Search

Your search keyword '"Korner G"' showing total 37 results
Start Over Author "Korner G"
37 results on '"Korner G"'

2. A gene therapeutic approach to correct splice defects with modified U1 and U6 snRNPs

Author

Schmid, F, Hiller, T, Korner, G, Glaus, E, Berger, W, Neidhardt, J, Schmid, F, Hiller, T, Korner, G, Glaus, E, Berger, W, and Neidhardt, J

Abstract

Splicing is an essential cellular process to generate mature transcripts from pre-mRNA. It requires the splice factor U1 small nuclear ribonucleoprotein (U1), which promotes exon recognition by base-pairing interaction with the splice donor site (SD). After U1 dissociation, exon recognition is maintained by U6 small nuclear ribonucleoproteins (U6). It has been shown that SD mutations lower the binding affinity of U1 and cause splice defects in about 10% of patients with monogenetic diseases. U1 isoforms specifically designed to bind the mutated SD with increased affinity can correct these splice defects. We investigated the applicability of this gene therapeutic approach for different mutated SD positions. A minigene-based splicing assay was established to study a typical SD derived from the gene BBS1. We found that mutations at seven SD positions caused splice defects. In four cases, mutation-adapted U1 isoforms completely corrected these splice defects. Partial correction was found for splice defects induced by the mutation at SD position +5. The limited therapeutic efficacy at this position was alleviated by applying a combined treatment with mutation-adapted U1 and U6. The sequence complementarity between U6 and three SD positions (+4, +5,and +6) was relevant for the outcome of the therapy. Between 30 and 100% of the normal transcripts can be restored. The treatment significantly decreased both exon skipping and intron retention. Massive missplicing of off-target transcripts was not detected. Our study helps to assess the therapeutic efficacy of mutation-adapted U snRNAs in gene therapy and illustrates their strong potential to correct splice defects, which cause many different inherited conditions.

Published
2013

3. A pressure-tolerant AUV for deep sea applications.

Author

Schmidt, T., Gelze, J., Lehr, H., Mischnick, D., Olenew, E., Preradovic, O., Korner, G., Korner, H.-M., Thiede, C., Kruger, S., Huth, H., Bannasch, R., Kebkal, A., and Yakovlev, S.

Published
2011

11. Messung des Beimengungsanteils in Kartoffeln an einer Einlagerungsstrecke mittels Zwei-Gammaenergie-Transmissionsverfahren

Author

Glaser, M., Thummel, H. -W., and Korner, G.

Abstract

Das ursprunglich fur die Ascheanteilsbestimmung in Braunkohle entwickelte Komplexe Radiometrische Analysen-system KRAS-2“, das auf der Grundlage des Zwei-Gammaenergie-Transmissionsverfahrens arbeitet und zur Eliminierung von Dichte- und Schichtdickenschwankungen des Meβgutes ein auf einem Mikroprozessor basierendes Datenver-arbeitungssystem enthalt, wurde hinsichtlich seiner Eignung fur die Messung des Anteils mineralischer Beimengungen in Erntegutern getestet. Die on-line-Messungen an einer Kartoffel-Einlagerungsstrecke einer Praxis-Anlage wahrend der Erntekampagne bestatigten die Ergebnisse aus vorausgegangenen Abschatzungen und Laborexperimenten, daβ der Beimengungsanteil mit einem Fehler von unter 3 Masseprozent bestimmbar ist.The 2-energy transmission gauge KRAS-2 applying a microprocessorbased on-line date processing for eliminating surface density variations - originally developed for ash content determination in raw lignite - has been checked for its applicability to measuring the content of mineral substance in crop materials. On-line measurements at one of the entrance conveyor belts of a potatoe store facility during the harvesting campaign proved, that the soil content can be measured with an accuracy of better than 3 mass-% as required in practice.

Published
1987
Full Text
View/download PDF

12. Messungen hinsichtlich der Materialabhangigkeit des Massenschwachungs-koeffizienten von Betastrahlung

Author

Thummel, H. -W., Korner, G., Becker, A., and Apel, K.

Abstract

Mit einem Endfenster-Zahlrohr warden fur die Betastrahlung des 144Pr (Maximalenergie 3 MeV, im Gleichgewicht mit 144Ce) fur 12 Absorberelemente (Beryllium bis Blei) die Massenschwachungskoeffizienten bestimmt. Die gefundene Kernladungszahlabhangigkeit laβt sich fur Kernladungszahlen oberhalb etwa 13 innerhalb des Meβfehlers (von 1 bis 2%) durch eine lineare Funktion darstellen. Anzahl der untersuchten Absorberelemente sowie ihre Lage innerhalb der 5. und 6. Periode schlieβen aus, daβ eine mit den Perioden des Systems der chemischen Elemente konform gehende Abhungigkeit des Massenschwachungskoeffizienten von der Kernladungszahl, wie sie beispielsweise von Crowther 1906 gemessen wurde, auftritt.

Published
1976
Full Text
View/download PDF

13. Bovine aortic endothelial cell transglutaminase. Enzyme characterization and regulation of activity

Author

Korner, G, Schneider, D E, Purdon, M A, and Bjornsson, T D

Abstract

Bovine aortic endothelial cells contain Ca2+-dependent tissue-type transglutaminase. Its activity in these cells was high, with apparent Km and Vmax. values with respect to putrescine of 0.203 mM and 18.5 nmol/min per mg of protein, and its activity was inhibited by the three competitive inhibitors dansylcadaverine, spermine and methylamine. The molecular mass of endothelial cell transglutaminase estimated by gel filtration chromatography was 88 kDa and it was immunoprecipitated by rabbit monospecific antiserum raised against rat liver transglutaminase. Its enzymic activity rose when the cell cultures reached confluence, and was further increased when their proliferation was arrested (synchronized at G0/G1 phase). Most of the enzymic activity was found in the 15,000 g soluble fraction, with only 4-22% of the activity found in the particulate fraction, depending on the state of cell proliferation. Examination of these cellular fractions by SDS/polyacrylamide-gel electrophoresis and immunoblotting revealed that at confluence endothelial cells have accumulated transglutaminase antigen in their 15,000 g particulate fraction. A series of experiments demonstrated the existence of a latent transglutaminase form in non-proliferating cells, and suggested that this might involve the formation of an inhibitory complex. Treatment of cell lysates and the 15,000 g particulate fraction with high salt concentration showed a significant increase in transglutaminase activity. Mixing experiments using the 100,000 g particulate fraction or purified rat liver transglutaminase on one hand and the cytosolic fraction on the other showed dose-dependent inhibition of the transglutaminase activity of the latter. It is concluded that endothelial cells contain a particulate fraction-residing inhibitor of transglutaminase which interacts via ionic interaction with the enzyme.

Published
1989
Full Text
View/download PDF

14. Zum Einfluss der Messgeometric auf den Massenschwachungskoeffizienten von Festabsorben fur Betastrahlung.

Author

Thummel, H. W. and Korner, G.

Abstract

Mit einem Glockenzahlrohr wurden die Transmissionskurven von 10 Absorberelementen (Al bis Pb) fur die Belastrahlung des 144Ce-144Pr in unterschiedlichen Meβanordnungen bestimmt. Es zeigen sich Gesetzmaβigkeiten fur die Abhangigkeit des Massenschwachungskoeffizienten von zwei maβgeblichen geometrischen Parametern, das sind der Raumwinkel der Einfallsgeometrie und der Raumwinkel der Detektionsgeometrie. Die wenigen bisher vorliegenden Meβwerte anderer Autoren lassen sich meist zwangslos in die gefundenen Geselzmaβigkeiten einordnen.Die in vorangegangenen Mitteilungen [1,2] diskutierten Periodizitaten in der Kernladungszahlabhangigkeit des Massenschwachungskoeffizienten konnten in keiner der untersuchten Geometrien nachgewiesen werden.

Published
1976
Full Text
View/download PDF

19. Ash On-Line Determination in Brown Coal by Means of Scattered Forward and Transmitted 60 keV and 660 keV Photons

Author

Leonhardt, J. W., Fritsche, D., Korner, G., and Thummel, H. -W.

Abstract

Combining the 60 keV scatter-transmission signal (s. d. about 4 wt % ash) with the 660 keV transmission signal thus eliminating residual influences of thickness and density variations the s. d. can be reduced to about 2 … 3 wt % ash. A gauge developed for on-line determination of ash content based on the 2-energy narrow beam transmission method using a micro-processor for data processing was tested at the main conveyour belt of a power station giving a s. d. of about 5 wt % ash with coal thickness variations between 5 and 40 cm.

Published
1985
Full Text
View/download PDF

23. Mildly compromised tetrahydrobiopterin cofactor biosynthesis due to Pts variants leads to unusual body fat distribution and abdominal obesity in mice.

Author

Korner G, Scherer T, Adamsen D, Rebuffat A, Crabtree M, Rassi A, Scavelli R, Homma D, Ledermann B, Konrad D, Ichinose H, Wolfrum C, Horsch M, Rathkolb B, Klingenspor M, Beckers J, Wolf E, Gailus-Durner V, Fuchs H, Hrabě de Angelis M, Blau N, Rozman J, and Thöny B

Subjects
Alleles, Animals, Biopterins biosynthesis, Biopterins genetics, Body Weight genetics, Cholesterol genetics, Female, Genotype, Glucose genetics, Heterozygote, Homozygote, Lipid Metabolism genetics, Male, Mice, Mice, Inbred C57BL, Mice, Knockout, Mutation genetics, Nitric Oxide Synthase genetics, Nitric Oxide Synthase Type III genetics, Phenylalanine genetics, Transcriptome genetics, Adipose Tissue metabolism, Biopterins analogs & derivatives, Body Fat Distribution, Obesity, Abdominal genetics, Phosphorus-Oxygen Lyases genetics
Abstract

Tetrahydrobiopterin (BH4) is an essential cofactor for the aromatic amino acid hydroxylases, alkylglycerol monooxygenase, and nitric oxide synthases (NOS). Inborn errors of BH4 metabolism lead to severe insufficiency of brain monoamine neurotransmitters while augmentation of BH4 by supplementation or stimulation of its biosynthesis is thought to ameliorate endothelial NOS (eNOS) dysfunction, to protect from (cardio-) vascular disease and/or prevent obesity and development of the metabolic syndrome. We have previously reported that homozygous knock-out mice for the 6-pyruvolytetrahydropterin synthase (PTPS; Pts-ko/ko) mice with no BH4 biosynthesis die after birth. Here we generated a Pts-knock-in (Pts-ki) allele expressing the murine PTPS-p.Arg15Cys with low residual activity (15% of wild-type in vitro) and investigated homozygous (Pts-ki/ki) and compound heterozygous (Pts-ki/ko) mutants. All mice showed normal viability and depending on the severity of the Pts alleles exhibited up to 90% reduction of PTPS activity concomitant with neopterin elevation and mild reduction of total biopterin while blood L-phenylalanine and brain monoamine neurotransmitters were unaffected. Yet, adult mutant mice with compromised PTPS activity (i.e., Pts-ki/ko, Pts-ki/ki or Pts-ko/wt) had increased body weight and elevated intra-abdominal fat. Comprehensive phenotyping of Pts-ki/ki mice revealed alterations in energy metabolism with proportionally higher fat content but lower lean mass, and increased blood glucose and cholesterol. Transcriptome analysis indicated changes in glucose and lipid metabolism. Furthermore, differentially expressed genes associated with obesity, weight loss, hepatic steatosis, and insulin sensitivity were consistent with the observed phenotypic alterations. We conclude that reduced PTPS activity concomitant with mildly compromised BH4-biosynthesis leads to abnormal body fat distribution and abdominal obesity at least in mice. This study associates a novel single gene mutation with monogenic forms of obesity.

Published
2016
Full Text
View/download PDF

24. Brain catecholamine depletion and motor impairment in a Th knock-in mouse with type B tyrosine hydroxylase deficiency.

Author

Korner G, Noain D, Ying M, Hole M, Flydal MI, Scherer T, Allegri G, Rassi A, Fingerhut R, Becu-Villalobos D, Pillai S, Wueest S, Konrad D, Lauber-Biason A, Baumann CR, Bindoff LA, Martinez A, and Thöny B

Subjects
Animals, Biopterins metabolism, Brain pathology, Disease Models, Animal, Dopamine Agents therapeutic use, Eating genetics, Female, Gene Expression Regulation genetics, Gene Knock-In Techniques, Levodopa therapeutic use, Male, Mice, Mice, Inbred C57BL, Mice, Transgenic, Motor Activity genetics, Movement Disorders drug therapy, Mutation genetics, Thyroxine metabolism, Brain metabolism, Catecholamines metabolism, Movement Disorders pathology, Tyrosine 3-Monooxygenase genetics, Tyrosine 3-Monooxygenase metabolism
Abstract

Tyrosine hydroxylase catalyses the hydroxylation of L-tyrosine to l-DOPA, the rate-limiting step in the synthesis of catecholamines. Mutations in the TH gene encoding tyrosine hydroxylase are associated with the autosomal recessive disorder tyrosine hydroxylase deficiency, which manifests phenotypes varying from infantile parkinsonism and DOPA-responsive dystonia, also termed type A, to complex encephalopathy with perinatal onset, termed type B. We generated homozygous Th knock-in mice with the mutation Th-p.R203H, equivalent to the most recurrent human mutation associated with type B tyrosine hydroxylase deficiency (TH-p.R233H), often unresponsive to l-DOPA treatment. The Th knock-in mice showed normal survival and food intake, but hypotension, hypokinesia, reduced motor coordination, wide-based gate and catalepsy. This phenotype was associated with a gradual loss of central catecholamines and the serious manifestations of motor impairment presented diurnal fluctuation but did not improve with standard l-DOPA treatment. The mutant tyrosine hydroxylase enzyme was unstable and exhibited deficient stabilization by catecholamines, leading to decline of brain tyrosine hydroxylase-immunoreactivity in the Th knock-in mice. In fact the substantia nigra presented an almost normal level of mutant tyrosine hydroxylase protein but distinct absence of the enzyme was observed in the striatum, indicating a mutation-associated mislocalization of tyrosine hydroxylase in the nigrostriatal pathway. This hypomorphic mouse model thus provides understanding on pathomechanisms in type B tyrosine hydroxylase deficiency and a platform for the evaluation of novel therapeutics for movement disorders with loss of dopaminergic input to the striatum., (© The Author (2015). Published by Oxford University Press on behalf of the Guarantors of Brain. All rights reserved. For Permissions, please email: journals.permissions@oup.com.)

Published
2015
Full Text
View/download PDF

25. A gene therapeutic approach to correct splice defects with modified U1 and U6 snRNPs.

Author

Schmid F, Hiller T, Korner G, Glaus E, Berger W, and Neidhardt J

Subjects
Animals, COS Cells, Chlorocebus aethiops, Humans, Microtubule-Associated Proteins genetics, Mutagenesis, Site-Directed, Mutation genetics, RNA Splice Sites genetics, Reverse Transcriptase Polymerase Chain Reaction, Ribonucleoprotein, U1 Small Nuclear genetics, Ribonucleoprotein, U4-U6 Small Nuclear genetics, Treatment Outcome, Alternative Splicing genetics, Genetic Therapy methods, Ribonucleoprotein, U1 Small Nuclear therapeutic use, Ribonucleoprotein, U4-U6 Small Nuclear therapeutic use
Abstract

Splicing is an essential cellular process to generate mature transcripts from pre-mRNA. It requires the splice factor U1 small nuclear ribonucleoprotein (U1), which promotes exon recognition by base-pairing interaction with the splice donor site (SD). After U1 dissociation, exon recognition is maintained by U6 small nuclear ribonucleoproteins (U6). It has been shown that SD mutations lower the binding affinity of U1 and cause splice defects in about 10% of patients with monogenetic diseases. U1 isoforms specifically designed to bind the mutated SD with increased affinity can correct these splice defects. We investigated the applicability of this gene therapeutic approach for different mutated SD positions. A minigene-based splicing assay was established to study a typical SD derived from the gene BBS1. We found that mutations at seven SD positions caused splice defects. In four cases, mutation-adapted U1 isoforms completely corrected these splice defects. Partial correction was found for splice defects induced by the mutation at SD position +5. The limited therapeutic efficacy at this position was alleviated by applying a combined treatment with mutation-adapted U1 and U6. The sequence complementarity between U6 and three SD positions (+4, +5,and +6) was relevant for the outcome of the therapy. Between 30 and 100% of the normal transcripts can be restored. The treatment significantly decreased both exon skipping and intron retention. Massive missplicing of off-target transcripts was not detected. Our study helps to assess the therapeutic efficacy of mutation-adapted U snRNAs in gene therapy and illustrates their strong potential to correct splice defects, which cause many different inherited conditions.

Published
2013
Full Text
View/download PDF

26. In the blink of an eye.

Author

Korner G

Subjects
Telecommunications trends, United Kingdom, Fiber Optic Technology, Telecommunications instrumentation
Published
2001

27. Purification and characterization of placental heparanase and its expression by cultured cytotrophoblasts.

Author

Goshen R, Hochberg AA, Korner G, Levy E, Ishai-Michaeli R, Elkin M, de Groot N, and Vlodavsky I

Subjects
Cells, Cultured, Culture Media, Conditioned, Extracellular Matrix metabolism, Female, Fibroblast Growth Factor 2 metabolism, Humans, In Vitro Techniques, Placenta metabolism, Placentation physiology, Pregnancy, Substrate Specificity, Trophoblasts cytology, Trophoblasts physiology, Glucuronidase, Glycoside Hydrolases isolation & purification, Glycoside Hydrolases metabolism, Placenta enzymology, Trophoblasts enzymology
Abstract

The role of different extracellular matrix (ECM)-degrading enzymes in the normal functioning of the placenta is well documented. Heparan sulphate proteoglycan (HSPG) is an integral constituent of the placental and decidual ECM. Because this proteoglycan specifically interacts with various macromolecules in the ECM, its degradation may disassemble the matrix. Hence, in the case of the placenta, this may facilitate normal placentation and trophoblast invasion. Crude placental specimens were collected from first and third trimester placentas. Heparanase (endo-beta-glucuronidase) was isolated and purified by ammonium sulphate precipitation followed by sequential chromatographies on carboxymethyl-, heparin- and ConA-Sepharose columns. The placental enzyme was further characterized for its molecular weight and specific inhibition by heparin, and was shown to resemble heparanase expressed by highly metastatic tumor cells and activated cells of the immune system. In order to locate the source of heparanase activity in the placenta, primary cytotrophoblast cultures were established. Intact cells, as well as conditioned medium and cell lysates, were analysed for heparanase activity using metabolically sulphate-labelled ECM as a natural substrate. Heparanase was highly active in lysates of cytotrophoblasts. This activity was also expressed by intact cytotrophoblasts seeded on ECM, but no activity could be detected in the culture medium. Incubation of the cytotrophoblasts in contact with ECM resulted in release of ECM-bound basic fibroblast growth factor (bFGF). We propose that the cytotrophoblastic heparanase facilitates placentation, through cytotrophoblast extravasation and localized neovascularization.

Published
1996
Full Text
View/download PDF

28. Packaging zinc, fibrinogen, and factor XIII in platelet alpha-granules.

Author

Marx G, Korner G, Mou X, and Gorodetsky R

Subjects
Humans, Rubidium blood, Rubidium Radioisotopes, Subcellular Fractions metabolism, Blood Platelets metabolism, Cytoplasmic Granules metabolism, Factor XIII metabolism, Fibrinogen metabolism, Zinc blood
Abstract

Zinc(II) accumulated by platelets has profound effects on platelet activity. This study is focused on the distribution of Zn(II) between human platelet subcellular compartments. After incubation with 86Rb+ and platelet lysis, the organelles were separated by sucrose density gradient centrifugation. Fibrinogen served as a marker for alpha-granules. 86Rb+ and factor XIII served as markers for the cytoplasmic fractions. Zn(II) was found to be distributed between the cytoplasm and the alpha-granules, with variations between different individual units. The total platelet Zn concentration and its relative subcellular distribution were dependent on its extracellular level. Incubation of platelets with 100 microM Zn(II) resulted in a twofold increase of its level in the cytoplasm and by one order of magnitude in the alpha-granules. In addition to the anticipated factor XIII activity in the cytoplasmic pool fraction, we found thrombin-inducible factor XIII activity within the alpha-granules. Immunoblotting confirmed the presence of both the a and b subunits of plasma factor XIII (a2b2 form) in the alpha-granules. As fibrinogen is not synthesized in the platelet, we propose that by virtue of their mutual binding, fibrinogen, Zn(II) and plasma factor XIII-a2b2 are simultaneously taken up into the alpha-granules by endocytosis, presumably through the vehicle of the GPIIb/IIIa fibrinogen receptor. A rationale for co-packaging these components within the alpha-granules is that Zn(II) inhibits factor XIII activity and thereby prevents the premature cross-linking of the concentrated fibrinogen prior to platelet activation and secretion. By contrast, cytoplasmic Zn(II) may increase platelet responsiveness to agonists due to its interaction with cytoplasmic modulators of platelet activity.

Published
1993
Full Text
View/download PDF

29. Extracellular matrix produced by cultured corneal and aortic endothelial cells contains active tissue-type and urokinase-type plasminogen activators.

Author

Korner G, Bjornsson TD, and Vlodavsky I

Subjects
Absorption, Animals, Aorta, Cattle, Cells, Cultured, Endothelium, Corneal chemistry, Endothelium, Vascular chemistry, Extracellular Matrix chemistry, Glycoside Hydrolases metabolism, Molecular Weight, Plasminogen Activator Inhibitor 1 analysis, Tissue Plasminogen Activator chemistry, Urokinase-Type Plasminogen Activator chemistry, Endothelium, Corneal enzymology, Endothelium, Vascular enzymology, Extracellular Matrix enzymology, Glucuronidase, Tissue Plasminogen Activator metabolism, Urokinase-Type Plasminogen Activator metabolism
Abstract

Incubation of plasminogen with the subendothelial extracellular matrix (ECM) synthesized by cultured bovine corneal and aortic endothelial cells resulted in generation of fibrinolytic activity, indicated by proteolysis of 125I-fibrin in a time- and dose-dependent manner. Both tissue-type plasminogen activator (t-PA) and urokinase-type plasminogen activator (u-PA) were identified in the ECM by fibrin zymography, immunoblotting, and inhibition of plasminogen activation by anti-u-PA and anti-t-PA antibodies. Most of the ECM-resident plasminogen activator (PA) activity did not originate from intracellular PA release occurring when the endothelial cells were lyzed and the ECM exposed, since a comparable amount of PA was associated with the ECM when the cells were lyzed with Triton X-100 or removed intact by treatment with 2 M urea. Active u-PA and t-PA were released from ECM by treatment with heparanase (endo-beta-D-glucuronidase), indicating that some of the ECM-resident PA activity is sequestered by heparan sulfate side chains. These results indicate that both u-PA and t-PA produced by endothelial cells are firmly sequestered in an active form by the subendothelial ECM. It is suggested that ECM-resident plasminogen activators participate in sequential matrix degradation during cell invasion and tumor metastasis. PA activity may also function in release of ECM-bound growth factors (i.e., basic fibroblast growth factor) and activation of proenzymes (i.e., prothrombin), resulting in modulation of the ECM growth-promoting and thrombogenic properties.

Published
1993
Full Text
View/download PDF

30. Importance of size and sulfation of heparin in release of basic fibroblast growth factor from the vascular endothelium and extracellular matrix.

Author

Ishai-Michaeli R, Svahn CM, Weber M, Chajek-Shaul T, Korner G, Ekre HP, and Vlodavsky I

Subjects
Animals, Autoradiography, Cattle, Electrophoresis, Polyacrylamide Gel, Glycoside Hydrolases metabolism, Humans, Magnetic Resonance Spectroscopy, Oligosaccharides metabolism, Recombinant Proteins metabolism, Sulfuric Acids chemistry, Swine, Endothelium, Vascular metabolism, Extracellular Matrix metabolism, Fibroblast Growth Factor 2 metabolism, Glucuronidase, Heparin metabolism
Abstract

We have characterized the importance of size, sulfation, and anticoagulant activity of heparin in release of basic fibroblast growth factor (bFGF) from the subendothelial extracellular matrix (ECM) and the luminal surface of the vascular endothelium. For this purpose, 125I-bFGF was first incubated with ECM and confluent endothelial cell cultures, or administered as a bolus into the blood of rats, the immobilized 125I-bFGF was then subjected to release by various chemically modified species of heparin and size-homogeneous oligosaccharides derived from depolymerized heparin. Both totally desulfated and N-desulfated heparin failed to release the ECM-bound bFGF. Likewise, substitution of N-sulfate groups of heparin and low molecular weight heparin (fragmin) by acetyl or hexanoyl residues resulted in an almost complete inhibition of bFGF release by these polysaccharides. The presence of O-sulfate groups in heparin increased but was not critical for release of ECM-bound bFGF. Similar structural requirements were identified for release of 125I-bFGF bound to low-affinity sites on the surface of vascular endothelial cells. Oligosaccharides derived from depolymerized heparin and containing as little as 8-10 sugar units were, on a weight basis, equivalent to whole heparin in their ability to release bFGF from ECM. Low-sulfate oligosaccharides were less effective releasers of bFGF as compared to medium- and high-sulfate fractions of the same size oligosaccharides. Heparin fractions with high and low affinity to antithrombin III exhibited a similar high bFGF-releasing activity despite a 200-fold difference in their anticoagulant activities.(ABSTRACT TRUNCATED AT 250 WORDS)

Published
1992
Full Text
View/download PDF

31. Extracellular matrix-resident basic fibroblast growth factor: implication for the control of angiogenesis.

Author

Vlodavsky I, Fuks Z, Ishai-Michaeli R, Bashkin P, Levi E, Korner G, Bar-Shavit R, and Klagsbrun M

Subjects
Animals, Basement Membrane chemistry, Blood Platelets metabolism, Cattle, Cell Differentiation, Cell Division, Cornea, Endothelium, Vascular chemistry, Endothelium, Vascular cytology, Extracellular Matrix chemistry, Glycoside Hydrolases metabolism, Growth Substances isolation & purification, Humans, Lymphoma pathology, Neoplastic Stem Cells metabolism, Neurons cytology, Neutrophils metabolism, Organ Specificity, Extracellular Matrix Proteins physiology, Fibroblast Growth Factor 2 physiology, Glucuronidase, Neovascularization, Pathologic
Abstract

Despite the ubiquitous presence of basic fibroblast growth factor (bFGF) in normal tissues, endothelial cell proliferation in these tissues is usually very low, suggesting that bFGF is somehow sequestered from its site of action. Immunohistochemical staining revealed the localization of bFGF in basement membranes of diverse tissues, suggesting that the extracellular matrix (ECM) may serve as a reservoir for bFGF. Moreover, functional studies indicated that bFGF is an ECM component required for supporting endothelial cell proliferation and neuronal differentiation. We have found that bFGF is bound to heparan sulfate (HS) in the ECM and is released in an active form when the ECM-HS is degraded by heparanase expressed by normal and malignant cells (i.e. platelets, neutrophils, lymphoma cells). It is proposed that restriction of bFGF bioavailability by binding to ECM and local regulation of its release provide a novel mechanism for neovascularization in normal and pathological situations. The subendothelial ECM contains also tissue type- and urokinase type-plasminogen activators which participate in cell invasion and tissue remodeling. These results and studies on the properties of other ECM-immobilized enzymes (i.e. thrombin, plasmin, lipoprotein lipase) and growth factors (GM-CSF, IL-3, osteogenin), suggest that the ECM provides a storage depot for biologically active molecules which are thereby stabilized and protected. This may allow a more localized and persistent mode of action, as compared to the same molecules in a fluid phase.

Published
1991
Full Text
View/download PDF

32. Extracellular matrix-resident growth factors and enzymes: possible involvement in tumor metastasis and angiogenesis.

Author

Vlodavsky I, Korner G, Ishai-Michaeli R, Bashkin P, Bar-Shavit R, and Fuks Z

Subjects
Animals, Extracellular Matrix enzymology, Fibroblast Growth Factor 2 physiology, Glycoside Hydrolases physiology, Heparitin Sulfate physiology, Humans, Plasminogen Activators physiology, Plasminogen Inactivators metabolism, Extracellular Matrix chemistry, Glucuronidase, Neoplasm Metastasis physiopathology, Neovascularization, Pathologic physiopathology
Abstract

Neoplastic cells require an appropriate pericellular environment and new formation of stroma and blood vessels in order to constitute a solid tumor. Tumor progression also involves degradation of various extracellular matrix (ECM) constituents. In this review we have focused on the possible involvement of ECM-resident growth factors and enzymes in neovascularization and cell invasion. We demonstrate that the pluripotent angiogenic factor, basic fibroblast growth factor (bFGF) is an ECM component required for supporting cell proliferation and differentiation. Basic FGF has been identified in the subendothelial ECM produced in vitro and in basement membranes of the cornea and blood vessels in vivo. Despite the ubiquitous presence of bFGF in normal tissues, endothelial cell (EC) proliferation in these tissues is usually very low, suggesting that bFGF is somehow sequestered from its site of action. Our results indicate that bFGF is bound to heparan sulfate (HS) in the ECM and is released in an active form when the ECM-HS is degraded by cellular heparanase. We propose that restriction of bFGF bioavailability by binding to ECM and local regulation of its release, provides a novel mechanism for regulation of capillary blood vessel growth in normal and pathological situations. Heparanase activity correlates with the metastatic potential of various tumor cells and heparanase inhibiting molecules markedly reduce the incidence of lung metastasis in experimental animals. Heparanase may therefore participate in both tumor cell invasion and angiogenesis through degradation of the ECM-HS and mobilization of ECM-resident EC growth factors. The subendothelial ECM contains also tissue type- and urokinase type- plasminogen activators (PA), as well as PA inhibitor which may regulate cell invasion and tissue remodeling. Heparanase and the ECM-resident PA participate synergistically in sequential degradation of HS-proteoglycans in the ECM. These results together with similar observations on the properties of other ECM-immobilized enzymes and growth factors, suggest that the ECM provides a storage depot for biologically active molecules which are thereby stabilized and protected. This may allow a more localized, regulated and persistent mode of action, as compared to the same molecules in a fluid phase.

Published
1990
Full Text
View/download PDF

33. A unique placental lactogen receptor: implications for fetal growth.

Author

Freemark M, Comer M, Korner G, and Handwerger S

Subjects
Animals, Binding, Competitive, Female, Gestational Age, Growth Hormone metabolism, Liver metabolism, Macromolecular Substances, Placental Lactogen metabolism, Pregnancy, Prolactin metabolism, Sheep, Embryonic and Fetal Development, Liver embryology, Pregnancy, Animal metabolism, Receptors, Peptide, Receptors, Prolactin physiology
Abstract

To determine whether there are structural differences between the binding sites for placental lactogen (PL) and GH, we have compared the molecular weights of complexes formed by the covalent cross-linking of [125I]ovine (o) PL and [125I]oGH to hepatic membranes from fetal and pregnant sheep in mid- and late gestation and from postnatal nonpregnant sheep at 3 days to 7 months of age. Specific [125I]oPL binding sites in fetal liver were detected as early as midgestation, and cross-linking of [125I]oPL to fetal hepatic membranes yielded a major radiographic band with a mol wt of 60 +/- 5 K (mean +/- SD). Unlabeled oPL at low concentrations (0.9-9 nM) specifically competed with [125I]oPL for binding to the 60 K complex. In contrast, oGH and oPRL competed for binding to the 60 K complex only at much higher concentrations (greater than or equal to 90 nM). In addition, no specific cross-linking of [125I]oGH or [125I]oPRL to fetal hepatic membranes was observed. These findings suggest the presence of a distinct and unique PL binding site in ovine fetal liver. Since the mol wt of oPL is 22 K, the estimated mol wt of the oPL receptor protein is 38 +/- 5 K. During the first week after birth, there was a striking increase in the number of [125I]oGH binding sites. Cross-linking of [125I]oGH to postnatal liver yielded radiographic bands with apparent mol wts of 75 K and 140 K. The relative potencies of oPL, oGH, and oPRL in competing for binding to the 75 K and 140 K complexes were similar to the relative potencies of these hormones in competing for [125I]oGH binding sites in postnatal liver, suggesting that the 75 K and 140 K bands represent subunits of the oGH receptor bound covalently to [125I]oGH. Cross-linking of [125I]oPL to pregnant and postnatal nonpregnant liver yielded three radiographic bands with mol wts of 60 K, 75 K, and 140 K. The intensities of all three bands were reduced by low concentrations (0.9-9 nM) of oPL. Higher concentrations of oGH abolished the 75 K and 140 K bands but reduced the intensity of the 60 K band by only 20-30%. oPRL had minimal effect on band intensities. These observations suggest the presence of two functionally and structurally distinct receptors in pregnant liver: the oPL receptor, which has high affinity for oPL and low affinity for oGH and oPRL.(ABSTRACT TRUNCATED AT 400 WORDS)

Published
1987
Full Text
View/download PDF

34. Role of polyamines in the stimulation of synthesis and secretion of plasminogen activator from bovine aortic endothelial cells.

Author

Kuo BS, Korner G, Dryjski M, and Bjornsson TD

Subjects
Animals, Cattle, Cells, Cultured, Cycloheximide pharmacology, Dactinomycin pharmacology, Dose-Response Relationship, Drug, Eflornithine pharmacology, Electrophoresis, Polyacrylamide Gel, Glycoproteins biosynthesis, Glycoproteins metabolism, Mitoguazone pharmacology, Plasminogen Activators antagonists & inhibitors, Plasminogen Activators metabolism, Plasminogen Inactivators, Putrescine pharmacology, Spermidine pharmacology, Spermine pharmacology, Endothelium, Vascular metabolism, Plasminogen Activators biosynthesis, Polyamines pharmacology
Abstract

The effects of the polyamines putrescine (PUT), spermidine (SPD), and spermidine (SPM) on the secretion of plasminogen activator (PA) and plasminogen activator inhibitor (PAI) were evaluated using cultured bovine aortic endothelial cells. All three polyamines enhanced PA secretion in a time- and dose-dependent manner, with a potency rank order of SPM greater than SPD greater than PUT. The PA stimulation required both RNA and protein synthesis, as evidenced by inhibition of polyamine-induced PA secretion by actinomycin D and cycloheximide. The inhibitors of polyamine biosynthesis methylglyoxal bis-(guanylhydrazone) (MGBG) and dl-(difluoromethyl) ornithine (DFMO) alone did not affect basal or polyamine-induced PA secretion, with the exception that MGBG reduced the effect of PUT. Polyamine-treated cells enhanced secretions of both tissue-type and urokinase-type PA. The results of the present study suggest that polyamines may play a role in the regulation of PA synthesis and secretion and that this function can be modified under pathophysiological conditions affecting cellular and tissue levels of polyamines.

Published
1988
Full Text
View/download PDF

35. Purification of decidual prolactin-releasing factor, a placental protein that stimulates prolactin release from human decidual tissue.

Author

Handwerger S, Capel D, Korner G, and Richards R

Subjects
Biological Assay, Female, Humans, Immunologic Techniques, In Vitro Techniques, Molecular Weight, Decidua metabolism, Placenta analysis, Placental Hormones isolation & purification, Pregnancy Proteins isolation & purification, Prolactin metabolism
Abstract

Decidual prolactin-releasing factor (PRL-RF), a placental protein that stimulates the release of prolactin from human decidual tissue, has been purified from conditioned medium of human placental explants. The purification scheme consisted of ethanol extraction, anion exchange chromatography on DEAE-cellulose, size exclusion chromatography on Spherogel TSK-3000, and either a) immunoaffinity chromatography using an antiserum to a partially purified PRL-RF preparation or b) acetic acid-urea/SDS 2-dimensional PAGE. The apparent molecular weight of the purified releasing factor, estimated by SDS-PAGE, was 23,500 Da; and the half-maximal dose for the acute stimulation of prolactin release from human decidual cells was 0.05-0.1 ug/ml (2.2-4.4 nM).

Published
1987
Full Text
View/download PDF

36. Differential solubilization of placental lactogen (PL)- and growth hormone-binding sites: further evidence for a unique PL receptor in fetal and maternal liver.

Author

Freemark M, Comer M, and Korner G

Subjects
Animals, Chemical Precipitation, Cross-Linking Reagents, Electrophoresis, Polyacrylamide Gel, Female, Iodine Radioisotopes, Liver embryology, Microsomes, Liver metabolism, Molecular Weight, Octoxynol, Polyethylene Glycols pharmacology, Pregnancy, Receptors, Prolactin drug effects, Receptors, Somatotropin drug effects, Solubility, Fetus metabolism, Growth Hormone metabolism, Liver metabolism, Placental Lactogen metabolism, Receptors, Peptide, Receptors, Prolactin metabolism, Receptors, Somatotropin metabolism
Abstract

Previous studies from this laboratory provided evidence for the existence of a specific placental lactogen (PL) receptor in tissues of fetal lambs and pregnant sheep. The PL receptor is structurally and functionally distinct from somatotropic (GH) and lactogenic (PRL) receptors, and there are conspicuous differences in the expression of the three receptors during ontogeny. The results of the present study indicate striking differences in the solubilization of PL- and GH-binding sites in maternal and fetal sheep liver. Radiolabeled ovine PL (oPL) bound specifically and with high affinity (Kd, 0.97 nM) to soluble detergent extracts of ovine fetal liver, but there was no specific binding of radiolabeled ovine GH (oGH) or oPRL to soluble extracts or insoluble fractions of fetal liver. When liver microsomes of pregnant sheep were extracted with Triton X-100, 80% of the [125I]oPL-binding sites were recovered in the soluble fraction, but 76% of the [125I]oGH binding sites were recovered in the insoluble pellet. Soluble extracts of maternal liver had high affinity for oPL (Kd, 1.45 nM), but low affinity for oGH (Kd 33 nM) and oPRL (Kd, 1-2 microM). On the other hand, Triton-insoluble fractions of maternal liver had high affinity for oGH (Kd, 0.95 nM) as well as oPL (Kd, 0.91 nM), but low affinity for oPRL (Kd, 1-2 microM). The subunit structure of the [125I]oPL-binding site in soluble fractions of fetal and maternal liver (mol wt, 38-47K) was distinct from that of the [125I]oGH-binding site in Triton-insoluble fractions of maternal liver (mol wt, 54/118K). These findings indicate that treatment of microsomal fractions of fetal and maternal sheep liver with Triton X-100 solubilizes the oPL receptor but not the oGH receptor. The differential solubilization of PL- and GH-binding sites may facilitate purification of the two distinct receptors and clarification of their respective roles in the regulation of fetal and postnatal growth.

Published
1988
Full Text
View/download PDF

Catalog

Books, media, physical & digital resources
See catalog results