Your search keyword '"Gunnar Ronquist"' showing total 304 results

1. Energy-requiring uptake of prostasomes and PC3 cell-derived exosomes into non-malignant and malignant cells

Author

Karl Göran Ronquist, Claire Sanchez, Louise Dubois, Dimitris Chioureas, Pedro Fonseca, Anders Larsson, Anders Ullén, Jeffrey Yachnin, Gunnar Ronquist, and Theocharis Panaretakis

Subjects

extracellular ATP, prostate cancer, extracellular vesicles, exosomes, prostasomes, ATPase, glycolysis, energy metabolism, exosome uptake, Cytology, QH573-671

Abstract

Epithelial cells lining the prostate acini release, in a regulated manner (exocytosis), nanosized vesicles called prostasomes that belong to the exosome family. Prostate cancer cells have preserved this ability to generate and export exosomes to the extracellular space. We previously demonstrated that human prostasomes have an ATP-forming capacity. In this study, we compared the capacity of extracellular vesicles (EVs) to generate ATP between normal seminal prostasomes and exosomes secreted by PC3 cells (PC3 exosomes), a prostate cancer cell line. Proteomic analyses identified enzymes of the glycolytic chain in both prostasomes and PC3 exosomes, and we found that both of them were capable of generating ATP when supplied with substrates. Notably, the net production of extracellular ATP was low for prostasomes due to a high ATPase activity contrary to an elevated net ATP level for PC3 exosomes because of their low ATPase activity. The uptake of the 2 types of EVs by normal prostate epithelial cells (CRL2221) and prostate cancer cells (PC3) was visualized and measured, demonstrating differential kinetics. Interestingly, this uptake was dependent upon an ongoing glycolytic flux involving extracellular ATP formation by EVs and/or intracellular ATP produced from the recipient cells. We conclude that the internalization of EVs into recipient cells is an energy-requiring process also demanding an active V-ATPase and the capacity of EVs to generate extracellular ATP may play a role in this process.

Published

2016

2. Myocardial ischemic preconditioning in a porcine model leads to rapid changes in cardiac extracellular vesicle messenger RNA content

Author

Kristina Svennerholm, Pouria Rodsand, Urban Hellman, Marie Lundholm, Anders Waldenström, Björn Biber, Gunnar Ronquist, and Michael Haney

Subjects

Extracellular vesicles, mRNA, Transcription, Ischemic preconditioning, Myocardium, Diseases of the circulatory (Cardiovascular) system, RC666-701

Abstract

Background: Extracellular vesicles (EVs) are thought to exert protective effects after ischemic and remote ischemic preconditioning. It is not well understood which EV content factors are most relevant for protective effects. We hypothesize that ischemic preconditioning leads to qualitative changes in EV mRNA content and quantitative changes in EV size and number. Methods: Using an in vivo porcine ischemic preconditioning model, EVs were collected from coronary venous blood, and isolated by differential ultracentrifugations. The presence and purity of EV were verified by electron microscopy and Western blot, and EV number was assessed by nanoparticle tracking analysis. The mRNA EV was identified by microarray. Results: Gene ontology analysis showed enrichment of EV mRNA coding for proteins associated with regulation of transcription, translation, extracellular matrix, morphogenic development and feeding behavior. There were 11,678 different mRNA transcripts detected in EV, where a total of 1103 was significantly increased or decreased after preconditioning, of which 638 mRNA sequences were up-regulated and/or emerged due to preconditioning. Several of them have known association with ischemic preconditioning. There was no significant difference in EV quantity or size before and after preconditioning. Conclusions: These findings demonstrate in an in vivo model that myocardial ischemic preconditioning influences the composition of mRNA in EV, including gene transcripts for proteins associated with the protective effect of ischemic preconditioning. The finding that preconditioned parental cells release EV containing mRNA that is qualitatively different from those released by non-preconditioned cells shows the importance of the external milieu on parental cell EV production.

Published

2015

3. Growth factor stimulation of cardiomyocytes induces changes in the transcriptional contents of secreted exosomes

Author

Gunnar Ronquist, Urban Hellman, Göran Larsson, Linus Malm, Nina Gennebäck, Anders Waldenström, and Stellan Mörner

Subjects

extracellular vesicles, exosomes, cardiomyocytes, growth factors, gene expression, Cytology, QH573-671

Abstract

Exosomes are nano-sized extracellular vesicles, released from various cells, which can stimulate or repress responses in targets cells. We recently reported that cultured cardiomyocytes are able to release exosomes and that they, in turn, are involved in facilitating events in target cells by alteration of gene expression. We investigated whether external stimuli of the cardiomyocyte might influence the transcriptional content of the released exosomes.Exosomes were isolated from media collected from cultured cardiomyocytes (HL-1) with or without growth factor treatment (TGF-β2 and PDGF-BB), with a series of differential centrifugations, including preparative ultracentrifugation and separation with a sucrose gradient. The exosomes were characterized with dynamic light scattering (DLS), electron microscopy (EM) and Western blot and analyzed with Illumina whole genome microarray gene expression.The exosomes were rounded in shape and had an average size of 50–90 nm in diameter with no difference between treatment groups. Analysis of the mRNA content in repeated experiments conclusively revealed 505 transcripts in the control group, 562 in the TGF-β2-treated group and 300 in the PDGF-BB-treated group. Common transcripts (217) were found in all 3 groups.We show that the mode of stimulation of parental cells affects the characteristics of exosomes released. Hence, there is a difference in mRNA content between exosomes derived from cultured cardiomyocytes stimulated, or not stimulated, with growth factors. We also conclude that all exosomes contain a basic package consisting of ribosomal transcripts and mRNAs coding for proteins with functions within the energy supply system. To access the supplementary material to this article, please see Supplementary files under Article Tools online.

Published

2013

4. DNA Content in Extracellular Vesicles Isolated from Porcine Coronary Venous Blood Directly after Myocardial Ischemic Preconditioning.

Author

Kristina Svennerholm, Pouria Rodsand, Urban Hellman, Anders Waldenström, Marie Lundholm, Dag Ahrén, Björn Biber, Gunnar Ronquist, and Michael Haney

Subjects

Medicine, Science

Abstract

BACKGROUND:Extracellular vesicles (EV) are nano-sized membranous structures released from most cells. They have the capacity to carry bioactive molecules and gene expression signals between cells, thus mediating intercellular communication. It is believed that EV confer protection after ischemic preconditioning (IPC). We hypothesize that myocardial ischemic preconditioning will lead to rapid alteration of EV DNA content in EV collected from coronary venous effluent. MATERIALS AND METHODS:In a porcine myocardial ischemic preconditioning model, EV were isolated from coronary venous blood before and after IPC by differential centrifugation steps culminating in preparative ultracentrifugation combined with density gradient ultracentrifugation. The EV preparation was validated, the DNA was extracted and further characterized by DNA sequencing followed by bioinformatics analysis. RESULTS:Porcine genomic DNA fragments representing each chromosome, including mitochondrial DNA sequences, were detected in EV isolated before and after IPC. There was no difference detected in the number of sequenced gene fragments (reads) or in the genomic coverage of the sequenced DNA fragments in EV isolated before and after IPC. Gene ontology analysis showed an enrichment of genes coding for ion channels, enzymes and proteins for basal metabolism and vesicle biogenesis and specific cardiac proteins. CONCLUSIONS:This study demonstrates that porcine EV isolated from coronary venous blood plasma contain fragments of DNA from the entire genome, including the mitochondria. In this model we did not find specific qualitative or quantitative changes of the DNA content in EV collected immediately after an in vivo myocardial IPC provocation. This does not rule out the possibility that EV DNA content changes in response to myocardial IPC which could occur in a later time frame.

Published

2016

5. Cardiomyocyte microvesicles contain DNA/RNA and convey biological messages to target cells.

Author

Anders Waldenström, Nina Gennebäck, Urban Hellman, and Gunnar Ronquist

Subjects

Medicine, Science

Abstract

BACKGROUND: Shedding microvesicles are membrane released vesicles derived directly from the plasma membrane. Exosomes are released membrane vesicles of late endosomal origin that share structural and biochemical characteristics with prostasomes. Microvesicles/exosomes can mediate messages between cells and affect various cell-related processes in their target cells. We describe newly detected microvesicles/exosomes from cardiomyocytes and depict some of their biological functions. METHODOLOGY/PRINCIPAL FINDINGS: Microvesicles/exosomes from media of cultured cardiomyocytes derived from adult mouse heart were isolated by differential centrifugation including preparative ultracentrifugation and identified by transmission electron microscopy and flow cytometry. They were surrounded by a bilayered membrane and flow cytometry revealed presence of both caveolin-3 and flotillin-1 while clathrin and annexin-2 were not detected. Microvesicle/exosome mRNA was identified and out of 1520 detected mRNA, 423 could be directly connected in a biological network. Furthermore, by a specific technique involving TDT polymerase, 343 different chromosomal DNA sequences were identified in the microvesicles/exosomes. Microvesicle/exosomal DNA transfer was possible into target fibroblasts, where exosomes stained for DNA were seen in the fibroblast cytosol and even in the nuclei. The gene expression was affected in fibroblasts transfected by microvesicles/exosomes and among 333 gene expression changes there were 175 upregulations and 158 downregulations compared with controls. CONCLUSIONS/SIGNIFICANCE: Our study suggests that microvesicles/exosomes released from cardiomyocytes, where we propose that exosomes derived from cardiomyocytes could be denoted "cardiosomes", can be involved in a metabolic course of events in target cells by facilitating an array of metabolism-related processes including gene expression changes.

Published

2012

6. Prostasomes (Exosomes) Mediate Functional Abilities to Recipient Cells through Transfer of Proteins and Nucleic Acids: A Comprehensive Model for Exosomal Intercellular Communication

Author

Gunnar Ronquist and Anders Waldenström

Subjects

General Medicine

Abstract

The prostasome is the first described exosome and constitutes the third communication system between cells mediating messages besides gap junctions and soluble compounds such as hormones. Exosomes are nanometer vesicles surrounded by a lipid bilayered membrane and released by most cell types including malignant cells. The exosomal messenger system reaches distant cells even on the other side of the blood brain barrier. In this way they are able to interact with their target cells for delivery of their cargo. We here describe prostasomal properties in more detail thus exemplifying common exosomal characteristics. Myocardial derived exosomes (cardiosomes), are also described in order to highlight other common biological functions including damaged tissue, i.e. tissue repair. Abnormal tissue such as malignant progression can be driven by cancer cell derived exosomes, believed mainly to be mediated by different forms of short RNAs exerting their action through specific signaling pathways related to metastases, therapeutic resistance and immunosuppression.

Published

2021

7. Human erythrocyte-derived nanovesicles can readily be loaded with doxorubicin and act as anticancer agents

Author

Liza Löf, Anders Larsson, Anders Waldenström, Masood Kamali-Moghaddam, Louise Dubois, Kjell Hultenby, K. Göran Ronquist, and Gunnar Ronquist

Subjects

Drug, Klinisk laboratoriemedicin, Chemistry, Clinical Laboratory Medicine, media_common.quotation_subject, medicine, Doxorubicin, General Medicine, Pharmacology, media_common, medicine.drug

Abstract

Purpose: In future therapeutics new formulas are needed that assure lower doses, fewer side effects, targeted administration and protection of the drug from degradation. In a first step to fulfil the requirements defined above, we carried out an in vitro study by developing a new procedure to encapsulate drugs using native vesicles first from prostasomes and then from erythrocyte membranes known to be well tolerated. The new method for production of drug delivery vesicles utilized osmotic loading of detergent resistant membranes (DRMs). Materials and methods: DRMs of prostasomes and prepared human erythrocyte membranes were extracted and separated in a sucrose gradient at a density of 1.10 g/mL containing 1% Triton X-100. These DRMs were characterized by electron microscopy (transmission and scanning EM) and loaded with low and high molecular compounds. PC3 prostate cancer cells were treated with doxorubicin loaded DRMs in triplicate. DAPI (nuclear fluorescent stain) was included and fluorescence microscopic pictures were taken before the cells were trypsinized and counted after 48h. Results: The content of the well separated band was observed ultrastructurally as small spherical, double layered membrane vesicles, (DRM vesicles) which harbored hyperosmolar sucrose of the gradient. Encapsulated hyperosmolar sucrose induced a transient osmotic lysis of the DRM vesicles when suspended in isotonic buffer containing loading molecules allowing vesicular inclusion. After this proof of concept, the method was finally employed for doxorubicin loading of DRM vesicles from human erythrocytes. When incubating such vesicles with PC3 cells a complete arrest of growth was observed in sharp contrast to PC3 cells incubated with plain doxorubicin in similar conditions. Conclusion: The present results open up new possibilities for using DRM vesicles as drug delivery vesicles. Louise Dubois and Liza Löf contributed equally to this work.

Published

2018

8. Proteomic Profiling of Detergent Resistant Membranes (Lipid Rafts) of Prostasomes

Author

Karl Göran Ronquist, Bo Ek, Louise Dubois, Anders Larsson, and Gunnar Ronquist

Subjects

Male, Proteome, Liquid Phase Microextraction, Octoxynol, Tetraspanins, Liquid ordered phase, Detergents, Exosomes, Biochemistry, Mass Spectrometry, Analytical Chemistry, chemistry.chemical_compound, Membrane Microdomains, Phosphatidylcholine, Centrifugation, Density Gradient, Humans, Molecular Biology, Lipid raft, Endosomal Sorting Complexes Required for Transport, Research, Bilayer, Vesicle, Prostate, Molecular Sequence Annotation, Lipids, chemistry, ras Proteins, lipids (amino acids, peptides, and proteins), Density gradient ultracentrifugation, Prostasomes, Sphingomyelin, Chromatography, Liquid

Abstract

Prostasomes are exosomes derived from prostate epithelial cells through exocytosis by multivesicular bodies. Prostasomes have a bilayered membrane and readily interact with sperm. The membrane lipid composition is unusual with a high contribution of sphingomyelin at the expense of phosphatidylcholine and saturated and monounsaturated fatty acids are dominant. Lipid rafts are liquid-ordered domains that are more tightly packed than the surrounding nonraft phase of the bilayer. Lipid rafts are proposed to be highly dynamic, submicroscopic assemblies that float freely within the liquid disordered membrane bilayer and some proteins preferentially partition into the ordered raft domains. We asked the question whether lipid rafts do exist in prostasomes and, if so, which proteins might be associated with them. Prostasomes of density range 1.13–1.19g/ml were subjected to density gradient ultracentrifugation in sucrose fabricated by phosphate buffered saline (PBS) containing 1% Triton X-100 with capacity for banding at 1.10 g/ml, i.e. the classical density of lipid rafts. Prepared prostasomal lipid rafts (by gradient ultracentrifugation) were analyzed by mass spectrometry. The clearly visible band on top of 1.10g/ml sucrose in the Triton X-100 containing gradient was subjected to liquid chromatography-tandem MS and more than 370 lipid raft associated proteins were identified. Several of them were involved in intraluminal vesicle formation, e.g. tetraspanins, ESCRTs, and Ras-related proteins. This is the first comprehensive liquid chromatography-tandem MS profiling of proteins in lipid rafts derived from exosomes. Data are available via ProteomeXchange with identifier PXD002163.

Published

2015

9. Myocardial ischemic preconditioning in a porcine model leads to rapid changes in cardiac extracellular vesicle messenger RNA content

Author

Marie Lundholm, Michael Haney, Urban Hellman, Gunnar Ronquist, Pouria Rodsand, Björn Biber, Kristina Svennerholm, and Anders Waldenström

Subjects

Pathology, medicine.medical_specialty, lcsh:Diseases of the circulatory (Cardiovascular) system, Cardiac & Cardiovascular Systems, Cell- och molekylärbiologi, mRNA, Biology, Extracellular vesicles, Article, Transcription (biology), medicine, myocardium, Cardiac and Cardiovascular Systems, Messenger RNA, Ischemic preconditioning, Kardiologi, Myocardium, Extracellular vesicle, Cell biology, Cell and molecular biology, ischemic preconditioning, lcsh:RC666-701, Cardiology and Cardiovascular Medicine, extracellular vesicles, transcription, Transcription, Cell and Molecular Biology

Abstract

Background: Extracellular vesicles (EVs) are thought to exert protective effects after ischemic and remote ischemic preconditioning. It is not well understood which EV content factors are most relevant for protective effects. We hypothesize that ischemic preconditioning leads to qualitative changes in EV mRNA content and quantitative changes in EV size and number. Methods: Using an in vivo porcine ischemic preconditioning model, EVs were collected from coronary venous blood, and isolated by differential ultracentrifugations. The presence and purity of EV were verified by electron microscopy and Western blot, and EV number was assessed by nanoparticle tracking analysis. The mRNA EV was identified by microarray. Results: Gene ontology analysis showed enrichment of EV mRNA coding for proteins associated with regulation of transcription, translation, extracellular matrix, morphogenic development and feeding behavior. There were 11,678 different mRNA transcripts detected in EV, where a total of 1103 was significantly increased or decreased after preconditioning, of which 638 mRNA sequences were up-regulated and/or emerged due to preconditioning. Several of them have known association with ischemic preconditioning. There was no significant difference in EV quantity or size before and after preconditioning. Conclusions: These findings demonstrate in an in vivo model that myocardial ischemic preconditioning influences the composition of mRNA in EV, including gene transcripts for proteins associated with the protective effect of ischemic preconditioning. The finding that preconditioned parental cells release EV containing mRNA that is qualitatively different from those released by non-preconditioned cells shows the importance of the external milieu on parental cell EV production.

Published

2015

10. Tracing Cellular Origin of Human Exosomes Using Multiplex Proximity Extension Assays

Author

Pia Larssen, Lotta Wik, Paulo Czarnewski, Maria Eldh, Liza Löf, K. Göran Ronquist, Louise Dubois, Eva Freyhult, Caroline J. Gallant, Johan Oelrich, Anders Larsson, Gunnar Ronquist, Eduardo J. Villablanca, Ulf Landegren, Susanne Gabrielsson, and Masood Kamali-Moghaddam

Subjects

Male, Principal Component Analysis, Milk, Human, Research, Prostate, Exosomes, Biochemistry, Body Fluids, Cell Line, High-Throughput Screening Assays, Analytical Chemistry, Cell-Derived Microparticles, Organ Specificity, MCF-7 Cells, Humans, Female, Additions and Corrections, K562 Cells, Molecular Biology, Biomarkers

Abstract

Extracellular vesicles (EVs) are membrane-coated objects such as exosomes and microvesicles, released by many cell-types. Their presence in body fluids and the variable surface composition and content render them attractive potential biomarkers. The ability to determine their cellular origin could greatly move the field forward. We used multiplex proximity extension assays (PEA) to identify with high specificity and sensitivity the protein profiles of exosomes of different origins, including seven cell lines and two different body fluids. By comparing cells and exosomes, we successfully identified the cells originating the exosomes. Furthermore, by principal component analysis of protein patterns human milk EVs and prostasomes released from prostate acinar cells clustered with cell lines from breast and prostate tissues, respectively. Milk exosomes uniquely expressed CXCL5, MIA, and KLK6, whereas prostasomes carried NKX31, GSTP1, and SRC, highlighting that EVs originating from different origins express distinct proteins. In conclusion, PEA provides a powerful protein screening tool in exosome research, for purposes of identifying the cell source of exosomes, or new biomarkers in diseases such as cancer and inflammation.

Published

2017

11. High Concentrations of the Angiogenic Peptide VEGF-A in Seminal Fluid and its Association to Prostasomes

Author

Karl Göran Ronquist, Anders Larsson, Lena M. S. Carlsson, Rune Elisasson, Gunnar Ronquist, and Louise Dubois

Subjects

Male, Vascular Endothelial Growth Factor A, 030213 general clinical medicine, Angiogenesis, Semen, Peptide, Enzyme-Linked Immunosorbent Assay, 030204 cardiovascular system & hematology, General Biochemistry, Genetics and Molecular Biology, Flow cytometry, Andrology, 03 medical and health sciences, chemistry.chemical_compound, Extracellular Vesicles, 0302 clinical medicine, Blood plasma, medicine, Humans, chemistry.chemical_classification, medicine.diagnostic_test, Chemistry, Flow Cytometry, Vascular endothelial growth factor, Vascular endothelial growth factor A, Prostasomes, Reagent Kits, Diagnostic

Abstract

Background Angiogenesis is the formation of new blood vessels by capillary sprouting from pre-existing vessels. This process is associated with increased expression of angiogenic factors like vascular endothelial growth factor (VEGF). The VEGF family consists of five members denoted VEGF-A, B, C, D and placenta growth factor (PlGF). Prostasomes are exosome-like extracellular vesicles existing in seminal plasma. The present study aimed at investigating the possible relationship between VEGF-A in seminal fluid and blood plasma and the prostasomal association of VEGF-A. Methods Measurement of VEGF-A concentrations was carried out in seminal plasma from 40 males and in blood plasma from 40 male blood donors utilizing commercial ELISA kits. The prostasomal association of VEGF-A was investigated by flow cytometry. Results We found highly elevated concentrations of VEGF-A in seminal fluid (median value 150000 pg/mL) compared with those of blood plasma. Flow cytometric analysis showed that VEGF-A is bound to the surface of prostasomes. Conclusions Prostasomes and seminal plasma contain the angiogenic factor VEGF-A in high concentrations exceeding that of blood plasma by 1000 times.

Published

2017

12. A novel model for studies of blood-mediated long-term responses to cellular transplants

Author

Gunnar Ronquist, Jaan Hong, Olle Korsgren, Maria Hårdstedt, Susanne Lindblom, and Bo Nilsson

Subjects

Blood Glucose, Time Factors, leukocytes, Cell Survival, Cell Transplantation, Antithrombin III, Islets of Langerhans Transplantation, Energy metabolism, electrolyte homeostasis, Hemolysis, Thromboplastin, Islets of Langerhans, Cell transplantation, Chlorides, Cations, energy metabolism, Animals, Humans, Medicine, coagulation, Complement Activation, Pancreas, Cell survival, Blood gas analysis, Ions, blood physiology, business.industry, Osmolar Concentration, General Medicine, Blood physiology, Carbon Dioxide, Hydrogen-Ion Concentration, Oxygen, Glucose, Peptide Hydrolases, Immunology, Original Article, Biocompatibility, Collagen, Rabbits, Blood Gas Analysis, business, Neuroscience, Electrolyte homeostasis

Abstract

Aims Interaction between blood and bio-surfaces is important in many medical fields. With the aim of studying blood-mediated reactions to cellular transplants, we developed a whole-blood model for incubation of small volumes for up to 48 h. Methods Heparinized polyvinyl chloride tubing was cut in suitable lengths and sealed to create small bags. Multiple bags, with fresh venous blood, were incubated attached to a rotating wheel at 37°C. Physiological variables in blood were monitored: glucose, blood gases, mono- and divalent cations and chloride ions, osmolality, coagulation (platelet consumption, thrombin-antithrombin complexes (TAT)), and complement activation (C3a and SC5b-9), haemolysis, and leukocyte viability. Results Basic glucose consumption was high. Glucose depletion resulted in successive elevation of extracellular potassium, while sodium and calcium ions decreased due to inhibition of energy-requiring ion pumps. Addition of glucose improved ion balance but led to metabolic acidosis. To maintain a balanced physiological environment beyond 6 h, glucose and sodium hydrogen carbonate were added regularly based on analyses of glucose, pH, ions, and osmotic pressure. With these additives haemolysis was prevented for up to 72 h and leukocyte viability better preserved. Despite using non-heparinized blood, coagulation and complement activation were lower during long-term incubations compared with addition of thromboplastin and collagen. Conclusion A novel whole-blood model for studies of blood-mediated responses to a cellular transplant is presented allowing extended observations for up to 48 h and highlights the importance of stringent evaluations and adjustment of physiological conditions.

Published

2014

13. Prostasomes from four different species are able to produce extracellular adenosine triphosphate (ATP)

Author

Patrice Humblot, Bo Ek, Jane M. Morrell, Anders Larsson, K. Göran Ronquist, Anneli Stavreus-Evers, Bodil Ström Holst, and Gunnar Ronquist

Subjects

Male, Endosome, Biophysics, Context (language use), Biology, Biochemistry, chemistry.chemical_compound, Extracellular ATP, Adenosine Triphosphate, Dogs, Prostasomes, Extracellular, Animals, Humans, Horses, Molecular Biology, Seminal plasma, chemistry.chemical_classification, Organelles, Vesicle, Energy metabolism, Microvesicles, Cell biology, Enzyme, chemistry, Cattle, Electrophoresis, Polyacrylamide Gel, Adenosine triphosphate

Abstract

Background Prostasomes are extracellular vesicles. Intracellularly they are enclosed by another larger vesicle, a so called “storage vesicle” equivalent to a multivesicular body of late endosomal origin. Prostasomes in their extracellular context are thought to play a crucial role in fertilization. Methods Prostasomes were purified according to a well worked-out schedule from seminal plasmas obtained from human, canine, equine and bovine species. The various prostasomes were subjected to SDS-PAGE separation and protein banding patterns were compared. To gain knowledge of the prostasomal protein systems pertaining to prostasomes of four different species proteins were analyzed using a proteomic approach. An in vitro assay was employed to demonstrate ATP formation by prostasomes of different species. Results The SDS-PAGE banding pattern of prostasomes from the four species revealed a richly faceted picture with most protein bands within the molecular weight range of 10–150 kDa. Some protein bands seemed to be concordant among species although differently expressed and the number of protein bands of dog prostasomes seemed to be distinctly fewer. Special emphasis was put on proteins involved in energy metabolic turnover. Prostasomes from all four species were able to form extracellular adenosine triphosphate (ATP). ATP formation was balanced by ATPase activity linked to the four types of prostasomes. Conclusion These potencies of a possession of functional ATP-forming enzymes by different prostasome types should be regarded against the knowledge of ATP having a profound effect on cell responses and now explicitly on the success of the sperm cell to fertilize the ovum. General significance This study unravels energy metabolic relationships of prostasomes from four different species.

Published

2013

14. High levels of cathepsins B, L and S in human seminal plasma and their association with prostasomes

Author

Lena Carlsson, R Eliasson, Gunnar Ronquist, Göran Ronquist, N Egberg, Anders Larsson, and S Inayat

Subjects

Adult, Male, medicine.medical_specialty, Cathepsin L, Urology, Semen, Cathepsin B, Endocrinology, Internal medicine, medicine, Humans, Aged, Cathepsin S, Cathepsin, biology, Cathepsins B, Chemistry, Secretory Vesicles, Prostate, Epithelial Cells, General Medicine, Middle Aged, Serum samples, Cathepsins, biology.protein, Prostasomes, Biomarkers

Abstract

Semen is a heterogenous and complex fluid with different functions, some of them well known, others still obscure. The aim of this study was to investigate the presence of cathepsins B, S and L in human seminal plasma and their possible associations with other semen variables. Cathepsin B, L and S concentrations were measured in seminal plasma from 99 men utilising commercial ELISA kits. Seminal plasma cathepsin B was approximately 70 times higher, while the cathepsin L values were approximately 500 times higher and the cathepsin S values approximately 40 times higher in seminal plasma than in a group of serum samples. The study shows that seminal plasma contains high levels of cathepsins B, L and S. All three cathepsins were also bound to the surface of prostasomes.

Published

2012

15. Prostasomes are mediators of intercellular communication: from basic research to clinical implications

Author

Gunnar Ronquist

Subjects

business.industry, Endosome, medicine.disease, Microvesicles, Cell biology, Andrology, Prostate cancer, medicine.anatomical_structure, Prostate, Internal Medicine, Extracellular, Medicine, Prostasomes, business, Receptor, Intracellular

Abstract

Ronquist G (University Hospital, Uppsala, Sweden). Prostasomes are mediators of intercellular communication: from basic research to clinical implications (Review). J Intern Med 2012; 271: 400–413 Abstract. Prostasomes are nanosized microvesicles secreted by acinar epithelial cells of the prostate gland. Furthermore, they are intracellular microvesicles inside another larger vesicle, a so-called storage vesicle, equivalent to multivesicular bodies of late endosomal origin. Prostasomes are thought to play an important role in intercellular communication by direct interaction primarily between the immobile acinar cells of the prostate gland and the mobile spermatozoa. Prostasomes transfer not only membrane components but also genetic material to spermatozoa. They are rich in various transferable bioactive molecules (e.g. receptors and enzymes) that promote the fertilizing ability of spermatozoa. In this review, the pleiotropic biological effects of prostasomes that are relevant for successful fertilization will be discussed. The ability to synthesize and export prostasomes to the extracellular space is observed not only in normal prostate epithelial cells but also in malignant prostate cells. Release of prostasomes by prostate cancer cells suggests a role in malignant cell growth and proliferation. These findings may provide new therapeutic and diagnostic strategies.

Published

2011

16. Ischaemic preconditioning reduces myocardial calcium overload in coronary-occluded pig hearts shown by continuous in vivo assessment using microdialysis

Author

Michael Haney, Björn Biber, Pernilla Abrahamsson, Anders Waldenström, Katarina Ahlström, Gunnar Ronquist, Göran Johansson, Anna-Maja Åberg, and Philip Hauck

Subjects

Myocardial ischaemia, Microdialysis, biology, Physiology, business.industry, ATPase, Ischemia, chemistry.chemical_element, General Medicine, Pharmacology, Calcium, medicine.disease, chemistry, Atp depletion, In vivo, Physiology (medical), Anesthesia, medicine, biology.protein, Myocardial calcium, business

Abstract

During ischaemia, ATP depletion leads to insufficient fuelling for Na+/K+ ATPase, decreased electrochemical potential and increased influx of calcium ions. This study demonstrated a means to assess ...

Published

2011

17. Prostasomal DNA characterization and transfer into human sperm

Author

Anders Isaksson, Julius Hreinsson, Lena Carlsson, Anders Larsson, Göran Ronquist, Gunnar Ronquist, and Anneli Stavreus-Evers

Subjects

Cell Biology, Biology, Molecular biology, Genome, Sperm, Microvesicles, chemistry.chemical_compound, chemistry, Agarose gel electrophoresis, Genetics, Fluorescence microscope, Prostasomes, Gene, DNA, Developmental Biology

Abstract

Human prostasomes, exosome-like microvesicles secreted by acinar cells of the prostate gland, contain chromosomal DNA. Agarose gel electrophoresis of DNA from seminal prostasomes displayed fragments of over 12 kb and smaller, with a distinct band around 1 kb that was excised, cloned, and sequenced. The sequences showed 8 out of 25 clones (32%) originating from genes. We elaborated the concept further by carrying out a genome-wide DNA copy number analysis of prostasomal DNA, hypothesizing that human prostasomes contain fragments of DNA randomly selected from the entire genome. Acridine orange-stained prostasomes were incubated with freshly prepared sperm for different times, and a transfer of acridine orange-stained prostasomal DNA to sperm (preferentially the head region) was observed. Fluorescence microscopy of slices in the center of 14 optical slides of the sperm head displayed an even fluorescence rather than a halo-like one, indicating DNA-uptake rather than just binding along the sperm head membrane.

Published

2011

18. Multiple recognition assay reveals prostasomes as promising plasma biomarkers for prostate cancer

Author

Junhong Yan, Lena Carlsson, Gholamreza Tavoosidana, Gunnar Ronquist, Spyros Darmanis, Elke Eltze, Di Wu, Tim Conze, Axel Semjonow, Pia Ek, Ulf Landegren, Masood Kamali-Moghaddam, and Anders Larsson

Subjects

Male, medicine.medical_specialty, medicine.medical_treatment, Proximity ligation assay, Sensitivity and Specificity, Antibodies, 03 medical and health sciences, Prostate cancer, 0302 clinical medicine, Antigen, Semen, Prostate, Internal medicine, Blood plasma, Humans, Medicine, Pharmacology (medical), Transport Vesicles, Early Detection of Cancer, Aged, 030304 developmental biology, Immunoassay, 0303 health sciences, Multidisciplinary, biology, Prostatectomy, business.industry, Prostatic Neoplasms, Cancer, Middle Aged, Biological Sciences, medicine.disease, Microvesicles, 3. Good health, Endocrinology, medicine.anatomical_structure, Oncology, Case-Control Studies, 030220 oncology & carcinogenesis, Immunology, biology.protein, Cancer research, Biomarker (medicine), Prostasomes, Antibody, business, Biomarkers

Abstract

Prostasomes are microvesicles (mean diameter, 150 nm) that are produced and secreted by normal and malignant prostate acinar cells. It has been hypothesized that invasive growth of malignant prostate cells may cause these microvesicles, normally released into seminal fluid, to appear in interstitial space and therewith into peripheral circulation. The suitability of prostasomes as blood biomarkers in patients with prostate cancer was tested by using an expanded variant of the proximity ligation assay (PLA). We developed an extremely sensitive and specific assay (4PLA) for detection of complex target structures such as microvesicles in which the target is first captured via an immobilized antibody and subsequently detected by using four other antibodies with attached DNA strands. The requirement for coincident binding by five antibodies to generate an amplifiable reporter results in both increased specificity and sensitivity. The assay successfully detected significantly elevated levels of prostasomes in blood samples from patients with prostate cancer before radical prostatectomy, compared with controls and men with benign biopsy results. The medians for prostasome levels in blood plasma of patients with prostate cancer were 2.5 to sevenfold higher compared with control samples in two independent studies, and the assay also distinguished patients with high and medium prostatectomy Gleason scores (8/9 and 7, respectively) from those with low score (≤6), thus reflecting disease aggressiveness. This approach that enables detection of prostasomes in peripheral blood may be useful for early diagnosis and assessment of prognosis in organ-confined prostate cancer.

Published

2011

19. Ischaemic pre-conditioning means an increased adenosine metabolism with decreased glycolytic flow in ischaemic pig myocardium

Author

Pernilla Abrahamsson, Gunnar Ronquist, Anders Waldenström, Philip Hauck, Björn Biber, Katarina Ahlström, Michael Haney, Anna-Maja Åberg, and Göran Johansson

Subjects

medicine.medical_specialty, Taurine, Microdialysis, Glycogen, business.industry, fungi, Ischemia, food and beverages, Hemodynamics, General Medicine, medicine.disease, Adenosine, chemistry.chemical_compound, Anesthesiology and Pain Medicine, Endocrinology, Biochemistry, chemistry, Internal medicine, medicine, Ischemic preconditioning, Glycolysis, business, medicine.drug

Abstract

This association between increased adenosine turnover and decreased glycolytic flow during prolonged ischaemia in response to IP can possibly be explained by the competitive effect for the metaboli ...

Published

2010

20. Secretions from seminal vesicles lack characteristic markers for prostasomes

Author

Anders Larsson, Lena M. S. Carlsson, O. Nilsson, Gunnar Ronquist, Göran Sahlén, and Bo Johan Norlén

Subjects

Male, medicine.medical_specialty, clusterin, markers, Biology, prostasomes, Flow cytometry, Seminal vesicle, Microscopy, Electron, Transmission, Prostate, Internal medicine, medicine, Animals, Humans, Secretion, HSP70, CD26, seminal-vesicle, Gel electrophoresis, medicine.diagnostic_test, electron microscopy, Vesicle, Seminal Vesicles, General Medicine, Flow Cytometry, Cell biology, medicine.anatomical_structure, Endocrinology, Ultrastructure, CD10, Prostasomes, Original Article, Electrophoresis, Polyacrylamide Gel, CD13

Abstract

Background Prostasomes are suggested to be produced in the prostate gland. Although biochemical studies support this, some immunohistochemical findings indicate that also the seminal vesicles could be a source of prostasomes. Therefore, we have compared the secretion of the vesicles with that of the prostate using biochemical and ultrastructural techniques. Methods Ultracentrifuged pellets of substance from seminal vesicle secretions were analysed by sodium dodecyl sulfate-polyacrylamide gel electrophoresis (SDS-PAGE) and flow cytometry. The secretory cells of the seminal vesicles were examined with transmission electron microscopy. These findings were then compared with published results from similar studies of the prostate secretory cells. Results In SDS-PAGE, the seminal vesicle pellets lacked the three prostasome-characteristic CD-markers, namely CD10, CD13, and CD26, but expressed two proteins of about 55 kDa and 70 kDa, corresponding to clusterin and heat shock protein (HSP70). Flow cytometry showed the presence of secretion particles in the seminal pellet, although of a smaller size than that of the prostasomes. Electron microscopy of the luminal part of the cells in the seminal vesicles demonstrated many secretion granules, each enclosed in a vesicle with a size of about 1 μm. Conclusions Pelleted seminal vesicle secretion is different to prostate secretion in several ways. No prostasome characteristics were detected in the pelleted seminal vesicle secretion.

Published

2010

21. Prostasome Involvement in the Development and Growth of Prostate Cancer~!2009-07-10~!2009-12-09~!2010-02-11~!

Author

Gunnar Ronquist, Bo Nilsson, Adil A. Babiker, and Kristina Nilsson Ekdahl

Subjects

Pathology, medicine.medical_specialty, business.industry, Urology, Semen, medicine.disease, humanities, Prostate cancer, medicine.anatomical_structure, Oncology, Prostate, medicine, Prostasomes, Secretion, business

Abstract

Prostasomes are extracellularly occurring submicron, membrane-surrounded organelles produced by the epithelial cells of the prostate and present in semen after secretion. Even dedifferentiated pros ...

Published

2010

22. Mapping pro- and antiangiogenic factors on the surface of prostasomes of normal and malignant cell origin

Author

Bo Nilsson, Adil A. Babiker, Peetra U. Magnusson, Kristina Nilsson Ekdahl, and Gunnar Ronquist

Subjects

Pathology, medicine.medical_specialty, Angiogenesis, business.industry, Urology, education, medicine.disease, Endothelin 1, Prostate cancer, Oncology, DU145, Thrombospondin 1, LNCaP, cardiovascular system, medicine, Prostasomes, Endostatin, business

Abstract

BACKGROUND. Angiogenesis is the formation of new blood vessels by capillary sprouting from pre-existing vessels. Tumor growth is angiogenesis-dependent and the formation of new blood vessels is ass ...

Published

2010

23. Metabolic responses in ischemic myocardium after inhalation of carbon monoxide

Author

Pernilla Abrahamsson, Per Strandén, Katarina Ahlström, Michael Haney, Gunnar Ronquist, Anna-Maja Åberg, Göran Johansson, Björn Biber, and Anders Waldenström

Subjects

medicine.medical_specialty, Microdialysis, Central Venous Pressure, Swine, Ischemic myocardium, Myocardial Ischemia, Ischemia, Blood Pressure, Carbohydrate metabolism, Protective Agents, chemistry.chemical_compound, Adenosine Triphosphate, Animal model, Heart Rate, Internal medicine, Pyruvic Acid, Animals, Medicine, Lactic Acid, Carbon Monoxide, Inhalation, business.industry, Myocardium, General Medicine, medicine.disease, Adenosine Diphosphate, Glucose, Anesthesiology and Pain Medicine, Carboxyhemoglobin, chemistry, Coronary occlusion, Anesthesia, Cardiology, Female, Energy Metabolism, business, Carbon monoxide

Abstract

To clarify the mechanisms of carbon monoxide (CO) tissue-protective effects, we studied energy metabolism in an animal model of acute coronary occlusion and pre-treatment with CO.In anesthetized pigs, a coronary snare and microdialysis probes were placed. CO (carboxyhemoglobin 5%) was inhaled for 200 min in test animals, followed by 40 min of coronary occlusion. Microdialysate was analyzed for lactate and glucose, and myocardial tissue samples were analyzed for adenosine tri-phosphate, adenosine di-phosphate, and adenosine mono-phosphate.Lactate during coronary occlusion was approximately half as high in CO pre-treated animals and glucose levels decreased to a much lesser degree during ischemia. Energy charge was no different between groups.CO in the low-doses tested in this model results in a more favorable energy metabolic condition in that glycolysis is decreased in spite of maintained energy charge. Further work is warranted to clarify the possible mechanistic role of energy metabolism for CO protection.

Published

2009

24. Human prostasomes contain chromosomal DNA

Author

Anders Larsson, K. Göran Ronquist, Gunnar Ronquist, and Lena Carlsson

Subjects

Male, Pathology, medicine.medical_specialty, Urology, Semen, Biology, Prostate cancer, Antigen, Prostate, Cell Line, Tumor, medicine, Humans, Cloning, Molecular, Deoxyribonucleases, Clusterin, Secretory Vesicles, Microvesicle, Autoantibody, Prostatic Neoplasms, DNA, Sequence Analysis, DNA, Flow Cytometry, medicine.disease, medicine.anatomical_structure, Oncology, biology.protein, Cancer research, Prostasomes, Sequence Alignment

Abstract

Background: The secretory epithelial cells of the prostate gland use sophisticated vehicles named prostasomes to relay important information to sperm cells in semen. This prostasome-forming and secretory ability of the epithelial cells is also preserved in poorly differentiated prostate cancer cells. Aim: The aim of this thesis was to examine different characteristics of prostasomes, especially those derived from malignant prostate cells, linked to their potential role in diagnosis and prognostication of prostate cancer. Results: Serum samples of prostate cancer patients contained autoantibodies against seminal prostasomes in a higher concentration than did control sera. These autoantibodies were most frequently directed against 25 prostasome-associated proteins, but no one was prostate specific. Clusterin was one of the most frequently occurring prostasomal proteins. Elevated titers were however seen in both patients´ and control sera. Clusterin turned out to be a major antigen of seminal prostasomes. No prostate specific or prostate cancer specific protein was discovered upon proteomic analysis of prostasomes deriving from malignant cells of vertebral metastases of prostate cancer patients. Human chromosomal DNA was identified in both seminal prostasomes and PC-3 cell prostasomes and strong evidence existed that the DNA was localized inside the prostasomes. Four out of 13 DNA clones of seminal prostasomes featured gene sequences (31%). The corresponding figures for PC-3 cell prostasomes were 4 out of 16 clones (25%). Conclusions: Prostasomes are immunogenic and give rise to serum autoantibodies. The most frequently occurring autoantibodies were directed against 25 prostasomal proteins but none of these was exclusively prostate specific. Thirty different proteins were identified in prostate cancer metastasis-derived prostasomes but none of these proteins was prostate cancer specific. Human chromosomal DNA was identified in prostasomes of both normal and malignant cell origin.

Published

2009

25. The Occurrence of a Metabolically Active Cytosine compound in a Protein Fraction from Human Erythrocyte Ghosts

Author

Gunnar Ronquist and Gunnar Ågren

Subjects

Chromatography, Erythrocytes, Cell Membrane, Phosphorus Isotopes, A protein, Fraction (chemistry), Blood Proteins, Cytosine Nucleotides, In Vitro Techniques, Biology, Blood Protein Electrophoresis, Cytosine, chemistry.chemical_compound, Biochemistry, chemistry, Spectrophotometry, Erythrocyte Ghosts, Internal Medicine, Humans, Phospholipids

Published

2009

26. Metabolic stress-like condition can be induced by prolonged strenuous exercise in athletes

Author

Stefan Branth, Birgitta Essén-Gustavsson, Gunnar Ronquist, Torbjörn Åkerfeldt, Roger Olsson, Leif Hambraeus, Mats Stridsberg, and Karin Piehl-Aulin

Subjects

Adult, Male, medicine.medical_specialty, Strenuous exercise, Lipolysis, Energy metabolism, Physiology, Internal medicine, Cellular swelling, Malondialdehyde, energy expenditure, taurine efflux, medicine, Humans, Insulin, Metabolic Stress, Muscle, Skeletal, biology, Athletes, business.industry, musculoskeletal, neural, and ocular physiology, lipid peroxidation, General Medicine, myocytes, biology.organism_classification, Endocrinology, Energy expenditure, Body Composition, Physical Endurance, Original Article, Female, business, Energy Metabolism, human activities, metabolism, Sports

Abstract

Few studies have examined energy metabolism during prolonged, strenuous exercise. We wanted therefore to investigate energy metabolic consequences of a prolonged period of continuous strenuous work with very high energy expenditure. Twelve endurance-trained athletes (6 males and 6 females) were recruited. They performed a 7-h bike race on high work-load intensity. Physiological, biochemical, endocrinological, and anthropometric muscular compartment variables were monitored before, during, and after the race. The energy expenditure was high, being 5557 kcal. Work-load intensity (% of VO(2) peak) was higher in females (77.7%) than in men (69.9%). Muscular glycogen utilization was pronounced, especially in type I fibres (90%). Additionally, muscular triglyceride lipolysis was considerably accelerated. Plasma glucose levels were increased concomitantly with an unchanged serum insulin concentration which might reflect an insulin resistance state in addition to proteolytic glyconeogenesis. Increased reactive oxygen species (malondialdehyde (MDA)) were additional signs of metabolic stress. MDA levels correlated with glycogen utilization rate. A relative deficiency of energy substrate on a cellular level was indicated by increased intracellular water of the leg muscle concomitantly with increased extracellular levels of the osmoregulatory amino acid taurine. A kindred nature of a presumed insulin-resistant state with less intracellular availability of glucose for erythrocytes was also indicated by the findings of decreased MCV together with increased MCHC (haemoconcentration) after the race. This strenuous energy-demanding work created a metabolic stress-like condition including signs of insulin resistance and deteriorated intracellular glucose availability leading to compromised fuelling of ion pumps, culminating in a disturbed cellular osmoregulation indicated by taurine efflux and cellular swelling.

Published

2009

27. Captopril may reduce biochemical (prostate-specific antigen) failure following radical prostatectomy for clinically localized prostate cancer

Author

Yu-Hui Wang, Gunnar Ronquist, Torsten Lindeborg, and Göran Frithz

Subjects

Male, Biochemical recurrence, medicine.medical_specialty, Captopril, Urology, medicine.medical_treatment, Angiotensin-Converting Enzyme Inhibitors, Prostate cancer, Prostate, Biopsy, medicine, Humans, Neoplasm Invasiveness, Postoperative Period, Aged, Prostatectomy, medicine.diagnostic_test, business.industry, Prostatic Neoplasms, Middle Aged, Prostate-Specific Antigen, medicine.disease, Prostate-specific antigen, medicine.anatomical_structure, Nephrology, Neoplasm Recurrence, Local, business, medicine.drug, Radical retropubic prostatectomy

Abstract

OBJECTIVE: A prior report suggested that individuals medicated with captopril showed a decreased incidence of prostate cancer. This study therefore investigated whether captopril given postoperatively had any preventive effect on biochemical recurrence for patients treated with radical prostatectomy. MATERIAL AND METHODS: Data were prospectively reviewed for 62 men subjected to radical retropubic prostatectomy due to biopsy-confirmed, clinically localized prostate cancer and comparisons were made between two groups, those receiving captopril postoperatively (12.5 mg twice daily; captopril group, n=32) and those not receiving any captopril (control group, n=30). One surgeon carried out the surgery. RESULTS: The two groups were comparable as regards age at surgery, prostate volume, preoperative prostate-specific antigen values, pathological stage, Gleason score, organ-confined disease, occurrence of positive surgical margins and extraprostatic extension. The incidence of biochemical failure was three out of 32 patients in the captopril group and 10 out of 30 in the control group (p=0.034) during a mean observational time of 29 months. CONCLUSIONS: A lower rate of biochemical recurrence was observed in men subjected to radical prostatectomy treated with captopril postoperatively than in those not receiving captopril. These results were based on only 32 observations; a larger study may show no evidence of an association.

Published

2009

28. Neuro- and Cardioprotective Effects of Blockade of Nitric Oxide Action by Administration of Methylene Blue

Author

Lars Wiklund, Per Wiklund, Gunnar Ronquist, Hari Shanker Sharma, Samar Basu, and Adriana Miclescu

Subjects

medicine.medical_specialty, Time Factors, Swine, Myocardial Ischemia, Blood Pressure, Myocardial Reperfusion, S100 Calcium Binding Protein beta Subunit, Dinoprost, Nitric Oxide, Neuroprotection, General Biochemistry, Genetics and Molecular Biology, Brain Ischemia, Nitric oxide, Lipid peroxidation, Random Allocation, chemistry.chemical_compound, History and Philosophy of Science, Internal medicine, Troponin I, Animals, Creatine Kinase, MB Form, Medicine, Nerve Growth Factors, Enzyme Inhibitors, biology, business.industry, General Neuroscience, S100 Proteins, History, 19th Century, Survival Analysis, Methylene Blue, Nitric oxide synthase, Disease Models, Animal, Endocrinology, chemistry, Cerebrovascular Circulation, Toxicity, biology.protein, Creatine kinase, business, Methylene blue

Abstract

Methylene blue (MB), generic name methylthioninium (C(16)H(18)ClN(3) S . 3H(2)O), is a blue dye synthesized in 1876 by Heinrich Caro for use as a textile dye and used in the laboratory and clinically since the 1890s, with well-known toxicity and pharmacokinetics. It has experimentally proven neuroprotective and cardioprotective effects in a porcine model of global ischemia-reperfusion in experimental cardiac arrest. This effect has been attributed to MB's blocking effect on nitric oxide synthase and guanylyl cyclase, the latter blocking the synthesis of the second messenger of nitric oxide. The physiological effects during reperfusion include stabilization of the systemic circulation without significantly increased total peripheral resistance, moderately increased cerebral cortical blood flow, a decrease of lipid peroxidation and inflammation, and less anoxic tissue injury in the brain and the heart. The last two effects are recorded as less increase in plasma concentrations of astroglial protein S-100beta, as well as troponin I and creatine kinase isoenzyme MB, respectively.

Published

2007

29. Inherited, non‐spherocytic haemolysis due to deficiency of glucose‐6‐phosphate dehydrogenase

Author

Elvar Theodorsson and Gunnar Ronquist

Subjects

chemistry.chemical_classification, Anemia, Hemolytic, Clinical Biochemistry, Dehydrogenase, General Medicine, Glutathione, Glucosephosphate Dehydrogenase, Biology, medicine.disease, Haemolysis, Hemolysis, Oxidative Stress, chemistry.chemical_compound, Glucosephosphate Dehydrogenase Deficiency, Enzyme, chemistry, Biochemistry, Cytoplasm, medicine, Humans, Glucose-6-phosphate dehydrogenase, Heinz Bodies, Glucose-6-phosphate dehydrogenase deficiency, Heinz body

Abstract

The about 400 million individuals worldwide suffering from a hereditary deficiency of the enzyme glucose-6-phosphate dehydrogenase (G6PD) may experience different degrees of haemolytic anaemia. Haemoglobin is present in very high concentrations in the erythrocyte cytoplasm, at risk of falling out of solution if the internal environment or the haemoglobin itself is changed. G6PD is a crucial enzyme producing reduced glutathione in the erythrocyte cytoplasm for the purpose of protecting haemoglobin against oxidative damage. The presence of unopposed oxidizing agents leading to oxidation of the sulfhydryl bridges between parts of the haemoglobin molecule decrease the solubility of haemoglobin, leading to precipitations called Heinz bodies. The laboratory investigation of G6PD deficiency is commonly done by a quantitative spectrophotometric analysis or by a rapid fluorescent spot test detecting the generation of NADPH from NADP. Genetic tests based on polymerase chain reaction detect specific mutations and may be used for population screening, family studies, or prenatal diagnosis.

Published

2007

30. Prothrombotic effect of prostasomes of metastatic cell and seminal origin

Author

Osama A. Hamad, Javier Sanchez, Adil A. Babiker, Kristina Nilsson Ekdahl, Bo Nilsson, and Gunnar Ronquist

Subjects

Male, medicine.medical_specialty, Urology, Semen, Thromboplastin, Metastasis, Immunoenzyme Techniques, Tissue factor, Prostate cancer, Metastatic cell, Nephelometry and Turbidimetry, Prostate, Cell Line, Tumor, Internal medicine, medicine, Humans, Phosphorylation, business.industry, Secretory Vesicles, Prostatic Neoplasms, Thrombosis, Flow Cytometry, medicine.disease, Seminiferous Epithelium, medicine.anatomical_structure, Endocrinology, Oncology, Coagulation, Cancer research, Calcium, Prostasomes, business, Protein Kinases

Abstract

Prostasomes are secretory granules produced by the glandular epithelial cells of the prostate. Seminal prostasomes contain high amounts of Tissue Factor (TF) but no studies of TF on malignant cell prostasomes have been made. Here we compare the expression, phosphorylation, and function of TF on prostasomes of different origin.TF was detected on prostasomes isolated from seminal fluid and human prostate cancer cell lines (PC-3, DU145, and LNCaP) using FACS and enzyme immunoassay (EIA). Incubation of prostasomes with radioactive ATP under conditions favoring protein kinase A activity led to phosphorylation of TF as detected by immunoprecipitation and SDS-PAGE. The prothrombotic effect of prostasomes was investigated in whole blood and recalcified plasma. Blocking experiments were performed using anti-TF antibodies and corn trypsin inhibitor.TF was expressed on all tested prostasome preparations with lowest values found for seminal ones. Prostasomal TF was the main endogenous substrate for prostasomal protein kinase A. All tested prostasome preparations greatly enhanced the rate of clot formation in a dose-dependent fashion, that is, the clotting capability of prostasomes seemed to be related to the extent of their expression of TF. In addition, the density of the clot varied between different prostasome preparations. When incubated in whole blood, prostasomes were found to associate to WBC thereby inducing them to express and release TF.These data show that TF is overexpressed and also subjected to phosphorylation by malignant cell prostasomes. This suggests major roles for prostasomes in thrombotic events that occur in some advanced cases of prostate cancer.

Published

2007

31. Energy-requiring uptake of prostasomes and PC3 cell-derived exosomes into non-malignant and malignant cells

Author

Gunnar Ronquist, Louise Dubois, Anders Ullén, Karl Göran Ronquist, Dimitris Chioureas, Theocharis Panaretakis, Pedro Fonseca, Claire Sanchez, Anders Larsson, Jeffrey Yachnin, and Karolinska Institutet, Uppsala University

Subjects

0301 basic medicine, Histology, ATPase, exosomes, Exosome, Exocytosis, prostasomes, 03 medical and health sciences, energy metabolism, Extracellular, Glycolysis, extracellular ATP, prostate cancer, extracellular vesicles, glycolysis, exosome uptake, Original Research Article, lcsh:QH573-671, Cancer och onkologi, biology, lcsh:Cytology, Cell Biology, Microvesicles, Cell biology, 030104 developmental biology, Biochemistry, Cancer and Oncology, biology.protein, Prostasomes, Intracellular

Abstract

Epithelial cells lining the prostate acini release, in a regulated manner (exocytosis), nanosized vesicles called prostasomes that belong to the exosome family. Prostate cancer cells have preserved this ability to generate and export exosomes to the extracellular space. We previously demonstrated that human prostasomes have an ATP-forming capacity. In this study, we compared the capacity of extracellular vesicles (EVs) to generate ATP between normal seminal prostasomes and exosomes secreted by PC3 cells (PC3 exosomes), a prostate cancer cell line. Proteomic analyses identified enzymes of the glycolytic chain in both prostasomes and PC3 exosomes, and we found that both of them were capable of generating ATP when supplied with substrates. Notably, the net production of extracellular ATP was low for prostasomes due to a high ATPase activity contrary to an elevated net ATP level for PC3 exosomes because of their low ATPase activity. The uptake of the 2 types of EVs by normal prostate epithelial cells (CRL2221) and prostate cancer cells (PC3) was visualized and measured, demonstrating differential kinetics. Interestingly, this uptake was dependent upon an ongoing glycolytic flux involving extracellular ATP formation by EVs and/or intracellular ATP produced from the recipient cells. We conclude that the internalization of EVs into recipient cells is an energy-requiring process also demanding an active V-ATPase and the capacity of EVs to generate extracellular ATP may play a role in this process.Keywords: extracellular ATP; prostate cancer; extracellular vesicles; exosomes; prostasomes; ATPase; glycolysis; energy metabolism; exosome uptake(Published: 7 March 2016)Citation: Journal of Extracellular Vesicles 2016, 5: 29877 - http://dx.doi.org/10.3402/jev.v5.29877

Published

2015

32. Prostasomes: Their Characterisation: Implications for Human Reproduction: Prostasomes and Human Reproduction

Author

Gunnar, Ronquist

Subjects

Male, Prostasomes, Reproduction, Prostate, Humans, Seminal fluid, Non-coding RNA, Spermatozoa, Article, Antioxidants, Immunosuppression

Abstract

The prostate is a principal accessory genital gland that is vital for normal fertility. Epithelial cells lining the prostate acini release in a defined fashion (exocytosis) organellar nanosized structures named prostasomes. They are involved in the protection of sperm cells against immune response in the female reproductive tract by modulating the complement system and by inhibiting monocyte and neutrophil phagocytosis and lymphocyte proliferation. The immunomodulatory function most probably involves small non-coding RNAs present in prostasomes. Prostasomes have also been proposed to regulate the timing of sperm cell capacitation and induction of the acrosome reaction, since they are rich in various transferable bioactive molecules (e.g. receptors and enzymes) that promote the fertilising ability of sperm cells. Antigenicity of sperm cells has been well documented and implicated in involuntary immunological infertility of human couples, and antisperm antibodies (ASA) occur in several body fluids. The propensity of sperm cells to carry attached prostasomes suggests that they are a new category of sperm antigens. Circulating human ASA recognise prostasomes, and among 12 identified prostasomal antigens, prolactin- inducible protein (95 %) and clusterin (85 %) were immunodominant at the expense of the other 10 that were sporadically occurring.

Published

2015

33. The polyphosphate-factor XII pathway drives coagulation in prostate cancer-associated thrombosis

Author

Evi X. Stavrou, Thomas Renné, Tobias A. Fuchs, Markus Graefen, Gunnar Ronquist, Göran Ronquist, Nigel Mackman, Florian Langer, Carsten Bokemeyer, Guido Sauter, Katrin F. Nickel, and Linda Labberton

Subjects

Male, medicine.medical_specialty, animal structures, Factor XIIa, High-molecular-weight kininogen, Immunology, Antibodies, Monoclonal, Humanized, Biochemistry, Prostate cancer, Mice, Thrombin, Polyphosphates, Internal medicine, Cell Line, Tumor, medicine, Animals, Humans, cardiovascular diseases, Factor XII, Fibrin, business.industry, Secretory Vesicles, Prostatic Neoplasms, Thrombosis, Cell Biology, Hematology, Kallikrein, medicine.disease, Endocrinology, Coagulation, Prostasomes, business, Pulmonary Embolism, circulatory and respiratory physiology, medicine.drug

Abstract

Cancer is a leading cause of thrombosis. We identify a new procoagulant mechanism that contributes to thromboembolism in prostate cancer and allows for safe anticoagulation therapy development. Prostate cancer-mediated procoagulant activity was reduced in plasma in the absence of factor XII or its substrate of the intrinsic coagulation pathway factor XI. Prostate cancer cells and secreted prostasomes expose long chain polyphosphate on their surface that colocalized with active factor XII and initiated coagulation in a factor XII-dependent manner. Polyphosphate content correlated with the procoagulant activity of prostasomes. Inherited deficiency in factor XI or XII or high-molecular-weight kininogen, but not plasma kallikrein, protected mice from prostasome-induced lethal pulmonary embolism. Targeting polyphosphate or factor XII conferred resistance to prostate cancer-driven thrombosis in mice, without increasing bleeding. Inhibition of factor XII with recombinant 3F7 antibody reduced the increased prostasome-mediated procoagulant activity in patient plasma. The data illustrate a critical role for polyphosphate/factor XII-triggered coagulation in prostate cancer-associated thrombosis with implications for anticoagulation without therapy-associated bleeding in malignancies.

Published

2015

34. Prostasomes: Their Characterisation: Implications for Human Reproduction

Author

Gunnar Ronquist

Subjects

Andrology, Immune system, medicine.anatomical_structure, Antigen, Capacitation, Monocyte, Acrosome reaction, medicine, Prostasomes, Lymphocyte proliferation, Biology, Sperm

Abstract

The prostate is a principal accessory genital gland that is vital for normal fertility. Epithelial cells lining the prostate acini release in a defined fashion (exocytosis) organellar nanosized structures named prostasomes. They are involved in the protection of sperm cells against immune response in the female reproductive tract by modulating the complement system and by inhibiting monocyte and neutrophil phagocytosis and lymphocyte proliferation. The immunomodulatory function most probably involves small non-coding RNAs present in prostasomes. Prostasomes have also been proposed to regulate the timing of sperm cell capacitation and induction of the acrosome reaction, since they are rich in various transferable bioactive molecules (e.g. receptors and enzymes) that promote the fertilising ability of sperm cells. Antigenicity of sperm cells has been well documented and implicated in involuntary immunological infertility of human couples, and antisperm antibodies (ASA) occur in several body fluids. The propensity of sperm cells to carry attached prostasomes suggests that they are a new category of sperm antigens. Circulating human ASA recognise prostasomes, and among 12 identified prostasomal antigens, prolactin- inducible protein (95 %) and clusterin (85 %) were immunodominant at the expense of the other 10 that were sporadically occurring.

Published

2015

35. Metabolic Manipulation of Glioblastoma in Vivo by Retrograde Microdialysis of L-2, 4 Diaminobutyric Acid (DAB)

Author

Urban Ungerstedt, Michael Roslin, Roger Henriksson, Anders Waldenström, Gunnar Ronquist, and A. Tommy Bergenheim

Subjects

Glycerol, Male, Antimetabolites, Antineoplastic, Cancer Research, Microdialysis, Taurine, Treatment outcome, Glutamic Acid, Monitoring, Ambulatory, Biology, Pharmacology, Glycerol metabolism, Stereotaxic Techniques, Catheters, Indwelling, In vivo, medicine, Humans, neoplasms, Aged, Infusions, Intralesional, Dose-Response Relationship, Drug, Brain Neoplasms, Aminobutyrates, Middle Aged, medicine.disease, nervous system diseases, Treatment Outcome, Neurology, Oncology, Biochemistry, Stereotaxic technique, Female, Neurology (clinical), Glutamic acid metabolism, Glioblastoma, Taurine metabolism

Abstract

To study the metabolic effects in vivo of L-2, 4 diaminobutyric acid (DAB) administered by retrograde microdialysis in glioblastoma and to evaluate the feasibility of the technique.In 10 patients with glioblastoma, a stereotactic biopsy was performed followed by implantation of microdialysis catheters. One or two catheters were implanted in tumor tissue and two reference catheters were implanted in normal brain tissue and subcutaneous abdominal tissue, respectively. Tumor catheters were perfused with 80 or 120 mmol/l DAB and reference catheters were perfused with a Ringer solution, all with a flow rate of 2.0 microl/min. Treatment was given for at mean 9.1 (5-19) days.The treatment was well tolerated by the patients with the exception of two patients in whom a transient brain edema appeared. No complications related to the technique were encountered. During treatment, an increase in the extracellular amino acids alanine, glycine, glutamate, aspartate, serine, threonine, and taurine was found demonstrating a significant influence on the intracellular pool of free amino acids induced by DAB. No change in glucose metabolism or glycerol was evident. The metabolism in normal brain was unaffected during treatment.Retrograde microdialysis is a feasible method for intracerebral administration of drugs to tumor tissue in patients with glioblastoma. We found it possible to deliver DAB to glioblastoma tumors in fully mobilized patients and to assess the metabolic effects induced by the treatment. The changes in extracellular amino acids were in concordance to what was expected from in vitro studies. Elevation of glutamate and taurine may be regarded as markers for an induced cellular toxicity while the unchanged level of glycerol may indicate no direct effects on phospholipase activity and membrane phospholipid composition. The effects were restricted to the tumor compartment. Although an improved survival could possibly be suspected no dramatic effect on outcome could be detected. However, the series was small and, most probably, the time for treatment was too short.

Published

2006

36. Overexpression of ecto-protein kinases in prostasomes of metastatic cell origin

Author

Gunnar Ronquist, Kristina Nilsson Ekdahl, Bo Nilsson, and Adil A. Babiker

Subjects

Male, medicine.medical_specialty, Angiogenesis, Urology, CD59, Biology, DU145, Internal medicine, LNCaP, Tumor Cells, Cultured, medicine, Humans, Neoplasm Metastasis, Phosphorylation, Protein kinase A, Adenosine Triphosphatases, Kinase, Gene Expression Profiling, Secretory Vesicles, Prostatic Neoplasms, Cell biology, Endocrinology, Oncology, Prostasomes, Protein Kinases

Abstract

Prostasomes are extracellularly occurring submicron, membrane-surrounded organelles produced by the epithelial cells of the prostate and present in semen. Their precise physiological role is not known, although some of their properties assign them to important physiological and patho-physiological functions. In this thesis, some new properties of seminal and malignant cell line (DU145, PC-3 and LNCaP) prostasomes have been identified. Differences in the expressions and activities of prostasomal CD59, ATPase, protein kinases and tissue factor (TF) have been characterized. The transfer of prostasomal CD59 to CD59-deficient erythrocytes (rabbit and human PNH erythrocytes) has been established. CD59, protein kinases and TF were overexpressed by malignant cell prostasomes. ATPase activity was highest on seminal prostasomes with minimal expression by malignant cell prostasomes resulting in more residual ATP available for phosphorylation reactions. Several proteins were phosphorylated by prostasomal protein kinases, viz. complement component C3, fibrinogen, vitronectin and E-cadherin. Furthermore, TF was identified as the main endogenous phosphorylation substrate on prostasomes. In addition, prothrombotic effects of prostasomes were established. DU145 and PC-3-derived prostasomes exerted a higher clotting effect on whole blood and plasma compared to LNCaP and seminal prostasomes.In conclusion, malignant cell prostasomes showed higher ability to interact with the biological system in favor of prostate cancer cell promotion and survival. The roles played by prostasomes in this context may improve the understanding of the mechanisms that help the prostate cancer cells to avoid the complement attack (CD59 transfer and phosphorylation of C3), to promote angiogenesis (TF) and to metastasize. It may also provide a better understanding of some of the complications usually seen in some terminal prostate cancer patients like thrombotic events and tendency to develop disseminated intravascular coagulation.

Published

2006

37. Antiprostasome antibodies: Possible serum markers for prostate cancer metastasizing liability

Author

Anders Larsson, Gunnar Ronquist, B. Ove Nilsson, Elke Eltze, Axel Semjonow, Olaf Bettendorf, Lena Carlsson, and Christian Wülfing

Subjects

Adult, Male, PCA3, Urology, Prostatic Hyperplasia, Enzyme-Linked Immunosorbent Assay, Metastasis, Prostate cancer, medicine, Humans, Aged, Autoantibodies, Aged, 80 and over, biology, medicine.diagnostic_test, business.industry, Secretory Vesicles, Prostate, Antibody titer, Prostatic Neoplasms, Middle Aged, Prostate-Specific Antigen, medicine.disease, Prostate-specific antigen, Oncology, Immunoassay, Immunology, biology.protein, Prostasomes, Antibody, business

Abstract

Prostasomes are secretory granules synthesized, stored, and secreted by normal and neoplastic human prostate epithelial cells. In prostate cancer, they are anticipated to be released into the blood circulation where they may be immunogenic. The aim of our study was to examine whether prostasome antibody presence in serum bears any prognostic significance for men with prostate cancer. We developed a sensitive and specific immunoassay (enzyme-linked immunosorbent assay) to establish the presence of antiprostasome antibodies in serum. The antiprostasome antibody titer in serum, sampled before any kind of therapy for prostate cancer, was examined together with clinicopathologic variables and outcome over a median follow-up of 350 days in 218 patients with verified prostate cancer. We detected these antibodies in 191 (88%) of these patients. This antibody titer did not correlate to serum values of prostate-specific antigen. Significant, inverse relationships were registered for antiprostasome antibody titer, and metastases to bone and/or lymph nodes (P = 0.035) and pT (P = 0.025). These results indicate that the antiprostasome antibody titer in serum may be a novel marker for prostate cancer liability to metastasize.

Published

2006

38. Prostasome-derived proteins capable of eliciting an immune response in prostate cancer patients

Author

Lena Carlsson, Sten Nilsson, Anders Larsson, Karl Göran Ronquist, and Gunnar Ronquist

Subjects

Electrophoresis, Male, PCA3, Cancer Research, medicine.medical_treatment, Blotting, Western, Mass Spectrometry, Prostate cancer, Semen, Prostate, medicine, Humans, Clusterin, biology, business.industry, Autoantibody, Prostatic Neoplasms, Immunotherapy, medicine.disease, Molecular Weight, medicine.anatomical_structure, Oncology, Immunology, biology.protein, Prostasomes, Antibody, business

Abstract

Prostate cancer consistently remains a difficult clinical enigma. Therefore, the development of novel strategies for diagnosis and treatment (e.g. immunotherapy) of prostate cancer is essential. We tried to identify the prostasome-derived proteins that were immunogenic in prostate cancer patients. Prostate cancer patients' sera (n = 44) with high enzyme-linked immunosorbent assay (ELISA) titers against prostasomes were selected for immunoblotting against purified seminal prostasomes. The SDS-PAGE and immunoblotting experiments were performed with Bio-Rad systems. Twenty-five of the recognized proteins were isolated and analyzed by means of mass spectrometry. Out of 44 patients' sera, 31 (70%) demonstrated in immunoblotting experiments reactivity against several prostasomal protein bands in the molecular weight range of 10-200 kDa. Some of the bands (55, 70 and 170 kDa) were more frequently recognized by the patients' sera. Concomitantly run control sera generated only very weak or no bands at all. The most frequently occurring prostasomal proteins were identified as heat shock proteins (HSP 70, 71) and clusterin. This study identified the most important molecular targets of autoantibodies against prostasomes generated in connection with the development of prostate cancer in man. These immunogenic prostasomal proteins could be appropriate target molecules for specific immunotherapy of prostate cancer patients.

Published

2006

39. Mode of Growth Determines Differential Expression of Prostasomes in Cultures of Prostate Cancer Cell Lines and Opens for Studies of Prostasome Gene Expression

Author

Lena Lennartsson, Sten Nilson, Lena Carlsson, Gunnar Ronquist, O. Nilsson, and Anders Larsson

Subjects

Male, Pathology, medicine.medical_specialty, Transplantation, Heterologous, Immunocytochemistry, Gene Expression, Biology, Rats, Nude, Microscopy, Electron, Transmission, Antigen, DU145, Cell Line, Tumor, Spheroids, Cellular, LNCaP, medicine, Animals, Humans, Secretion, Oligonucleotide Array Sequence Analysis, Secretory Vesicles, Prostatic Neoplasms, General Medicine, Rats, Cell biology, Transplantation, Cell culture, Prostasomes, Neoplasm Transplantation

Abstract

The exocrine secretion of the acinar gland cells in the human prostate consists of, among other components, a serous secretion and prostasomes. The prostasomes are functionally associated with both reproduction and prostate cancer development and are capable to raise autoantibodies at various pathologies. Therefore, we are trying to characterize prostasome antigens by analysing prostasome-producing cell lines of prostate cancers with the cDNA microarray technique. To obtain one state with synthesis of prostasomes and another state without synthesis, we checked whether the prostasome differentiation was influenced by the mode of growing the cells, that is, whether the cells had been growing on a solid support or on a flexible one. We studied the expression of prostasomes in the cell lines PC3, DU145 and LNCaP. We grew the cells with the following methods: Monocellular layers on microbeads, multicellular spheroids, single cells in suspension cultures, and xenotransplants in nude rats. The presence of prostasomes was examined by ELISA, immunocytochemistry or electron microscopy. The results showed that growing the cells on microbeads (solid support) produced a differentiation of prostasomes, while growing the cells in multicellular spheroids (flexible support) did not. Thus it should be possible to apply cDNAmicroarray analyses for characterizing the genes which are active at the cellular expression of prostasomes and then deduce the prostasome antigens.

Published

2006

40. Dominant Prostasome Immunogens for Sperm-Agglutinating Autoantibodies of Infertile Men

Author

Gunnar Ronquist, Lena Carlsson, B. Ove Nilsson, and Anders Larsson

Subjects

Male, Agglutination, Urology, Endocrinology, Diabetes and Metabolism, Blotting, Western, Context (language use), Peroxiredoxin 2, Autoantigens, Endocrinology, Antigen, Humans, Electrophoresis, Gel, Two-Dimensional, Infertility, Male, Autoantibodies, biology, Clusterin, Prostate, Autoantibody, Spermatozoa, Sperm, Molecular biology, Reproductive Medicine, Spectrometry, Mass, Matrix-Assisted Laser Desorption-Ionization, biology.protein, Prostasomes, Antibody

Abstract

The presence of naturally occurring anti-sperm anti- bodies (ASA) is a well-known cause of infertility in men and women, but the antigens for these antibodies are poorly characterized. We have previously shown that prostasomes adhere to sperm cells and that prostasomes are major targets for ASA associated with infertil- ity. These autoantigens have not been characterized. We used 2- dimensional electrophoresis, immunoblotting, and mass-spectrom- etry to identify the prostasome antigens for these autoantibodies. By these techniques, we revealed that prolactin-inducible protein (PIP) and clusterin were dominant prostasome immunogens for sperm- agglutinating autoantibodies of 20 patients with immunological infer- tility. PIP was identified by 19 of 20 (95%) patient sera and clusterin by 17 of 20 (85%). In addition, 10 sporadically occurring prostasomal antigens were identified in this context, viz alcohol dehydrogenase (NADP1), annexin I, annexin III, BRCA1-associated ring domain pro- tein 1, heat shock 27-kd protein, isocitrate dehydrogenase, lactoyl- glutathione lyase, NG,NG-dimethylarginine dimethylaminohydrolase 1, peroxiredoxin 2, and syntenin 1.

Published

2004

41. A new test for immunological infertility: an ELISA based on prostasomes

Author

Gunnar Ronquist, M. Lundquist, Anders Larsson, Bo Nilsson, and Lena Carlsson

Subjects

Male, Infertility, Urology, Endocrinology, Diabetes and Metabolism, Enzyme-Linked Immunosorbent Assay, Antibodies, Andrology, Antigen, Semen, medicine, Humans, In patient, Antigens, Infertility, Male, Organelles, biology, Prostate, Reproducibility of Results, Elisa assay, medicine.disease, Spermatozoa, Immunological infertility, Sperm, digestive system diseases, surgical procedures, operative, Reproductive Medicine, Immunology, Immunologic Techniques, biology.protein, Prostasomes, Antibody

Abstract

Antisperm antibodies (ASA) are present in patients with immunological infertility, but the antigens are poorly characterized. Prostasomes adhere to sperm cells and are recognized as antigens for ASA. This investigation aimed to study the prevalence of antiprostasome antibodies in ASA-classified sera. We studied the reactivity of ASA-positive sera from 116 immunoinfertile patients. Ninety-seven per cent (113 of 116) of the patients' sera contained IgG antibodies against seminal prostasomes. Accordingly, prostasomes are one of the major targets for ASA. An enzyme-linked immunosorbent assay based on prostasomes is simpler to perform than ASA tests presently in use. It is also easier to achieve reproducible and standardized results.

Published

2004

42. Prostasomes are secreted from poorly differentiated cells of prostate cancer metastases

Author

B. Ove Nilsson, Anders Ahlander, Gunnar Ronquist, Anders Frost, Göran Sahlén, and Bo Johan Norlén

Subjects

Pathology, medicine.medical_specialty, biology, Urology, medicine.disease, Metastasis, Prostate cancer, medicine.anatomical_structure, Immune system, Oncology, Antigen, Prostate, medicine, biology.protein, Secretion, Prostasomes, Antibody

Abstract

Prostasomes are submicron-sized, membrane-bound organelles produced by the epithelial cells of the prostate and normally found in the secretion in the gland ducts. Their physiological role is in the promotion of sperm-function in human reproduction. This thesis contains four papers dealing with the production of prostasomes and some possible applications in clinical urology of the prostasome. Paper I and II provided an ultrastructural description of the synthesis, storage and secretion of prostasomes in benign as well as in malignant tissue. Most notable were the extracellular appearances of prostasomes in metastatic lesions whereby the prostasomes become exposed to the immune system of the patient. This supported findings in earlier studies in which patients with advanced prostate cancer had elevated levels of anti-prostasome antibodies. The results of paper III reinforced the view of the prostate-unique origin of the prostasome. In particular, there were no indications in SDS-PAGE patterns or flow-cytometric studies of material from seminal vesicle secretion that it contained components that could be associated with a production of prostasomes. Some possible clinical functions of the prostasomes were investigated in paper IV. Exposure of prostasomes to the immune system through mechanical and thermal trauma to the prostate did not induce an evident formation of anti-prostasome autoantibodies. Furthermore, the serum levels of anti-prostasome antibodies registered by assays with preparations of prostasomes from seminal plasma as antigen did not correlate with existing prostate cancer. Seminal prostasomes seemed not to function as substitute markers for prostate cancer in the test kit used. A possible explanation could be underestimated differences in antigen properties between seminal or prostate gland-derived prostasomes and prostasomes from tumor tissue.

Published

2004

43. The Janus-faced nature of prostasomes: their pluripotency favours the normal reproductive process and malignant prostate growth

Author

Gunnar Ronquist and Bo Nilsson

Subjects

Male, Aging, Cancer Research, Urology, Motility, Biology, Antioxidants, Prostate cancer, Prostate, Prevalence, medicine, Extracellular, Humans, Aged, Secretory Vesicles, Prostatic Neoplasms, Epithelial Cells, Middle Aged, medicine.disease, Sperm, Epithelium, Cell biology, medicine.anatomical_structure, Oncology, Immunology, Sperm Motility, Neoplastic cell, Prostasomes

Abstract

Prostasomes are submicron secretory granules synthesized, stored and secreted by the epithelial cells of the human prostate gland. They are membrane-surrounded also in their extracellular appearance and the membrane architecture is composite. They are believed to be life-giving and act as protectors of the spermatozoa in the lower and upper female genital tract on their way to the ovum. Hence, the prostasomes are immunosuppressive and inhibitory of complement activation. Further, they promote sperm's forward motility and have antioxidant and antibacterial capacities. The prostasomes with their many composite abilities seem to turn against the host cell after the age of 50 y being conducive to the transition of the normal prostate epithelial cell into a neoplastic cell and therewith lay the foundations of the very high prevalence of prostate cancer of men of more than 50 y of age.

Published

2004

44. Transfer of functional prostasomal CD59 of metastatic prostatic cancer cell origin protects cells against complement attack

Author

Lena Carlsson, Bo Nilsson, Gunnar Ronquist, Adil A. Babiker, and Kristina Nilsson Ekdahl

Subjects

Male, medicine.medical_specialty, Erythrocytes, Angiogenesis, Urology, Cell, CD59 Antigens, CD59, Hemolysis, Antibodies, Prostate cancer, DU145, Semen, Cell Line, Tumor, Internal medicine, LNCaP, medicine, Animals, Humans, Kinase, business.industry, Phosphatidylinositol Diacylglycerol-Lyase, Secretory Vesicles, Prostatic Neoplasms, Complement System Proteins, Flow Cytometry, medicine.disease, medicine.anatomical_structure, Endocrinology, Oncology, Cancer research, Prostasomes, Rabbits, business

Abstract

Prostasomes are extracellularly occurring submicron, membrane-surrounded organelles produced by the epithelial cells of the prostate and present in semen. Their precise physiological role is not known, although some of their properties assign them to important physiological and patho-physiological functions. In this thesis, some new properties of seminal and malignant cell line (DU145, PC-3 and LNCaP) prostasomes have been identified. Differences in the expressions and activities of prostasomal CD59, ATPase, protein kinases and tissue factor (TF) have been characterized. The transfer of prostasomal CD59 to CD59-deficient erythrocytes (rabbit and human PNH erythrocytes) has been established. CD59, protein kinases and TF were overexpressed by malignant cell prostasomes. ATPase activity was highest on seminal prostasomes with minimal expression by malignant cell prostasomes resulting in more residual ATP available for phosphorylation reactions. Several proteins were phosphorylated by prostasomal protein kinases, viz. complement component C3, fibrinogen, vitronectin and E-cadherin. Furthermore, TF was identified as the main endogenous phosphorylation substrate on prostasomes. In addition, prothrombotic effects of prostasomes were established. DU145 and PC-3-derived prostasomes exerted a higher clotting effect on whole blood and plasma compared to LNCaP and seminal prostasomes.In conclusion, malignant cell prostasomes showed higher ability to interact with the biological system in favor of prostate cancer cell promotion and survival. The roles played by prostasomes in this context may improve the understanding of the mechanisms that help the prostate cancer cells to avoid the complement attack (CD59 transfer and phosphorylation of C3), to promote angiogenesis (TF) and to metastasize. It may also provide a better understanding of some of the complications usually seen in some terminal prostate cancer patients like thrombotic events and tendency to develop disseminated intravascular coagulation.

Published

2004

45. Inhibition of the L-dopa transport system in human epidermal Langerhans cells by omeprazole and its analogues

Author

Niels Bendsoe and Gunnar Ronquist

Subjects

Clinical Biochemistry, Biological Transport, Active, Inhibitory postsynaptic potential, Biochemistry, Levodopa, medicine, Humans, Lactic Acid, Enzyme Inhibitors, Energy charge, Cells, Cultured, Omeprazole, Adenosine Triphosphatases, chemistry.chemical_classification, Polarity (international relations), Cytoplasmic Vesicles, Organic Chemistry, Cationic polymerization, Amino acid, Membrane, Epidermal Cells, chemistry, Gastric Mucosa, Langerhans Cells, Potassium, Ultrastructure, Hydrogen, medicine.drug

Abstract

L-3,4-dihydroxyphenylalanine (L-dopa) transport into human Langerhans cells (LC) occurs by a saturable mediation. This plasma membrane agency is, due to its characteristics, distinguishable from systems transporting other neutral, cationic and anionic amino acids into other cells and serves to catalyze the flow of L-dopa, only, into LC. The uphill operation of this L-dopa transport system is believed to occur by down-gradient countermigration of H(+). Due to the uniqueness of the L-dopa transport system, the widely used analogue inhibition approach was not applicable. Instead we studied omeprazole and its analogues in our search for suitable inhibitory candidates. Omeprazole and most of its analogues were indeed inhibitory in the concentration range 1-100 micromol/L. Conspicuously, the compounds with strongest polarity were least inhibitory. The inhibitory pattern displayed by omeprazole and the other analogues on L-dopa uptake in LC corresponded to some extent to what has been observed previously for purified H(+),K(+)-ATPase from tubulovesicles of the stomach. No effects of the inhibitors were registered on energy charge and lactate production of epidermal biopsies, nor were any gross alterations of ultrastructure of LC noticed.

Published

2003

46. Association between captopril, other antihypertensive drugs and risk of prostate cancer

Author

Ana Ruigómez, Saga Johansson, Luis A. García Rodríguez, Gunnar Ronquist, Göran Frithz, Mari-Ann Wallander, and Kurt Svärdsudd

Subjects

Oncology, Gynecology, medicine.medical_specialty, business.industry, Urology, Captopril, medicine.disease, Lower risk, Prostate cancer, medicine.anatomical_structure, Prostate, Internal medicine, Relative risk, ACE inhibitor, medicine, Prostatism, Risk factor, business, medicine.drug

Abstract

BACKGROUND There has been some debate on the existence of an association between hypertension, antihypertensive medications and cancer risk. METHODS We performed a nested case-control study to assess the association between the risk of prostate cancer and the use of the angiotensin converting enzyme (ACE)-inhibitor captopril, and other antihypertensive drugs. We used data from the General Practice Research Database in UK. RESULTS We found an incidence rate of prostate cancer of 1.61 per 1,000 person-years among male patients aged 50–79 years old. Patients with a history of benign prostatic hyperplasia and/or prostatism carried a two-fold greater risk of prostate cancer than those without such antecedents. None of the other studied co-morbidities were associated with prostate cancer. We found that users of captopril had a relative risk of 0.7 (95% CI: 0.4–1.2) to develope prostate cancer. None of the other studied individual ACE-inhibitors shared a similar effect with the one observed for captopril. CONCLUSIONS No clear association was apparent between the use of antihypertensive drugs and prostate cancer. However, specific focus on users of captopril showed a lower risk of subsequent prostate cancer. Further research is needed to explore this association. © 2003 Wiley-Liss, Inc.

Published

2003

47. New mechanism for amino acid influx into human epidermal Langerhans cells: L-dopa/proton counter-transport system

Author

Gunnar Ronquist, Bengt Falck, and Niels Bendsoe

Subjects

chemistry.chemical_classification, integumentary system, Birbeck granules, Dermatology, Biology, Biochemistry, Proton pump, Amino acid, chemistry, Anaerobic glycolysis, Proton transport, Biophysics, Extracellular, Energy source, Molecular Biology, Intracellular

Abstract

We have characterized a stereospecific transport mechanism for L-dopa into human epidermal Langerhans cells (LCs). It is different from any other amino acid transport system. It is highly concentrative, largely pH-independent, and independent of exogenous Na+, glucose and oxygen, and fuelled by a renewable intracellular energy source inhibited by iodoacetate but not by arsenate. We propose that the mechanism is a unidirectional L-dopa/proton counter-transport system. We have recently demonstrated anaerobic glycolysis in human epidermis, which substantiates the need of proton pumps for resident LCs. The findings prompt a re-evaluation of the profound changes LCs undergo when exposed to oxygen in aerobic culture. L-dopa is not metabolized by LCs but can rapidly be dislocated to the intercellular space by certain extracellular amino acids, i.e. LCs can profit by L-dopa in a dualistic way, altogether a remarkable biological phenomenon.

Published

2003

48. Human epidermal energy metabolism is functionally anaerobic

Author

Niels Bendsoe, Anders F. Andersson, Bengt Falck, and Gunnar Ronquist

Subjects

chemistry.chemical_classification, Glycogenolysis, Epidermis (botany), Extracellular transport, Dermatology, Mitochondrion, Biology, Biochemistry, Cell biology, chemistry, Extracellular, Energy charge, Molecular Biology, Anaerobic exercise, Organic acid

Abstract

We have reported that epidermal Langerhans cells possess an H+-extruding mechanism signalling their existence in an anaerobic environment. This study highlights the energy metabolism of human epidermis. In their habitual state the keratinocytes contain more lactate than do most other cell types. Their lactate production in vitro is vigorous and independent of oxygen and most of it is released to the medium. Autoincubation of the epidermis under starved conditions resulted in a 30% increase of lactate, indicating ongoing glycogenolysis. Iodoacetate inhibited lactate production by > 90%. Energy charge values were low, approximately 0.82, and comparable with those previously reported for smooth muscle. Moreover, the overwhelming majority of the keratinocytic mitochondria had an appearance markedly deviating from those in the Langerhans cells, melanocytes and fibroblasts, and, above all, were characterized by an enormous reduction of the inner membrane. This structure is in all probability incompatible with an effective oxidative metabolism of glucose. We conclude that epidermal energy metabolism is predominantly anaerobic in spite of the formal presence of mitochondria. The high production of lactate obviously demands extracellular transport pathways for rapid elimination of this organic acid. An extracellular space complying with such a demand emerges on electron microscopy when an isotonic glutaraldehyde-based fixative is used. The prevailing view regarding the size of the extracellular space is based on the common use of hypotonic fixatives, such as Karnovski's fixative, which causes gross cellular swelling and concomitant near total elimination of the extracellular space, leaving interstices with a diameter significantly smaller than that allowing fluid flow. (Less)

Published

2003

49. Validity of the microdialysis technique for experimental in vivo studies of myocardial energy metabolism

Author

Anders Waldenström, Mohammad Kavianipour, Gerhard Wikström, and Gunnar Ronquist

Subjects

medicine.medical_specialty, Microdialysis, medicine.diagnostic_test, Physiology, Metabolite, Urology, Ischemia, Biology, medicine.disease, Adenosine, chemistry.chemical_compound, Endocrinology, chemistry, In vivo, Internal medicine, Biopsy, Circulatory system, medicine, Hypoxanthine, medicine.drug

Abstract

Objectives: The validity of the microdialysis technique for experimental in vivo studies of myocardial energy metabolism is not known. To address this question interstitial levels of energy-related metabolites (lactate, adenosine, inosine and hypoxanthine) obtained by the microdialysis technique were compared with corresponding metabolites from myocardial biopsies at given intervals in a porcine heart model using different protocols of ischaemia and reperfusion. Methods: In an open chest porcine heart model, interstitial levels of energy-related metabolites were monitored using the microdialysis technique. All animals (n = 23) were subjected to 120-min pretreatment followed by 40 min of regional ischaemia and 120 min of reperfusion. Tissue biopsies were obtained in the beginning, middle and at the end of the 40-min ischaemic period and at the end of the reperfusion period. Pretreatment consisted of either rest (group 1, n = 7), or rest for 90 min and one ischaemia/reperfusion (10 + 20 min) cycle (group 2, n = 9), or four ischaemia/reperfusion cycles (10 + 20 min each) (group 3, n = 7). Results: Interstitial levels of energy-related metabolites monitored by the microdialysis technique correlated with tissue biopsy levels of lactate (r = 0.90, P

Published

2003

50. Ischaemic preconditioning alters the energy metabolism and protects the ischaemic myocardium in a stepwise fashion

Author

Mohammad Kavianipour, Anders Waldenström, Gunnar Ronquist, and Gerhard Wikström

Subjects

Microdialysis, medicine.medical_specialty, Physiology, business.industry, Ischemia, Adenylate kinase, medicine.disease, Adenosine, chemistry.chemical_compound, Endocrinology, chemistry, Adenine nucleotide, Internal medicine, Circulatory system, medicine, business, Inosine, Hypoxanthine, medicine.drug

Abstract

Aims and Methods: Recently it was suggested that ischaemic preconditioning (IP) protects the myocardium in a graded pattern as assessed by myocardial infarct size estimation. Using tissue biopsies we investigated the impact of the proposed graded pattern of protection on myocardial energy state in an open-chest porcine model of IP with either one (1xIP) or four (4xIP) episodes of preconditioning. Furthermore, we evaluated the relationship between interstitial energy-related metabolite levels obtained by the microdialysis technique and the degree of subsequent ischaemic insult. Results: During the long ischaemia the difference between pre-ischaemic and post-ischaemic total adenylate pools and the sum of adenylate breakdown products (adenosine, inosine and hypoxanthine) as well as tissue lactate levels appeared as follows: non-IP > 1xIP > 4xIP (P 1xIP > 4xIP. Conclusions: We present for the first time concordant energy metabolic and morphometric data in support of IP being a stepwise phenomenon for protection of the ischaemic myocardium. Furthermore, IP resulted in proportionally higher levels of hypoxanthine (relative to inosine) in the ischaemic myocardium, suggesting a different handling of adenine nucleotide breakdown products in the IP myocardium.

Published

2003