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Dive into the research topics where Despina Kokkinou is active.

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Featured researches published by Despina Kokkinou.


PLOS ONE | 2011

Zinc deficiency leads to lipofuscin accumulation in the retinal pigment epithelium of pigmented rats.

Sylvie Julien; Antje Biesemeier; Despina Kokkinou; O. Eibl; Ulrich Schraermeyer

Background Age-related macular degeneration (AMD) is associated with lipofuscin accumulation whereas the content of melanosomes decreases. Melanosomes are the main storage of zinc in the pigmented tissues. Since the elderly population, as the most affected group for AMD, is prone to zinc deficit, we investigated the chemical and ultrastructural effects of zinc deficiency in pigmented rat eyes after a six-month zinc penury diet. Methodology/Principal Findings Adult Long Evans (LE) rats were investigated. The control animals were fed with a normal alimentation whereas the zinc-deficiency rats (ZD-LE) were fed with a zinc deficient diet for six months. Quantitative Energy Dispersive X-ray (EDX) microanalysis yielded the zinc mole fractions of melanosomes in the retinal pigment epithelium (RPE). The lateral resolution of the analysis was 100 nm. The zinc mole fractions of melanosomes were significantly smaller in the RPE of ZD-LE rats as compared to the LE control rats. Light, fluorescence and electron microscopy, as well as immunohistochemistry were performed. The numbers of lipofuscin granules in the RPE and of infiltrated cells (Ø>3 µm) found in the choroid were quantified. The number of lipofuscin granules significantly increased in ZD-LE as compared to control rats. Infiltrated cells bigger than 3 µm were only detected in the choroid of ZD-LE animals. Moreover, the thickness of the Bruchs membrane of ZD-LE rats varied between 0.4–3 µm and thin, rangy ED1 positive macrophages were found attached at these sites of Bruchs membrane or even inside it. Conclusions/Significance In pigmented rats, zinc deficiency yielded an accumulation of lipofuscin in the RPE and of large pigmented macrophages in the choroids as well as the appearance of thin, rangy macrophages at Bruchs membrane. Moreover, we showed that a zinc diet reduced the zinc mole fraction of melanosomes in the RPE and modulated the thickness of the Bruchs membrane.


Zeitschrift für Naturforschung C | 2006

Melanin Protects Choroidal Blood Vessels against Light Toxicity

Swaantje Peters; Thomas Lamah; Despina Kokkinou; Karl Ulrich Bartz-Schmidt; Ulrich Schraermeyer

Low ocular pigmentation and high long-term exposure to bright light are believed to increase the risk of developing age-related macular degeneration (ARMD). To investigate the role of pigmentation during bright light exposure, cell damage in retinae and choroids of pigmented and non-pigmented rats were compared. Pigmented Long Evans (LE) rats and non-pigmented (albino) Wistar rats were exposed to high intensity visible light from a cold light source with 140,000 lux for 30 min. Control animals of both strains were not irradiated. The animals had their pupils dilated to prevent light absorbance by iris pigmentation. 22 h after irradiation, the rats were sacrificed and their eyes enucleated. Posterior segments, containing retina and choroid, were prepared for light and electron microscopy. Twenty different sections of specified and equal areas were examined in every eye. In albino rats severe retinal damage was observed after light exposure, rod outer segments (ROS) were shortened and the thickness of the outer nuclear layer (ONL) was significantly diminished. Choriocapillaris blood vessels were obstructed. In wide areas the retinal pigment epithelium (RPE) was absent in albino rats after irradiation. In contrast, LE rats presented much less cell damage in the RPE and retina after bright light exposure, although intra-individual differences were observed. The thickness of the ONL was almost unchanged compared to controls. ROS were shortened in LE rats, but the effect was considerably less than that seen in the albinos. Only minimal changes were found in choroidal blood vessels of pigmented rats. The RPE showed certain toxic damage, but cells were not destroyed as in the non-pigmented animals. The number of melanin granules in the RPE of LE rats was reduced after irradiation. Ocular melanin protects the retina and choroid of pigmented eyes against light-induced cell toxicity. Physical protection of iris melanin, as possible in eyes with non-dilated pupils, does not seem to play a major role in our setup. Biochemical mechanisms, like reducing oxidative intracellular stress, are more likely to be responsible for melanin-related light protection in eyes with dilated lens aperture.


Toxicologic Pathology | 2007

Melanin Precursor 5,6-Dihydroxyindol: Protective Effects and Cytotoxicity on Retinal Cells in vitro and in vivo

Peter Heiduschka; Petra Blitgen-Heinecke; Aysegül Tura; Despina Kokkinou; Sylvie Julien; Sabine Hofmeister; Karl Ulrich Bartz-Schmidt; Ulrich Schraermeyer

5,6-Dihydroxyindole (DHI) is a melanin pigment precursor with antioxidant properties. In the light of a report about cytotoxicity of DHI, the aim of this study was to assess possible toxic effects of DHI on cells related to the eye, such as human ARPE-19 cells and mouse retinal explants. Moreover, DHI was tested on its effects on retinal function in vivo using electroretinography. We found cytotoxicity of DHI against ARPE-19 cells at 100 μM, but not at 10 μM. 10 μM DHI exhibited a slight, though not significant protective activity against UV-A damage in ARPE-19 cells. We found cytoprotection in cultured mouse retinas by 50 μM DHI or its diacetylated derivative 5,6-diacetoxyindole (DAI), respectively. In ERG measurements in vivo, amplitudes were decreased only slightly by 100 μM DHI compared to saline, whereas a better preservation of amplitudes was visible at 10 μM DHI, in particular with respect to cones. In histological sections, more cones were found at 10 μM DHI than at 100 μM DHI. As a conclusion, DHI shows a slight protective effect at 10 μM both in vitro and in vivo. At 100 μM, it shows a strong cytotoxicity in vitro, which is strongly reduced in vivo.


Journal of Photochemistry and Photobiology B-biology | 2008

UV-A induced oxidative stress is more prominent in naturally pigmented aged human RPE cells compared to non-pigmented human RPE cells independent of zinc treatment

Antje Biesemeier; Despina Kokkinou; Sylvie Julien; Peter Heiduschka; Mark Berneburg; Karl Ulrich Bartz-Schmidt; Ulrich Schraermeyer

To investigate the effects of zinc supplementation on human amelanotic (ARPE-19) and native pigmented retinal pigment epithelial cells (hRPE) under normal light conditions and after ultraviolet A light exposure. hRPE cells, containing both melanin and lipofuscin granules, were prepared from human donor eyes of 60-70 year old patients. Cells of the amelanotic ARPE-19 cell line and pigmented hRPE cells were treated with zinc chloride and subjected to oxidative stress by UV-A irradiation. Intracellular H(2)O(2) formation was measured using a fluorescence oxidation assay. Additionally, apoptosis and viability assays were performed. Control cells were treated identically except for irradiation and zinc supplementation. Under normal light conditions, zinc treated hRPE cells produced less H(2)O(2) than unsupplemented hRPE cells. Viability and apoptosis events did not change. After UV-A irradiation, ARPE and hRPE cells were greatly impaired in all tests performed compared to the non-irradiated controls. No differences were found after zinc supplementation. hRPE cells showed a higher apoptosis and mortality rate than non-pigmented cells when stressed by UV-A light. ARPE cells never showed any zinc related effects. In contrast, without irradiation, zinc supplementation reduced H(2)O(2) production in pigmented hRPE cells slightly. We did not find any zinc effect in irradiated hRPE cells. After UV light exposure, pigmented cells showed a higher apoptosis and mortality than cells lacking any pigmentation. We conclude that cells with pigmentation consisting of melanin and lipofuscin granules have more prooxidative than antioxidative capacity when stressed by UV light exposure compared to cells lacking any pigmentation.


Experimental Eye Research | 2006

Tyrosinase biosynthesis in adult mammalian retinal pigment epithelial cells.

Ulrich Schraermeyer; Jürgen Kopitz; Swaantje Peters; Sigrid Henke-Fahle; Petra Blitgen-Heinecke; Despina Kokkinou; Tobias Schwarz; Karl Ulrich Bartz-Schmidt


Graefes Archive for Clinical and Experimental Ophthalmology | 2005

Zinc uptake and storage: the role of fundus pigmentation.

Despina Kokkinou; Haino Uwe Kasper; Tobias Schwarz; Karl Ulrich Bartz-Schmidt; Ulrich Schraermeyer


Pigment Cell Research | 2004

The pigmentation of human iris influences the uptake and storing of zinc

Despina Kokkinou; Haino Uwe Kasper; Karl Ulrich Bartz-Schmidt; Ulrich Schraermeyer


Metallomics | 2012

A low zinc diet leads to loss of Zn in melanosomes of the RPE but not in melanosomes of the choroidal melanocytes

Antje Biesemeier; Sylvie Julien; Despina Kokkinou; Ulrich Schraermeyer; O. Eibl


Investigative Ophthalmology & Visual Science | 2011

Zinc Deficiency Leads To Lipofuscin Accumulation In The Retinal Pigment Epithelium Of Pigmented Rats

Sylvie Julien; Antje Biesemeier; Despina Kokkinou; Sigrid Schultheiss; Sabine Hofmeister; O. Eibl; Ulrich Schraermeyer


Archive | 2008

Reduction of Oxidative Stress in Retinal Disease

Ulrich Schraermeyer; Petra Blitgen-Heinecke; Despina Kokkinou; Tobias Schwarz; Jürgen Kopitz

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O. Eibl

University of Tübingen

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