TY - JOUR A1 - Abebe, Zeweter A1 - Haki, Gulelat Desse A1 - Schweigert, Florian J. A1 - Henkel, Ina M. A1 - Baye, Kaleab T1 - Low breastmilk vitamin A concentration is prevalent in rural Ethiopia JF - European journal of clinical nutrition N2 - Background There is scant information on the breastmilk vitamin A (BMVA) concentration of lactating women in developing countries, partly due to lack of methods applicable in-field. Objective To assess BMVA concentrations of samples collected from lactating women of children aged 6-23 months, in Mecha district, Ethiopia. Subjects/methods Data on socio-demographic and anthropometric characteristics were collected from randomly selected lactating women (n = 104). Breast milk samples were collected and vitamin A concentrations were analyzed using HPLC and iCheck FLUORO then the two measurements were compared. Results The prevalence of underweight (BMI < 18.5 kg/m(2)) among lactating women was 17%. Seventy six percent of the BMVA values were < 1.05 mu mol/l and 81% were < 8 mu g/g fat. The mean BMVA concentration accounted to 41% of the estimated average value for mothers in developing countries. The BMVA values from HPLC and iCheck were correlated (r = 0.59, p = < 0.001), but it was not strong. Conclusions The result indicates the low vitamin A status of the lactating women and their children. It further indicates that intake assessments should not use average BMVA composition. The possibility of using iCheck for monitoring interventions designed to improve vitamin A status of lactating women with low BMVA requires further investigation. Y1 - 2019 U6 - https://doi.org/10.1038/s41430-018-0334-4 SN - 0954-3007 SN - 1476-5640 VL - 73 IS - 8 SP - 1110 EP - 1116 PB - Nature Publ. Group CY - London ER - TY - JOUR A1 - Abraham, Klaus T1 - Minimal Inflammation, Acute Phase Response and Avoidance of Misclassification of Vitamin A and Iron Status in Infants-Importance of a High-Sensitivity C-Reactive Protein (CRP) Assay Y1 - 2003 ER - TY - THES A1 - Aga-Barfknecht, Heja T1 - Investigation of the phenotype and genetic variant(s) of the diabetes locus Nidd/DBA N2 - Diabetes is a major public health problem with increasing global prevalence. Type 2 diabetes (T2D), which accounts for 90% of all diagnosed cases, is a complex polygenic disease also modulated by epigenetics and lifestyle factors. For the identification of T2D-associated genes, linkage analyses combined with mouse breeding strategies and bioinformatic tools were useful in the past. In a previous study in which a backcross population of the lean and diabetes-prone dilute brown non-agouti (DBA) mouse and the obese and diabetes-susceptible New Zealand obese (NZO) mouse was characterized, a major diabetes quantitative trait locus (QTL) was identified on chromosome 4. The locus was designated non-insulin dependent diabetes from DBA (Nidd/DBA). The aim of this thesis was (i) to perform a detailed phenotypic characterization of the Nidd/DBA mice, (ii) to further narrow the critical region and (iii) to identify the responsible genetic variant(s) of the Nidd/DBA locus. The phenotypic characterization of recombinant congenic mice carrying a 13.6 Mbp Nidd/DBA fragment with 284 genes presented a gradually worsening metabolic phenotype. Nidd/DBA allele carriers exhibited severe hyperglycemia (~19.9 mM) and impaired glucose clearance at 12 weeks of age. Ex vivo perifusion experiments with islets of 13-week-old congenic mice revealed a tendency towards reduced insulin secretion in homozygous DBA mice. In addition, 16-week-old mice showed a severe loss of β-cells and reduced pancreatic insulin content. Pathway analysis of transcriptome data from islets of congenic mice pointed towards a downregulation of cell survival genes. Morphological analysis of pancreatic sections displayed a reduced number of bi-hormonal cells co-expressing glucagon and insulin in homozygous DBA mice, which could indicate a reduced plasticity of endocrine cells in response to hyperglycemic stress. Further generation and phenotyping of recombinant congenic mice enabled the isolation of a 3.3 Mbp fragment that was still able to induce hyperglycemia and contained 61 genes. Bioinformatic analyses including haplotype mapping, sequence and transcriptome analysis were integrated in order to further reduce the number of candidate genes and to identify the presumable causative gene variant. Four putative candidate genes (Ttc39a, Kti12, Osbpl9, Calr4) were defined, which were either differentially expressed or carried a sequence variant. In addition, in silico ChIP-Seq analyses of the 3.3 Mbp region indicated a high number of SNPs located in active regions of binding sites of β-cell transcription factors. This points towards potentially altered cis-regulatory elements that could be responsible for the phenotype conferred by the Nidd/DBA locus. In summary, the Nidd/DBA locus mediates impaired glucose homeostasis and reduced insulin secretion capacity which finally leads to β-cell death. The downregulation of cell survival genes and reduced plasticity of endocrine cells could further contribute to the β-cell loss. The critical region was narrowed down to a 3.3 Mbp fragment containing 61 genes, of which four might be involved in the development of the diabetogenic Nidd/DBA phenotype. N2 - Die Diabetesprävalenz nimmt seit Jahren weltweit zu, wobei etwa 90% der diagnostizierten Diabeteserkrankungen einem Typ-2-Diabetes (T2D) zuzuordnen sind. T2D ist eine komplexe polygene Stoffwechselerkrankung, die auch durch epigenetische Faktoren und den Lebensstil beeinflusst wird. Die Identifizierung und Untersuchung von Diabetes-assoziierten Genen wird unter anderem durch Kopplungsanalysen und darauf aufbauende zuchtstrategische und bioinformatische Analysen ermöglicht. In einer vorangegangenen Studie wurde der schlanke, Diabetes-anfällige dilute brown non-agouti (DBA)-Mausstamm mit der adipösen und ebenfalls Diabetes-suszeptiblen New Zealand obese (NZO)-Maus verpaart und die erste Rückkreuzungsgeneration einer Kopplungsanalyse unterzogen. Hierbei wurde ein hoch signifikanter quantitative trait locus (QTL) für Diabetes auf Chromosom 4 nachgewiesen. Dieser Locus ist mit erhöhten Blutzuckerwerten, reduzierten Plasmainsulinkonzentrationen und einem niedrigen pankreatischen Insulingehalt assoziiert und wurde als Nidd/DBA (engl. für nicht insulinabhängiger Diabetes von DBA-Allelen) bezeichnet. Das Ziel der vorliegenden Arbeit war es, (i) das kritische Fragment des Nidd/DBA-Locus‘ zu verkleinern, (ii) die phänotypische Ausprägung des Nidd/DBA-Locus‘ zu untersuchen sowie (iii) die ursächliche(n) genetische(n) Variante(n) zu identifizieren. Die phänotypische Charakterisierung von kongenen Mäusen mit einem kritischen Fragment von 13.6 Mbp, welches 284 Gene enthält, zeigte bereits im Alter von 12 Wochen eine starke Hyperglykämie (~19.9 mM) und eine unzureichende Glucose-Clearance bei Nidd/DBA-Allelträgern. Ex-vivo Perifusionsversuche mit isolierten Inseln von 13 Wochen alten kongenen Mäusen zeigten eine tendenziell reduzierte Insulinsekretion in homozygoten DBA-Allelträgern. Im Alter von 16 Wochen wiesen die Tiere einen erheblichen Verlust der β-Zellen, sowie eine Abnahme der pankreatischen Insulinkonzentration auf. Transkriptomdaten der Langerhans-Inseln mit anschließender Signalweganalyse deuteten darauf hin, dass Nidd/DBA-Allelträger eine verminderte Expression von Genen aufzeigen, die für das Überleben von Zellen essentiell sind. In homozygoten DBA-Allelträgern wurde eine reduzierte Anzahl von Glucagon/Insulin-bi-hormonellen Zellen nachgewiesen, was auf eine verminderte Plastizität der endokrinen Zellen hinweisen könnte. Die Zucht weiterer kongener Mäuse und ihre Phänotypisierung ermöglichten die Isolierung eines 3.3 Mbp großen Fragments, das 61 Gene enthielt und eine Hyperglykämie auslöste. Bioinformatische Analysen, wie die Kartierung von Haplotypen und Datenbank-, Sequenz- sowie Transkriptomanalysen, wurden integriert, um die Anzahl der Kandidatengene weiter zu reduzieren und die Hyperglykämie auslösende(n) Genvariante(n) zu identifizieren. Es konnten vier potentielle Kandidatengene (Ttc39a, Osbpl9, Kti12, Calr4) definiert werden, die entweder eine differenzielle Expression oder eine Sequenzvariante aufwiesen. Mit Hilfe von in-silico-Analysen von ChIP-Seq-Daten wurden SNPs in aktiven Bindungsstellen von β-Zell-Transkriptionsfaktoren identifiziert. Diese könnten cis-regulatorische Elemente darstellen, die Gene außerhalb dieses 3.3 Mbp großen Fragments beeinflussen und möglichweise für den Phänotyp verantwortlich sind. Zusammenfassend konnte gezeigt werden, dass der Nidd/DBA-Locus für eine beeinträchtigte Glucosehomöostase und eine Verschlechterung der Insulinsekretion verantwortlich ist, welche langfristig zum Verlust von β-Zellen führen. Die bisherigen Ergebnisse deuten darauf hin, dass sowohl die verringerte Expression der für das Zellüberleben essentiellen Gene als auch eine verringerte Plastizität der endokrinen Zellen zum Untergang von Langerhans-Inseln beitragen. Das kritische Fragment wurde auf eine Größe von 3.3 Mbp mit 61 Genen reduziert, von denen vier Gene als verantwortliche Kandidaten für den beschriebenen Nidd/DBA-Phänotyp bedeutsam sein können KW - Diabetes KW - Genetics KW - Glucose intolerance KW - Insulin secretion KW - Susceptibility-genes KW - Diabetes KW - Genetik KW - Glukoseintoleranz KW - Insulinsekretion KW - Suszeptibilitätsgene Y1 - 2021 ER - TY - JOUR A1 - Aga-Barfknecht, Heja A1 - Hallahan, Nicole A1 - Gottmann, Pascal A1 - Jähnert, Markus A1 - Osburg, Sophie A1 - Schulze, Gunnar A1 - Kamitz, Anne A1 - Arends, Danny A1 - Brockmann, Gudrun A1 - Schallschmidt, Tanja A1 - Lebek, Sandra A1 - Chadt, Alexandra A1 - Al-Hasani, Hadi A1 - Joost, Hans-Georg A1 - Schürmann, Annette A1 - Vogel, Heike T1 - Identification of novel potential type 2 diabetes genes mediating beta-cell loss and hyperglycemia using positional cloning JF - Frontiers in genetics N2 - Type 2 diabetes (T2D) is a complex metabolic disease regulated by an interaction of genetic predisposition and environmental factors. To understand the genetic contribution in the development of diabetes, mice varying in their disease susceptibility were crossed with the obese and diabetes-prone New Zealand obese (NZO) mouse. Subsequent whole-genome sequence scans revealed one major quantitative trait loci (QTL),Nidd/DBAon chromosome 4, linked to elevated blood glucose and reduced plasma insulin and low levels of pancreatic insulin. Phenotypical characterization of congenic mice carrying 13.6 Mbp of the critical fragment of DBA mice displayed severe hyperglycemia and impaired glucose clearance at week 10, decreased glucose response in week 13, and loss of beta-cells and pancreatic insulin in week 16. To identify the responsible gene variant(s), further congenic mice were generated and phenotyped, which resulted in a fragment of 3.3 Mbp that was sufficient to induce hyperglycemia. By combining transcriptome analysis and haplotype mapping, the number of putative responsible variant(s) was narrowed from initial 284 to 18 genes, including gene models and non-coding RNAs. Consideration of haplotype blocks reduced the number of candidate genes to four (Kti12,Osbpl9,Ttc39a, andCalr4) as potential T2D candidates as they display a differential expression in pancreatic islets and/or sequence variation. In conclusion, the integration of comparative analysis of multiple inbred populations such as haplotype mapping, transcriptomics, and sequence data substantially improved the mapping resolution of the diabetes QTLNidd/DBA. Future studies are necessary to understand the exact role of the different candidates in beta-cell function and their contribution in maintaining glycemic control. KW - type 2 diabetes KW - beta-cell loss KW - insulin KW - positional cloning KW - transcriptomics KW - haplotype Y1 - 2020 U6 - https://doi.org/10.3389/fgene.2020.567191 SN - 1664-8021 VL - 11 PB - Frontiers Media CY - Lausanne ER - TY - JOUR A1 - Aga-Barfknecht, Heja A1 - Soultoukis, George A. A1 - Stadion, Mandy A1 - Garcia-Carrizo, Francisco A1 - Jähnert, Markus A1 - Gottmann, Pascal A1 - Vogel, Heike A1 - Schulz, Tim Julius A1 - Schürmann, Annette T1 - Distinct adipogenic and fibrogenic differentiation capacities of mesenchymal stromal cells from pancreas and white adipose tissue JF - International journal of molecular sciences N2 - Pancreatic steatosis associates with beta-cell failure and may participate in the development of type-2-diabetes. Our previous studies have shown that diabetes-susceptible mice accumulate more adipocytes in the pancreas than diabetes-resistant mice. In addition, we have demonstrated that the co-culture of pancreatic islets and adipocytes affect insulin secretion. The aim of this current study was to elucidate if and to what extent pancreas-resident mesenchymal stromal cells (MSCs) with adipogenic progenitor potential differ from the corresponding stromal-type cells of the inguinal white adipose tissue (iWAT). miRNA (miRNome) and mRNA expression (transcriptome) analyses of MSCs isolated by flow cytometry of both tissues revealed 121 differentially expressed miRNAs and 1227 differentially expressed genes (DEGs). Target prediction analysis estimated 510 DEGs to be regulated by 58 differentially expressed miRNAs. Pathway analyses of DEGs and miRNA target genes showed unique transcriptional and miRNA signatures in pancreas (pMSCs) and iWAT MSCs (iwatMSCs), for instance fibrogenic and adipogenic differentiation, respectively. Accordingly, iwatMSCs revealed a higher adipogenic lineage commitment, whereas pMSCs showed an elevated fibrogenesis. As a low degree of adipogenesis was also observed in pMSCs of diabetes-susceptible mice, we conclude that the development of pancreatic steatosis has to be induced by other factors not related to cell-autonomous transcriptomic changes and miRNA-based signals. KW - MSCs KW - fatty pancreas KW - WAT KW - lineage commitment KW - transcriptomics KW - miRNAs Y1 - 2022 U6 - https://doi.org/10.3390/ijms23042108 SN - 1422-0067 VL - 23 IS - 4 PB - Molecular Diversity Preservation International CY - Basel ER - TY - JOUR A1 - Ahlberg, Sebastian A1 - Rancan, Fiorenza A1 - Epple, Matthias A1 - Loza, Kateryna A1 - Höppe, David A1 - Lademann, Jürgen A1 - Vogt, Annika A1 - Kleuser, Burkhard A1 - Gerecke, Christian A1 - Meinke, Martina C. T1 - Comparison of different methods to study effects of silver nanoparticles on the pro- and antioxidant status of human keratinocytes and fibroblasts JF - Methods : focusing on rapidly developing techniques KW - Oxidative stress KW - Dichlorofluorescein assay KW - Electron paramagnetic resonance spectroscopy KW - HaCaT cells KW - Glutathione KW - Free radicals Y1 - 2016 U6 - https://doi.org/10.1016/j.ymeth.2016.05.015 SN - 1046-2023 SN - 1095-9130 VL - 109 SP - 55 EP - 63 PB - Elsevier CY - San Diego ER - TY - JOUR A1 - Al Fadel, Frdoos A1 - Fayyaz, Susann A1 - Japtok, Lukasz A1 - Kleuser, Burkhard T1 - Involvement of Sphingosine 1-Phosphate in Palmitate-Induced Non-Alcoholic Fatty Liver Disease JF - Cellular physiology and biochemistry : international journal of experimental cellular physiology, biochemistry and pharmacology N2 - Background/Aims: Ectopic lipid accumulation in hepatocytes has been identified as a risk factor for the progression of liver fibrosis and is strongly associated with obesity. In particular, the saturated fatty acid palmitate is involved in initiation of liver fibrosis via formation of secondary metabolites by hepatocytes that in turn activate hepatic stellate cells (HSCs) in a paracrine manner Methods: a-smooth muscle actin-expression (alpha-SMA) as a marker of liver fibrosis was investigated via western blot analysis and immunofluorescence microscopy in HSCs (LX-2). Sphingolipid metabolism and the generation of the bioactive secondary metabolite sphingosine I-phosphate (SIP) in response to palmitate were analyzed by LC-MS/MS in hepatocytes (HepG2). To identify the molecular mechanism involved in the progression of liver fibrosis real-time PCR analysis and pharmacological modulation of SIP receptors were performed. Results: Palmitate oversupply increased intra- and extracellular SIP-concentrations in hepatocytes. Conditioned medium from HepG2 cells initiated fibrosis by enhancing alpha-SMA-expression in LX-2 in a S1P-dependent manner In accordance, fibrotic response in the presence of SIP was also observed in HSCs. Pharmacological inhibition of SIP receptors demonstrated that S1P(3) is the crucial receptor subtype involved in this process. Conclusion: SIP is synthesized in hepatocytes in response to palmitate and released into the extracellular environment leading to an activation of HSCs via the S1P(3) receptor (C) 2016 The Author(s) Published by S. Karger AG, Basel KW - Palmitate KW - Liver fibrosis KW - Sphingosine 1-phosphate KW - Hepatic stellate cells KW - Hepatocytes KW - alpha-SMA Y1 - 2016 U6 - https://doi.org/10.1159/000453213 SN - 1015-8987 SN - 1421-9778 VL - 40 SP - 1637 EP - 1645 PB - Karger CY - Basel ER - TY - THES A1 - Aleksandrova, Krasimira T1 - Understanding the link between obesity and colorectal cancer BT - the role of biomarkers of iflammation, immunity and metabolic dysfunction Y1 - 2020 ER - TY - THES A1 - Alfine, Eugenia T1 - Investigation of Sirtuin 3 overexpression as a genetic model of fasting in hypothalamic neurons Y1 - 2021 ER - TY - GEN A1 - Alker, Wiebke A1 - Schwerdtle, Tanja A1 - Schomburg, Lutz A1 - Haase, Hajo T1 - A Zinpyr-1-based fluorimetric microassay for free zinc in human serum T2 - Postprints der Universität Potsdam : Mathematisch-Naturwissenschaftliche Reihe N2 - Zinc is an essential trace element, making it crucial to have a reliable biomarker for evaluating an individual’s zinc status. The total serum zinc concentration, which is presently the most commonly used biomarker, is not ideal for this purpose, but a superior alternative is still missing. The free zinc concentration, which describes the fraction of zinc that is only loosely bound and easily exchangeable, has been proposed for this purpose, as it reflects the highly bioavailable part of serum zinc. This report presents a fluorescence-based method for determining the free zinc concentration in human serum samples, using the fluorescent probe Zinpyr-1. The assay has been applied on 154 commercially obtained human serum samples. Measured free zinc concentrations ranged from 0.09 to 0.42 nM with a mean of 0.22 ± 0.05 nM. It did not correlate with age or the total serum concentrations of zinc, manganese, iron or selenium. A negative correlation between the concentration of free zinc and total copper has been seen for sera from females. In addition, the free zinc concentration in sera from females (0.21 ± 0.05 nM) was significantly lower than in males (0.23 ± 0.06 nM). The assay uses a sample volume of less than 10 µL, is rapid and cost-effective and allows us to address questions regarding factors influencing the free serum zinc concentration, its connection with the body’s zinc status, and its suitability as a future biomarker for an individual’s zinc status. T3 - Zweitveröffentlichungen der Universität Potsdam : Mathematisch-Naturwissenschaftliche Reihe - 1086 KW - zinc KW - free zinc KW - serum KW - biomarker KW - fluorescent probe KW - Zinypr-1 Y1 - 2021 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:kobv:517-opus4-472833 SN - 1866-8372 IS - 1086 ER - TY - JOUR A1 - Alter, Markus L. A1 - Kretschmer, Axel A1 - Von Websky, Karoline A1 - Tsuprykov, Oleg A1 - Reichetzeder, Christoph A1 - Simon, Alexandra A1 - Stasch, Johannes-Peter A1 - Hocher, Berthold T1 - Early urinary and plasma biomarkers for experimental diabetic Nephropathy JF - Clinical laboratory : the peer reviewed journal for clinical laboratories and laboratories related to blood transfusion N2 - Background: As the prevalence of diabetes rises, its complications such as diabetic nephropathy affect an increaseing number of patients. Consequently, the need for biomarkers in rodent models which reflect the stage and course of diabetic nephropathy is high. This article focuses on Heart-type fatty acid binding protein (H-FABP), osteopontin (OPN), nephrin, and Neutrophil gelatinase-associated lipocalin (NGAL) in urine, and kidney injury molecule (KIM)-1, clusterin, and tissue inhibitior of metalloproteinases (TIMP) 1 in plasma in uni-nephrectomized rats with streptocotozin-induced type 1 diabetes mellitus, a common animal model to explore renal impairment in the setting of diabetes mellitus. Methods: 23 male Wistar rats were uni-nephrectomized and subsequently divided into two study groups. The diabetic group received streptozotocin (STZ) via tail-vein injection, the non-diabetic group received citrate buffer without STZ. Subsequently, blood glucose, body weight, and blood pressure were checked regularly. After 18 weeks, animals were placed in metabolic cages, blood and urine obtained and subsequently organs were harvested after sacrifice. Results: Blood glucose levels were highly increased in diabetic animals throughout the experiment, whereas systolic blood pressure did not differ between the study groups. At study end, classical biomarkers such as urinary albumin and protein and plasma cystatin c were only slightly but not significantly different between groups indicating a very early disease state. In contrast, urinary excretion of H-FABP, OPN, nephrin, and NGAL were highly increased in diabetic animals with a highly significant p-value (p<0.01 each) compared to non-diabetic animals. In plasma, differences were found for calbindin, KIM-1, clusterin, TIMP-1, and OPN. These findings were confirmed by means of the area under the receiver operating characteristic curve (ROC-AUC) analysis. Conclusions: In summary, our study revealed elevated levels of new plasma and urinary biomarkers (urinary osteopontin, urinary nephrin, urinary NGAL, urinary H-FABP, plasma KIM-1, plasma TIMP-1) in uni-nephrectomized diabetic rats, an established rat model of diabetic nephropathy. These biomarkers appeared even before the classical biomarkers of diabetic nephropathy such as albuminuria and urinary protein excretion. The new biomarkers might offer advantage to urinary albumin and plasma cystatin c with respect to early detection. KW - diabetic nephropathy KW - urinary biomarker KW - blood biomarker KW - heart-type fatty acid binding protein KW - osteopontin KW - nephrin KW - neutrophil gelatinase-associated lipocalin KW - kidney injury molecule 1 KW - clusterin KW - tissue inhibitior of metalloproteinases 1 Y1 - 2012 U6 - https://doi.org/10.7754/Clin.Lab.2011.111010 SN - 1433-6510 VL - 58 IS - 7-8 SP - 659 EP - 671 PB - Clin Lab Publ., Verl. Klinisches Labor CY - Heidelberg ER - TY - JOUR A1 - Alter, Markus L. A1 - Ott, Ina M. A1 - von Websky, Karoline A1 - Tsuprykov, Oleg A1 - Sharkovska, Yuliya A1 - Krause-Relle, Katharina A1 - Raila, Jens A1 - Henze, Andrea A1 - Klein, Thomas A1 - Hocher, Berthold T1 - DPP-4 Inhibition on top of angiotensin receptor blockade offers a new therapeutic approach for diabetic nephropathy JF - Kidney & blood pressure research : official organ of the Gesellschaft für Nephrologie N2 - Background: The need for an improved treatment for diabetic nephropathy is greatest in patients who do not adequately respond to angiotensin II receptor blockers (ARBs). This study investigated the effect of the novel dipeptidyl peptidase-4 inhibitor linagliptin alone and in combination with the ARB telmisartan on the progression of diabetic nephropathy in diabetic endothelial nitric oxide synthase (eNOS) knockout mice. Methods: Sixty male eNOS knockout C57BL/6J mice were divided into four groups after receiving intraperitoneal high-dose streptozotocin: telmisartan (1 mg/kg), linagliptin (3 mg/kg), linagliptin + telmisartan (3 mg/kg + 1 mg/kg) and vehicle. Fourteen mice were used as non-diabetic controls. Results: After 12 weeks, urine and blood were obtained and blood pressure measured. Glucose concentrations were increased and similar in all diabetic groups. Telmisartan alone reduced systolic blood pressure by 5.9 mmHg versus diabetic controls (111.2 +/- 2.3 mmHg vs 117.1 +/- 2.2 mmHg; mean +/- SEM; P = 0.071). Combined treatment significantly reduced albuminuria compared with diabetic controls (71.7 +/- 15.3 mu g/24 h vs 170.8 +/- 34.2 mu g/24 h; P = 0.017), whereas the effects of single treatment with either telmisartan (97.8 +/- 26.4 mu g/24 h) or linagliptin (120.8 +/- 37.7 mu g/24 h) were not statistically significant. DPP-4 inhibition, alone and in combination, led to significantly lower plasma osteopontin levels compared with telmisartan alone. Histological analysis revealed reduced glomerulosclerosis after Linagliptin alone and in combination with telmisartan in comparison to non treated diabetic animals (p < 0.01 and p < 0.05). Kidney malonaldehyde immune-reactivity, a marker of oxidative stress, was significantly lower in animals treated with linagliptin. Conclusions: DPP-4 inhibition on top of ARB treatment significantly reduced urinary albumin excretion and oxidative stress in diabetic eNOS knockout mice. Linagliptin on top of an angiotensin II receptor blocker may offer a new therapeutic approach for patients with diabetic nephropathy. KW - Diabetic nephropathy KW - DPP-4 inhibitor KW - Linagliptin KW - Renin-angiotensin system Y1 - 2012 U6 - https://doi.org/10.1159/000341487 SN - 1420-4096 VL - 36 IS - 1 SP - 119 EP - 130 PB - Karger CY - Basel ER - TY - THES A1 - Ambrosi, Thomas H. T1 - The Role of Bone-residing Adipocyte Progenitors in Age-related Stem Cell Dysfunction and Regenerative Processes Y1 - 2016 ER - TY - JOUR A1 - Andert, Christoph U. A1 - Sanchaisuriya, Pattara A1 - Sanchaisuriya, Kanokwan A1 - Schelp, Frank P. A1 - Schweigert, Florian J. T1 - Nutritional status of pregnant women in Northeast Thailand N2 - A comparative study on the nutritional status of primiparous and multiparous women in the first trimester of pregnancy was conducted in the northeastern province of Thailand, Khon Kaen, to investigate differences in protein- energy-mal nutrition, iron deficiency anaemia, vitamin A deficiency and carotenoid status between both parity groups. 94 subjects were recruited at first attendance of antenatal clinic. Data about weight, height, haemoglobin and haematocrit were obtained from hospital records. Anthropometric measurements of mid-upper arm circumference and triceps skinfold were done on a sub sample. Retinol, carotenoids and alpha-tocopherol were analysed using a reversed-phase high- performance liquid chromatography method. Ferritin, transthyretin and retinol-binding protein were determined by enzyme- linked immunosorbent assay. Primiparous women showed lower body mass index, mid-upper arm circumference, corrected arm muscle area (P <0.001) as well as lower retinol, cholesterol and triceps skinfold (P <0.05). After adjusting for age and socio-economical status the significant difference persisted for all parameters but triceps skinfold. No significant differences of alpha-tocopherol, serum proteins, carotenoids and iron indices could be observed, even though a tendency to higher values for ferritin, haemoglobin and haematocrit was shown in multiparous women. Prevalence of protein-energy- malnutrition (body mass index <18.5 kg/m(2)) in the primiparous group was significantly higher compared to the multiparous group (P<0.05). Prevalence of protein-energy-malnutrition, iron deficiency anaemia and vitamin A deficiency were 15.1%, 6.3% and 3.3%, respectively, in the total study population. No differences between parity groups could be observed for prevalence of iron deficiency anaemia and vitamin A deficiency Y1 - 2006 UR - http://www.healthyeatingclub.com/APJCN/ SN - 0964-7058 ER - TY - JOUR A1 - Anger, Horst A1 - Walzel, Erwin A1 - Kahrmann, Bettina T1 - About the absorption of oligogalacturonates from the caecum of rats Y1 - 1994 ER - TY - THES A1 - Appl, Thomas T1 - Neurochemical and functional characterisation of the Melanin-concentrating hormone system in the rat brain T1 - Neurochemische und funktionelle Charakterisierung des Melanin-konzentrierenden Hormone Systems im Rattenhirn N2 - The central melanin-concentrating hormone (MCH) system has been intensively studied for its involvement in the regulation of feeding behaviour and body weight regulation. The importance of the neuropeptide MCH in the control of energy balance has been underlined by MCH knock out and Melanin-concentrating hormone receptor subtype 1 (MCHR-1) knock-out animals. The anorectic and anti-obesity effects of selective MCHR-1 antagonists have confirmed the notion that pharmacological blockade of MCHR-1 is a potential therapeutic approach for obesity. First aim of this work is to study the neurochemical “equipment” of MCHR-1 immunoreactive neurons by double-labelling immunohistochemistry within the rat hypothalamus. Of special interest is the neuroanatomical identification of other hypothalamic neuropeptides that are co-distributed with MCHR-1. A second part of this study deals with the examination of neuronal activation patterns after pharmacological or physiological, feeding-related stimuli and was introduced to further understand central regulatory mechanisms of the MCH system. In the first part of work, I wanted to neurochemically characterize MCHR-1 immunoreactive neurons in the rat hypothalamus for colocalisation with neuropeptides of interest. Therefore I performed an immunohistochemical colocalisation study using a specific antibody against MCHR-1 in combination with antibodies against hypothalamic neuropeptides. I showed that MCHR-1 immunoreactivity (IR) was co-localised with orexin A in the lateral hypothalamus, and with adrenocorticotropic hormone and neuropeptide Y in the arcuate nucleus. Additionally, MCHR-1 IR was co-localised with the neuropeptides vasopressin and oxytocin in magnocellular neurons of the supraoptic and paraventricular hypothalamic nucleus and corticotrophin releasing hormone in the parvocellular division of the paraventricular hypothalamic nucleus. Moreover, for the first time MCHR-1 immunoreactivity was found in both the adenohypophyseal and neurohypophyseal part of the rat pituitary. These results provide the neurochemical basis for previously described potential physiological actions of MCH at its target receptor. In particular, the MCHR-1 may be involved not only in food intake regulation, but also in other physiological actions such as fluid regulation, reproduction and stress response, possibly through here examined neuropeptides. Central activation patterns induced by pharmacological or physiological stimulation can be mapped using c-Fos immunohistochemistry. In the first experimental design, central administration (icv) of MCH in the rat brain resulted in acute and significant increase of food and water intake, but this animal treatment did not induce a specific c-Fos induction pattern in hypothalamic nuclei. In contrast, sub-chronic application of MCHR-1 antagonist promoted a significant decrease in food- and water intake during an eight day treatment period. A qualitative analysis of c-Fos immunohistochemistry of sections derived from MCHR-1 antagonist treated animals showed a specific neuronal activation in the paraventricular nucleus, the supraoptic nucleus and the dorsomedial hypothalamus. These results could be substantiated by quantitative evaluation of an automated, software-supported analysis of the c-Fos signal. Additionally, I examined the activation pattern of rats in a restricted feeding schedule (RFS) to identify pathways involved in hunger and satiety. Animals were trained for 9 days to feed during a three hour period. On the last day, food restricted animals was also allowed to feed for the three hours, while food deprived (FD) animals did not receive food. Mapping of neuronal activation showed a clear difference between stareved (FD) and satiated (FR) rats. FD animals showed significant induction of c-Fos in forebrain regions, several hypothalamic nuclei, amygdaloid thalamus and FR animals in the supraoptic nucleus and the paraventricular nucleus of the hypothalamus, and the nucleus of the solitary tract. In the lateral hypothalamus of FD rats, c-Fos IR showed strong colocalisation for Orexin A, but no co-staining for MCH immunoreactivity. However, a large number of c-Fos IR neurons within activated regions of FD and FR animals was co-localised with MCHR-1 within selected regions. To conclude, the experimental set-up of scheduled feeding can be used to induce a specific hunger or satiety activation pattern within the rat brain. My results show a differential activation by hunger signals of MCH neurons and furthermore, demonstrates that MCHR-1 expressing neurons may be essential parts of downstream processing of physiological feeding/hunger stimuli. In the final part of my work, the relevance of here presented studies is discussed with respect to possible introduction of MCHR-1 antagonists as drug candidates for the treatment of obesity. N2 - Die Regulation des Körpergewichts in einem physiologischen Rahmen setzt ein internes Energiegleichgewicht voraus und wird langfristig durch Abgleich von Nahrungsaufnahme einerseits und Energieverbrauch andererseits gewährleistet. Dieses Gleichgewicht ist bei massivem Übergewicht (Adipositas) oder chronischem Untergewicht (Kachexie) dauerhaft gestört. Bei der Regulation des Energiegleichgewichts spielt der im Zwischenhirn gelegene Hypothalamus als Schaltstation eine wichtige Rolle. Hypothalamische Regelkreise gleichen sensorische, viszerale und humorale Signale miteinander ab und setzen sie in adäquates Verhalten (z.B. Nahrungsaufnahme) um. Innerhalb des Hypothalamus werden Hunger und Sättigung durch zentralnervöse Regulationssysteme kodiert. Dadurch stellt eine pharmakologische Inhibierung eines hunger-stimulierenden (orexigenen), hypothalamischen Regelkreises eine Möglichkeit dar, um Nahrungsaufnahme und Körpergewichts zu reduzieren. Das im lateralen Hypothalamus gebildete Neuropeptid Melanin-konzentrierendes Hormon (MCH) ist ein solches orexigenes Signal. In unterschiedlichen Tiermodellen wurde gezeigt, dass MCH seine physiologischen Effekte auf das Energiegleichgewicht durch den funktionellen MCH Rezeptor Subtyp 1 (MCHR-1) vermittelt. Die Behandlung von Labornagern mit selektiv wirksamen MCHR-1 Antagonisten hat in verschiedenen Tiermodellen zu einer Verminderung der Nahrungsaufnahme und Körpergewichtsreduktion geführt (anorexigene Wirkung). Das Ziel dieser Arbeit ist eine vertiefte Untersuchung des zentralen MCH Systems. Im ersten Teil der Arbeit werden MCHR-1 enthaltene Nervenzellen (Neurone) im Hypothalamus von Ratten immunhistochemisch identifiziert und neurochemisch charakterisiert. Dieser Teil der Arbeit soll mit Hilfe von Kolokalisationsstudien mögliche Interaktionen des MCH Systems mit anderen neuropeptidergen, hypothalamischen Systemen identifizieren. Der zweite Teil der Arbeit befasst sich mit der Untersuchung von pharmakologischen Effekten bei MCH und MCHR-1 Antagonist behandelten Ratten auf Nahrungsaufnahme, Wasseraufnahme sowie Veränderung des Körpergewichts. Zentrale Regulationsmechanismen wurden durch den immunhistochemischen Nachweis des Transkriptionsfaktors und neuronalen Aktivierungsmarkers c-Fos im Rattenhirn ermittelt. Diese neuronalen Aktivierungsmuster wurden mit solchen Mustern verglichen, die nach einem definierten physiologischen Stimulus (Fütterungsregime) mit derselben Methode aufgezeichnet wurden. Erste Ergebnisse zeigten, dass der hier etablierte Antikörper gegen MCHR-1 spezifisch ist und MCHR-1 in mehreren hypothalamischen Kernarealen mit Hilfe dieses Antikörpers nachgewiesen werden konnte. So konnte im lateralen Hypothalamus eine Kolokalisation von MCHR-1 mit Orexin A nachgewiesen werden, im arcuate Nukleus des Hypothalamus, einem Kernareal, das eine bedeutende Funktion in der Integration von Hunger- und Sättigungssignalen hat, zeigten MCHR-1 positive Neurone eine Kolokalisation mit dem orexigenen Neuropeptid Y oder mit dem Adrenocorticotrophin Hormon, einem Marker für das anorexigen wirkende, zentrale Melanokortin System. Der Paraventrikuläre Nukleus und der Supraoptische Nukleus des Hypothalamus spielen eine wichtige Rolle in neuroendokrinen Regulationen. Im paraventrikulären Hypothalamus konnte eine Kolokalisation von MCHR-1 mit den Neuropeptiden Vasopressin, Oxytocin und Corticotrophin-releasing Hormon festgestellt werden, außerdem konnte eine Kolokalisierung von MCHR-1 mit Vasopressin und Oxytocin im Supraoptischen Nukleus gezeigt werden. Zusätzlich konnte MCHR-1 immunhistochemisch auf Zellen der Adeno- und der Neurohypophyse nachgewiesen werden. Diese Ergebnisse lassen auf eine Interaktion von MCHR-1 im Hypothalamus nicht nur mit orexigenen (Orexin A und Neuropeptid Y) und anorexigenen (Adrenocorticotrophin Hormon) Signalen schließen, sondern weisen zusätzlich auf eine Rolle von MCHR-1 bei der Regulation des Wasserhaushalts (Vasopressin), der Fortpflanzung (Oxytocin) und bei Stress (Corticotrophin-releasing Hormon) hin. Im zweiten Versuchsvorhaben führte die zentraler Gabe (intrazerebroventrikular) von MCH ins Rattengehirn zu einer akuten und signifikanten Steigerung der Futter- und Wasseraufnahme, es konnte jedoch kein spezifisches Aktivierungsmuster in hypothalamischen Kernarealen (Nuklei) definiert werden. Im Gegensatz dazu führte eine sub-chronische Gabe eines oral verfügbaren MCHR-1 Antagonisten in Ratten zu einer signifikanten Verminderung der Nahrungs-, Wasseraufnahme und des Körpergewichts. Bei qualitativer Analyse des immunhistochemischen Signals für c-Fos bei MCHR-1 Antagonist behandelten Ratten konnte eine spezifische Aktivierung im Paraventrikulären Hypothalamus, im Supraoptischen Nukleus und im Dorsomedialen Hypothalamus gezeigt werden. Diese Ergebnisse ließen sich durch automatisierte, software-unterstützte Quantifizierung des c-Fos Signals bestätigen und heben diese Hirnareale als mögliche neuroanatomische Substrate von MCHR-1 Antagonisten hervor. Um eine mögliche neuronale Aktivierung des MCH Systems nach einem physiologischen Stimulus, hier Hunger oder Sättigung, zu untersuchen, wurden in einem weiteren Versuchsansatz Ratten in einem angepassten, neun Tage dauernden Fütterungsregime, täglich für nur drei Stunden Zugang zu Futter gewährt. Tiere, die am letzten Tag des Fütterungsregimes im 3 Stunden Zeitraum kein Futter bekamen und so als „Hunger-Stimulierte“ definiert wurden, zeigten eine signifikante Induktion von c-Fos in unterschiedlichen hypothalamischen (arcuate Nukleus, Dorsomedial Hypothalamischen Nuklei, Lateral Hypothalamus) und extrahypothalamischen Hirnarealen (Nukleus Accumbens, Basolaterale Amygdala, Paraventriculärer Thalamischer Nukleus). Dieses Aktivierungsmuster unterschied sich von Ratten, die am letzten Tag des Fütterungsregims Futter erhalten hatten, den „gesättigte Tieren“ (Aktivierung vor allem im supraoptischen Nukleus, im paraventrikulären Hypothalamus und Nukleus Tractus Solitarius), oder ad libitum gefütterten Kontrolltieren. Um durch das Fütterungsregime aktivierte Neurone dem MCH System zuzuordnen, wurden immunhistochemische Kolokalisationsexperimente von c-Fos mit MCH beziehungsweise MCHR-1 spezifischen Antikörpern durchgeführt. Zwar konnte keine Kolokalisation von c-Fos mit MCH im lateralen Hypothalamus nachgewiesen werden, aber eine Vielzahl von durch Hunger oder Sättigung aktivierte, c-Fos positive Neurone zeigte MCHR-1 Immunoreaktivität. Zusammenfassend lässt sich daraus schließen, dass Nahrungskarenz differenziert unterschiedliche intra-hypothalamische und extra-hypothalamische Zielstrukturen aktiviert. Die funktionelle Rolle des MCHR-1 in solch aktivierten Neuronen bedarf weiterer Klärung. Im abschließenden Teil der Arbeit wird eine mögliche Relevanz der hier beschriebenen Ergebnisse im Hinblick auf die Entwicklung von MCHR-1 Antagonisten und deren möglicher Einsatz bei Adipositas, diskutiert. KW - Ratte KW - Immunhistochemie KW - Kolokalisation KW - MCHR-1 KW - Neuropeptides KW - c-Fos KW - rat KW - immunohistochemistry KW - colocalisation study KW - MCHR-1 KW - neuropeptides KW - c-Fos Y1 - 2007 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:kobv:517-opus-14604 ER - TY - JOUR A1 - Aschner, Michael A. A1 - Palinski, Catherine A1 - Sperling, Michael A1 - Karst, U. A1 - Schwerdtle, Tanja A1 - Bornhorst, Julia T1 - Imaging metals in Caenorhabditis elegans JF - Metallomics : integrated biometal science N2 - Systemic trafficking and storage of essential metal ions play fundamental roles in living organisms by serving as essential cofactors in various cellular processes. Thereby metal quantification and localization are critical steps in understanding metal homeostasis, and how their dyshomeostasis might contribute to disease etiology and the ensuing pathologies. Furthermore, the amount and distribution of metals in organisms can provide insight into their underlying mechanisms of toxicity and toxicokinetics. While in vivo studies on metal imaging in mammalian experimental animals are complex, time- and resource-consuming, the nematode Caenorhabditis elegans (C. elegans) provides a suitable comparative and complementary model system. Expressing homologous genes to those inherent to mammals, including those that regulate metal homeostasis and transport, C. elegans has become a powerful tool to study metal homeostasis and toxicity. A number of recent technical advances have been made in the development and application of analytical methods to visualize metal ions in C. elegans. Here, we briefly summarize key findings and challenges of the three main techniques and their application to the nematode, namely sensing fluorophores, microbeam synchrotron radiation X-ray fluorescence as well as laser ablation ( LA) coupled to inductively coupled plasma-mass spectrometry (ICP-MS). Y1 - 2017 U6 - https://doi.org/10.1039/c6mt00265j SN - 1756-5901 SN - 1756-591X VL - 9 SP - 357 EP - 364 PB - Royal Society of Chemistry CY - Cambridge ER - TY - JOUR A1 - Auyyuenyong, Ratchada A1 - Henze, Andrea A1 - Ungru, Julia A1 - Schweigert, Florian Johannes A1 - Raila, Jens A1 - Vervuert, Ingrid T1 - Determination of lipid profiles in serum of obese ponies before and after weight reduction by using multi-one-dimensional thin-layer chromatography JF - Research in veterinary science N2 - Obesity is a key component of equine metabolic syndrome, which is highly associated with laminitis. Feed restriction and/or exercise are known to alleviate the detrimental effects of insulin resistance in obese ponies. However, little is known about changes in the serum lipid patterns due to weight reduction and its association with disease outcomes. Therefore, the lipid patterns in the serum of 14 mature ponies before and after a 14-week body weight reduction program (BWRP) were investigated by multi-one-dimensional thin-layer chromatography (MOD-TLC). Additionally, sensitivity to insulin (SI), body condition scores (BCS) and cresty neck scores (CNS) were measured. A BWRP resulted in a significant loss of body weight (P < 0.001), which was associated with beneficial decreases in BCS and CNS (both, P < 0.001). Serum lipid compositions revealed significantly increased free fatty acid (FFA), sphingomyelin (SM; both P < 0.001), total cholesterol (C) and cholesterol ester (CE) (both P < 0.01) and triacylglycerol (TG; P < 0.05) densities. Improvement of SI after the BWRP was associated with increases in neutral lipids (C, CE and TG, all P < 0.01), FFA and the phospholipid SM (both, P < 0.001). The results show that a BWRP in obese ponies was effective and associated with changes in the concentrations of neutral lipids and the phospholipid SM, indicating that SM may play a role in insulin signaling pathways and thus in the pathogenesis of insulin resistance and the progression of metabolic syndrome in obese ponies. KW - Neutral lipids KW - Equine metabolic syndrome KW - Phospholipids KW - Horse KW - Thin layer chromatography Y1 - 2017 U6 - https://doi.org/10.1016/j.rvsc.2017.11.013 SN - 0034-5288 SN - 1532-2661 VL - 117 SP - 111 EP - 117 PB - Elsevier CY - Oxford ER - TY - GEN A1 - Avila, Daiana Silva A1 - Benedetto, Alexandre A1 - Au, Catherine A1 - Bornhorst, Julia A1 - Aschner, Michael A. T1 - Involvement of heat shock proteins on Mn-induced toxicity in Caenorhabditis elegans T2 - BMC pharmacology and toxicology N2 - Background: All living cells display a rapid molecular response to adverse environmental conditions, and the heat shock protein family reflects one such example. Hence, failing to activate heat shock proteins can impair the cellular response. In the present study, we evaluated whether the loss of different isoforms of heat shock protein ( hsp ) genes in Caenorhabditis elegans would affect their vulnerability to Manganese (Mn) toxicity. Methods: We exposed wild type and selected hsp mutant worms to Mn (30 min) and next evaluated further the most susceptible strains. We analyzed survi val, protein carbonylation (as a marker of oxidative stress) and Parkinson ’ s disease related gene expression immediately after Mn exposure. Lastly, we observed dopaminergic neurons in wild type worms and in hsp-70 mutants following Mn treatment. Analysis of the data was performed by one-way or two way ANOVA, depending on the case, followed by post-hoc Bonferroni test if the overall p value was less than 0.05. Results: We verified that the loss of hsp-70, hsp-3 and chn-1 increased the vulnerability to Mn, as exposed mutant worms showed lower survival rate and increased protein oxidation. The importance of hsp-70 against Mn toxicity was then corroborated in dopaminergic neurons, where Mn neurotoxicity was aggravated. The lack of hsp-70 also blocked the transcriptional upregulation of pink1 , a gene that has been linked to Parkinson ’ sdisease. Conclusions: Taken together, our data suggest that Mn exposu re modulates heat shock protein expression, particularly HSP-70, in C. elegans .Furthermore,lossof hsp-70 increases protein oxidation and dopaminergic neuronal degeneration following manganese exposure, which is associated with the inhibition of pink1 increased expression, thus pot entially exacerbating the v ulnerability to this metal. T3 - Zweitveröffentlichungen der Universität Potsdam : Mathematisch-Naturwissenschaftliche Reihe - 439 KW - Caenorhabitis elegans KW - Manganese KW - heat shock proteins KW - hsp-70 KW - pink1 Y1 - 2018 U6 - http://nbn-resolving.de/urn/resolver.pl?urn:nbn:de:kobv:517-opus4-407286 ER - TY - JOUR A1 - Avila, Daiana Silva A1 - Benedetto, Alexandre A1 - Au, Catherine A1 - Bornhorst, Julia A1 - Aschner, Michael A. T1 - Involvement of heat shock proteins on Mn-induced toxicity in Caenorhabditis elegans JF - Plant Methods N2 - Background: All living cells display a rapid molecular response to adverse environmental conditions, and the heat shock protein family reflects one such example. Hence, failing to activate heat shock proteins can impair the cellular response. In the present study, we evaluated whether the loss of different isoforms of heat shock protein (hsp) genes in Caenorhabditis elegans would affect their vulnerability to Manganese (Mn) toxicity. Conclusions: Taken together, our data suggest that Mn exposure modulates heat shock protein expression, particularly HSP-70, in C. elegans. Furthermore, loss of hsp-70 increases protein oxidation and dopaminergic neuronal degeneration following manganese exposure, which is associated with the inhibition of pink1 increased expression, thus potentially exacerbating the vulnerability to this metal. KW - Caenorhabitis elegans KW - Manganese KW - Heat shock proteins KW - hsp-70 KW - pink1 Y1 - 2016 U6 - https://doi.org/10.1186/s40360-016-0097-2 SN - 2050-6511 VL - 17 PB - BioMed Central CY - London ER -