydrogen peroxide and hydroxyl radicals. The latter in close proximity to the cells and acting on the plasma membrane, while the former, after diffusing into the cell, may have several intracellular targets. The FDA/PI technique proved its value as a quantifiable method for the evaluation not only of cell death but also of cell damage with computer-based fluorometry.

Published

1991

89. Microfluorometric and fluorometric lipofuscin spectral discrepancies: a concentration-dependent metachromatic effect?

Author

Yin DZ and Brunk UT

Subjects

Aging metabolism, Animals, Dihydropyridines analysis, Evaluation Studies as Topic, Humans, Lipid Peroxidation, Malondialdehyde analysis, Microscopy, Fluorescence, Schiff Bases analysis, Spectrometry, Fluorescence, Lipofuscin analysis

Abstract

The fluorescent spectral patterns of some lipid peroxidation products and their derivatives have been investigated. A significant concentration-dependent fluorescence shift was found. A variety of suggested age pigment fluorophores, 1,4-dihydropyridines, Schiff base and MDA polymers, all demonstrated a potential for spectral shifts. Along with increased concentration, the fluorescence peaks of these fluorophores shifted from blue (400-490 nm) to golden-yellow or orange-red (500-600 nm). The demonstrated metachromasia is supposed to be an inner-filter effect resulting from molecular polymerization or stacking. Thus, the striking differences between lipofuscin fluorescence spectra obtained by different investigators may be explained as due to large differences in lipofuscin concentration during measurement with different techniques. The pigments are either studied in situ by morphologists and recorded by microscopic fluorometry or by biochemists using spectrofluorometers to measure the extracted and dissolved pigments.

Published

1991

90. Mechanisms of lipofuscinogenesis: effect of the inhibition of lysosomal proteinases and lipases under varying concentrations of ambient oxygen in cultured rat neonatal myocardial cells.

Author

Marzabadi MR, Sohal RS, and Brunk UT

Subjects

Animals, Animals, Newborn, Cells, Cultured, Cysteine Proteinase Inhibitors pharmacology, Heart drug effects, Kinetics, Leucine pharmacology, Lysosomes enzymology, Microscopy, Electron, Myocardium cytology, Myocardium ultrastructure, Oxygen pharmacology, Rats, Cathepsins antagonists & inhibitors, Leucine analogs & derivatives, Leupeptins pharmacology, Lipofuscin biosynthesis, Myocardium metabolism, Netilmicin pharmacology, Phospholipases antagonists & inhibitors

Abstract

The objective of this study was to analyse the relative roles of oxidative stress and lysosomal lytic enzymes in lipofuscin formation in cultured neonatal rat cardiac myocytes. Myocytes were exposed to E-64 (an inhibitor of lysosomal cathepsins L. D and H), netilmicin (an inhibitor of lysosomal phospholipases A1 and C) and leupeptin (an inhibitor of cytosolic and lysosomal thiolproteinases) under varied conditions of oxidative stress (20% and 40% ambient oxygen) for up 14 days. Lipofuscin was quantified by microspectrofluorometry. The amount of lipofuscin accumulation was enhanced by the lytic enzyme inhibitors as well as by the increase in the ambient oxygen concentration. However, the effects of enzyme inhibitors was less obvious under 40% ambient oxygen than under 20% oxygen. Data are interpreted as suggesting that, under high levels of oxidative stress, intralysosomal peroxidative changes related to lipofuscin formation occur so rapidly that lytic activity assumes a minor role in lipofuscinogenesis whereas, under low oxidative stress, inhibition of lytic activity makes a greater contribution to lipofuscinogenesis by allowing a longer period of time for peroxidative changes. The results further substantiate the hypotheses that (a) lipofuscinogenesis is strongly related to oxidative stress, and (b) lipofuscin forms intralysosomally as a result of processes involving incomplete degradation of heterophagocytosed and or autophagocytosed material.

Published

1991

91. Effect of alpha-tocopherol and some metal chelators on lipofuscin accumulation in cultured neonatal rat cardiac myocytes.

Author

Marzabadi MR, Sohal RS, and Brunk UT

Subjects

Animals, Animals, Newborn, Antioxidants pharmacology, Cells, Cultured, Deferoxamine pharmacology, Pentetic Acid pharmacology, Rats, Rats, Inbred Strains, Chelating Agents pharmacology, Lipofuscin metabolism, Myocardium metabolism, Oxygen metabolism, Vitamin E pharmacology

Abstract

The objective of this study was to test further the hypothesis that oxidative stress is a major causal factor in lipofuscin formation. We have previously shown that cultured cardiac myocytes constitute a suitable model system for the study of factors influencing lipofuscinogenesis. The specific aim of the present study was to elucidate the effects of the chain-breaking free radical scavenger alpha-tocopherol, and the chelators desferrioxamine, EDTA and DTPA on the accumulation of lipofuscin. The effects were examined at different degrees of oxidative stress, obtained by varying the ambient oxygen concentration from 5 to 40%. Lipofuscin was quantified by microspectrofluorometry. Lipofuscin-specific, yellow autofluorescence increased with time in culture, and with enhanced oxidative stress. Increasing concentration of alpha-tocopherol, up to 40 microM, had an inhibitory effect on lipofuscin accumulation that was most pronounced at high oxidative stress. Desferrioxamine and DTPA, both caused a pronounced reduction in lipofuscin formation, while EDTA had no significant effect. The findings are interpreted to support the concept that oxidative stress is a causal factor in lipofuscinogenesis, and that lipofuscin is a product of autophagocytosed, membrane-rich material subjected to free radical-induced, metal-catalyzed peroxidation, fragmentation, and polymerization within the lysosomal vacuome.

Published

1990

92. Hydrogen peroxide production by liver mitochondria in different species.

Author

Sohal RS, Svensson I, and Brunk UT

Subjects

Animals, Antimycin A pharmacology, Cattle, Drosophila melanogaster, Free Radicals, Guinea Pigs, Houseflies, In Vitro Techniques, Mice, Mitochondria, Muscle metabolism, Rats, Rotenone pharmacology, Species Specificity, Swine, Hydrogen Peroxide metabolism, Longevity physiology, Mitochondria, Liver metabolism

Abstract

The objective of this study was to further examine the relationship between oxygen free radicals and the aging process in animals. The rate of H2O2, a product of superoxide anion radical dismutation, released by liver mitochondria, was measured in the mouse, rat, guinea pig, rabbit, pig and cow as well as in flight muscle mitochondria of Drosophila melanogaster and the housefly, Musca domestica. The rate of H2O2 generation was inversely related to the maximum life span potential (MLSP) of the species. A 42-fold difference in the rate of H2O2 secretion was found among mammals and an up to 300-fold difference was noted between the insects and the mammals. Results of this study indicate that under identical conditions mitochondria from animals with low MLSP release relatively greater amounts of H2O2.

Published

1990

93. Relationship between antioxidant defenses and longevity in different mammalian species.

Author

Sohal RS, Sohal BH, and Brunk UT

Subjects

Animals, Brain metabolism, Catalase metabolism, Cattle, Free Radicals, Glutathione metabolism, Glutathione Peroxidase metabolism, Guinea Pigs, Liver metabolism, Mice, Myocardium metabolism, Organ Specificity physiology, Rabbits, Rats, Rats, Inbred Strains, Species Specificity, Superoxide Dismutase metabolism, Swine, Aging metabolism, Antioxidants metabolism, Longevity physiology

Abstract

The general objective of this investigation was to examine the relationship between oxygen free radicals and the aging process. Comparisons of antioxidant defenses were made in six different mammalian species, namely, mouse, rat, guinea pig, rabbit, pig and cow, which range from 3.5 to 30 years in their maximum life span potential (MLSP). Activities of superoxide dismutase (SOD), catalase, and glutathione peroxidase, and concentration of glutathione were measured in the liver, the heart, and the brain. SOD and catalase activities were positively correlated whereas glutathione concentration was negatively correlated with MLSP. Glutathione peroxidase activity exhibited a variable pattern: being positively correlated with MLSP in the brain and negatively correlated in the liver and the heart. In each organ, MLSP was correlated with relatively high levels of one or two of the above antioxidants and low levels of the other antioxidants, indicating the possibility of a compensatory balance among various components of the antioxidant system. No obvious pattern of a relationship was detectable between the overall level of antioxidant defenses and MLSP among the mammalian species examined. The implications of this finding concerning the role of oxidative stress in the aging process and the free radical hypothesis of aging are discussed.

Published

1990

94. Photooxidative damage to lysosomes of cultured macrophages by acridine orange.

Author

Zdolsek JM, Olsson GM, and Brunk UT

Subjects

Animals, Cell Survival drug effects, Cell Survival radiation effects, Cells, Cultured, Cysteine Proteinase Inhibitors, Fluorescence, Leucine analogs & derivatives, Leucine pharmacology, Lysosomes drug effects, Lysosomes radiation effects, Mice, Microscopy, Electron, Microscopy, Electron, Scanning, Oxidation-Reduction, Acridine Orange pharmacology, Light, Lysosomes enzymology, Macrophages ultrastructure

Abstract

Cultured cells accumulate acridine orange (AO), which is a weak basic dye and a photosensitizer, in lysosomes and other acidic compartments. During exposure to blue light, AO-loaded macrophages show decreasing red granular fluorescence and increasing green diffuse fluorescence. This is hypothesized to represent peroxidative damage to lysosomal membranes resulting in an impaired proton gradient with deprotonation of the AO to its uncharged form and subsequent leakage of the dye. Further damage to the lysosomal membranes will result in release of lytic enzymes from the lysosomal compartment into the cytosol, leading to degeneration and finally cell death. The survival of AO-loaded and light-exposed macrophages is controllable by varying the exposure times to blue light. Inhibition of lysosomal proteases by E-64 results in increased cell survival after AO and blue light-mediated damage, indicating a role of proteolytic enzymes in this type of damage. Morphological analysis shows 'rounding up' with formation of retraction fibrils and pronounced plasma membrane blebbing. The formation of autophagic vacuoles is an early and pronounced event. After protease inhibition, however, all these phenomena are inhibitable to a considerable degree. We have thus directed photooxidative damage selectively to lysosomal membranes and their contents. This technique will allow further detailed studies of the role of lysosomes in degeneration-regeneration processes.

Published

1990

95. TEM and SEM findings in cat fibroblasts cultivated in vitro with and without Mycoplasma.

Author

Larsson E and Brunk UT

Subjects

Animals, Cats, Cells, Cultured, Fibroblasts drug effects, Kanamycin pharmacology, Lysosomes enzymology, Microscopy, Electron, Microscopy, Electron, Scanning, Phagocytosis, Fibroblasts ultrastructure, Mycoplasma drug effects

Abstract

Mycoplasma contamination of cultured cells may cause considerable interference with their behaviour and metabolism. Whether or not mycoplasma are actually taken up by cells in vitro has long been a matter of dispute. In the present study mycoplasma were shown to phagocytosed by feline lung fibroblasts and to end up in the lysosomal vacuome of the cells, where the organisms were only partially degraded by the hydrolytic enzymes leading to a rapid (within a few days) accumulation of secondary lysosomes of the residual body variety. It is thus obvious that studies on the structure and function of the lysosomal vacuome in cultured cells are possible only if precautions are taken to avoid that the cultures become contaminated by mycoplasma.

Published

1981

96. High resolution SEM of cultured cells: preparatory procedures.

Author

Arro E, Collins VP, and Brunk UT

Subjects

Cell Line, Fixatives, Glioblastoma, Glutaral, Gold, Humans, Hydrolyzable Tannins, Microvilli ultrastructure, Osmium Tetroxide, Palladium, Cell Membrane ultrastructure, Cells, Cultured ultrastructure, Cytological Techniques, Microscopy, Electron, Scanning methods

Published

1981

97. Discharge of newly-synthesized dolichol and ubiquinone with lipoproteins to rat liver perfusate and to the bile.

Author

Elmberger PG, Kalén A, Brunk UT, and Dallner G

Subjects

Animals, Bile metabolism, Dolichol Phosphates metabolism, In Vitro Techniques, Lipoproteins metabolism, Lipoproteins ultrastructure, Liver ultrastructure, Male, Microscopy, Electron, Perfusion, Rats, Rats, Inbred Strains, Dolichols metabolism, Liver metabolism, Ubiquinone metabolism

Abstract

An effective system for perfusing rat liver using complete tissue culture medium and washed calf erythrocytes as oxygen carriers was devised. Infusion of taurocholate and glucose proved necessary to maintain stable metabolic activity and bile secretion during a 6-hr period. Perfusate pO2, pCO2 and pH values were monitored continuously and found to be stable. Electron microscopic examination revealed the maintenance of normal hepatic structure, even after 6 hr. Normal rates of protein and urea synthesis, no leakage of cytoplasmic enzymes, and continuous bile acid production demonstrated the functional integrity of this system. Using [3H]mevalonic acid as precursor, dolichol, dolichyl phosphate, ubiquinone and cholesterol were found to be continuously synthesized in this perfused liver system. All these lipids appeared in the perfusate, indicating discharge through the ER-Golgi system. The lipoproteins of the perfusate were isolated by ultracentrifugation and characterized with respect to size distribution and lipid composition. Dolichol was found in VLDL, LDL and HDL fractions, with the highest concentration present in the latter. In rat and human blood plasma this lipid was mainly associated with HDL. The ubiquinone in the perfusate was primarily associated with the VLDL fraction, while in rat plasma it was found more evenly distributed among all the three lipoprotein fractions studied. Dolichol, ubiquinone and cholesterol were also discharged to the bile, whereas dolichyl phosphate was not. Thus, newly-synthesized dolichol and ubiquinone are transported out of the hepatocyte to the blood and to the bile.

Published

1989

98. Quantitation of residual bodies in cultured human glial cells during stationary and logarithmic growth phases.

Author

Collins VP and Brunk UT

Subjects

Cell Cycle, Cell Nucleus ultrastructure, Cells, Cultured, Cytoplasm ultrastructure, Humans, Neuroglia cytology, Cytoplasmic Granules ultrastructure, Lipofuscin, Neuroglia ultrastructure, Pigments, Biological

Published

1978

99. Cytoplasmic effects of X-irradiation on cultured cells in a non-dividing stage. 4. Studies of sparsely grown, serum-deprived cells.

Author

Hamberg H, Brunk UT, Ericsson JL, and Jung B

Subjects

Cell Movement radiation effects, Cytoskeleton radiation effects, Cytoskeleton ultrastructure, Fluorescent Antibody Technique, Humans, Interphase radiation effects, Microscopy, Electron, Microscopy, Phase-Contrast, Microtubules radiation effects, Microtubules ultrastructure, Neuroglia ultrastructure, Organoids radiation effects, Organoids ultrastructure, Neuroglia radiation effects

Abstract

Cultured human glial cells were blocked in interphase (G1) by 24 h of serum starvation and subsequently subjected to 200 Gy, 8 MV X-radiation. Immediately following irradiation the cultures were transferred to serum-containig medium. Time-lapse cinemicrography performed during the next 48 h showed a profoundly disturbed motility with decreased ability for polarization and locomotion of the irradiated cells. Specimens fixed 24 and 48 h after irradiation and investigated by immunofluorescence with tubulin-antibodies and DNase/DNase-antibodies, and by whole cell transmission electron microscopy showed derangements in the distribution of microfilament bundles related to the cytoplasmic ramification of the irradiated cells, but otherwise no detectable alterations in structure or distribution of either microtubules or microfilaments. It is suggested that the alteration in the arrangement of filament bundles is of importance to the impaired locomotion of the irradiated cells.

Published

1980

100. Cytoplasmic effects of x-irradiation on cultured cells in a nondividing stage. 1. Establishment of an experimental model.

Author

Hamberg H, Brunk UT, Ericsson JL, and Jung B

Subjects

Cell Line, Cells, Cultured, Dose-Response Relationship, Radiation, Humans, Neuroglia ultrastructure, Radiation Dosage, Neuroglia radiation effects, Radiation Effects

Abstract

The investigation was initiated with the aim of establishing a suitable experimental model with respect to mode of radiation and radiation dose for elucidating morphologically the sequential development of radiation induced damage of interphase cells (human glia cells in vitro). Adequately defined and reproducible cellular changes were obtained using X-radiation generated by an 8 MeV linear accelerator at a dose of 20,000 rad. The cellular alterations were studied in the light microscope and by scanning and transmission electron microscopy. The most conspicuous changes--first appreciable about 5 hours after irradiation--occurred in the lysosomal vacuome, and the plasma membrane and associated structures.

Published

1976