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4. Y-chromosomal diversity within Europe is clinal and influenced primarily by geography rather than language

Author

Rosser, Z. H., Zerjal, T., Hurles, M. E., Adojaan, M., Alavantic, D., Amorim, A., Amos, W., Armenteros, M., Arroyo, E., Barbujani, Guido, Beckman, L., BERTRANPETIT J., Bosch E., Bradley, D. G., Brede, G., Cooper, G., Corte Real, H. B. S. M., de Knijff, P., Decorte, R., Dubrova, Y. E., Evgrafov, O., Gilissen, A, Glisic, S., Golge, M, Hill, E. W., Jeziorowska, A, Kalaydjieva, L, Kayser, M, Kivisild, T, Kravchenko, S., Krumina, A, Kucinskas, V, Lavinha, J, Livshits, L. A., Malaspina, P, Syrrou, M, Mcelreavey, K, Meitinger, Ta, Mikelsaar, Av, Mitchell, Rj, Nafa, K, Nicholson, J, Nørby, S, Pandya, A, Parik, J, Patsalis, Pc, Pereira, L, Peterlin, B, Pielberg, G, Prata, Mj, Previderè, C, Roewer, L, Rootsi, S, Rubinsztein, Dc, Saillard, J, Santos, Fr, Stefanescu, G, Sykes, Bc, Tolun, A, Villems, R, Tyler Smith, C, and Jobling, Ma

Published
2000

7. Y-chromosomal diversity in Europe is clinal and influenced primarily by geography, rather than by language.

Author

Rosser, Z H, Zerjal, T, Hurles, M E, Adojaan, M, Alavantic, D, Amorim, A, Amos, W, Armenteros, M, Arroyo, E, Barbujani, G, Beckman, G, Beckman, L, Bertranpetit, J, Bosch, E, Bradley, D G, Brede, G, Cooper, G, Côrte-Real, H B, de Knijff, P, Decorte, R, Dubrova, Y E, Evgrafov, O, Gilissen, A, Glisic, S, Gölge, M, Hill, E W, Jeziorowska, A, Kalaydjieva, L, Kayser, M, Kivisild, T, Kravchenko, S A, Krumina, A, Kucinskas, V, Lavinha, J, Livshits, L A, Malaspina, P, Maria, S, McElreavey, K, Meitinger, T A, Mikelsaar, A V, Mitchell, R J, Nafa, K, Nicholson, J, Nørby, S, Pandya, A, Parik, J, Patsalis, P C, Pereira, L, Peterlin, B, Pielberg, G, Prata, M J, Previderé, C, Roewer, L, Rootsi, S, Rubinsztein, D C, Saillard, J, Santos, F R, Stefanescu, G, Sykes, B C, Tolun, A, Villems, R, Tyler-Smith, C, Jobling, M A, Rosser, Z H, Zerjal, T, Hurles, M E, Adojaan, M, Alavantic, D, Amorim, A, Amos, W, Armenteros, M, Arroyo, E, Barbujani, G, Beckman, G, Beckman, L, Bertranpetit, J, Bosch, E, Bradley, D G, Brede, G, Cooper, G, Côrte-Real, H B, de Knijff, P, Decorte, R, Dubrova, Y E, Evgrafov, O, Gilissen, A, Glisic, S, Gölge, M, Hill, E W, Jeziorowska, A, Kalaydjieva, L, Kayser, M, Kivisild, T, Kravchenko, S A, Krumina, A, Kucinskas, V, Lavinha, J, Livshits, L A, Malaspina, P, Maria, S, McElreavey, K, Meitinger, T A, Mikelsaar, A V, Mitchell, R J, Nafa, K, Nicholson, J, Nørby, S, Pandya, A, Parik, J, Patsalis, P C, Pereira, L, Peterlin, B, Pielberg, G, Prata, M J, Previderé, C, Roewer, L, Rootsi, S, Rubinsztein, D C, Saillard, J, Santos, F R, Stefanescu, G, Sykes, B C, Tolun, A, Villems, R, Tyler-Smith, C, and Jobling, M A

Abstract

Clinal patterns of autosomal genetic diversity within Europe have been interpreted in previous studies in terms of a Neolithic demic diffusion model for the spread of agriculture; in contrast, studies using mtDNA have traced many founding lineages to the Paleolithic and have not shown strongly clinal variation. We have used 11 human Y-chromosomal biallelic polymorphisms, defining 10 haplogroups, to analyze a sample of 3,616 Y chromosomes belonging to 47 European and circum-European populations. Patterns of geographic differentiation are highly nonrandom, and, when they are assessed using spatial autocorrelation analysis, they show significant clines for five of six haplogroups analyzed. Clines for two haplogroups, representing 45% of the chromosomes, are continentwide and consistent with the demic diffusion hypothesis. Clines for three other haplogroups each have different foci and are more regionally restricted and are likely to reflect distinct population movements, including one from north of the Black Sea. Principal-components analysis suggests that populations are related primarily on the basis of geography, rather than on the basis of linguistic affinity. This is confirmed in Mantel tests, which show a strong and highly significant partial correlation between genetics and geography but a low, nonsignificant partial correlation between genetics and language. Genetic-barrier analysis also indicates the primacy of geography in the shaping of patterns of variation. These patterns retain a strong signal of expansion from the Near East but also suggest that the demographic history of Europe has been complex and influenced by other major population movements, as well as by linguistic and geographic heterogeneities and the effects of drift.

Published
2000
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8. Y-chromosomal diversity in Europe is clinal and influenced primarily by geography, rather than by language

Author

Rosser, ZH, Zerjal, T, Hurles, ME, Adojaan, M, Alavantić, Dragan, Amorim, A, Amos, W, Armenteros, M, Arroyo, E, Barbujani, G, Beckman, G, Beckman, L, Bertranpetit, J, Bosch, E, Bradley, DG, Brede, G, Cooper, G, Corte-Real, HBSM, de Knijff, P, Decorte, R, Dubrova, YE, Evgrafov, O, Gilissen, A, Glišić, Sanja (I), Golge, M, Hill, EW, Jeziorowska, A, Kalaydjieva, L, Kayser, M, Kivisild, T, Kravchenko, SA, Krumina, A, Kucinskas, V, Lavinha, J, Livshits, LA, Malaspina, P, Maria, S, McElreavey, K, Meitinger, TA, Mikelsaar, AV, Mitchell, RJ, Nafa, K, Nicholson, J, Norby, S, Pandya, A, Parik, J, Patsalis, PC, Pereira, L, Peterlin, B, Pielberg, G, Prata, ML, Previdere, C, Roewer, L, Rootsi, S, Rubinsztein, DC, Saillard, J, Santos, FR, Stefanescu, G, Sykes, BC, Tolun, A, Villems, R, Tyler-Smith, C, Jobling, MA, Rosser, ZH, Zerjal, T, Hurles, ME, Adojaan, M, Alavantić, Dragan, Amorim, A, Amos, W, Armenteros, M, Arroyo, E, Barbujani, G, Beckman, G, Beckman, L, Bertranpetit, J, Bosch, E, Bradley, DG, Brede, G, Cooper, G, Corte-Real, HBSM, de Knijff, P, Decorte, R, Dubrova, YE, Evgrafov, O, Gilissen, A, Glišić, Sanja (I), Golge, M, Hill, EW, Jeziorowska, A, Kalaydjieva, L, Kayser, M, Kivisild, T, Kravchenko, SA, Krumina, A, Kucinskas, V, Lavinha, J, Livshits, LA, Malaspina, P, Maria, S, McElreavey, K, Meitinger, TA, Mikelsaar, AV, Mitchell, RJ, Nafa, K, Nicholson, J, Norby, S, Pandya, A, Parik, J, Patsalis, PC, Pereira, L, Peterlin, B, Pielberg, G, Prata, ML, Previdere, C, Roewer, L, Rootsi, S, Rubinsztein, DC, Saillard, J, Santos, FR, Stefanescu, G, Sykes, BC, Tolun, A, Villems, R, Tyler-Smith, C, and Jobling, MA

Abstract

Clinal patterns of autosomal genetic diversity within Europe have been interpreted in previous studies in terms of a Neolithic demic diffusion model for the spread of agriculture; in contrast, studies using mtDNA have traced many founding lineages to the Paleolithic and have not shown strongly clinal variation. We have used 11 human Y-chromosomal biallelic polymorphisms, defining 10 haplogroups, to analyze a sample of 3,616 Y chromosomes belonging to 47 European and circum-European populations. Patterns of geographic differentiation are highly nonrandom, and, when they are assessed using spatial autocorrelation analysis, they show significant dines for five of six haplogroups analyzed. Clines for two haplogroups, representing 45% of the chromosomes, are continentwide and consistent with the demic diffusion hypothesis. Clines for three other haplogroups each have different foci and are more regionally restricted and are likely to reflect distinct population movements, including one from north of the Black Sea. principal-components analysis suggests that populations are related primarily on the basis of geography, rather than on the basis of linguistic affinity. This is confirmed in Mantel tests, which show a strong and highly significant partial correlation between genetics and geography but a low nonsignificant partial correlation between genetics and language. Genetic-barrier analysis also indicates the primacy of geography in the shaping of patterns of variation. These patterns retain a strong signal of expansion from the Near East but also suggest that the demographic history of Europe has been complex and influenced by other major population movements, as well as by linguistic and geographic heterogeneities and the effects of drift.

Published
2000

15. Cloning and characterization of MDDX28, a putative dead-box helicase with mitochondrial and nuclear localization.

Author

Valgardsdottir, R, Brede, G, Eide, L G, Frengen, E, and Prydz, H

Abstract

A cDNA encoding a novel member of the helicase family, MDDX28, has been cloned from a human testis library. This apparently intronless gene was transcribed in all tissues studied. MDDX28 encodes a protein of 540 amino acids, with approximately 30% homology to other helicases over the core region, containing all the conserved DEAD-box helicase motifs. No homologue is known. MDDX28 has RNA and Mg(2+)-dependent ATPase activity. Subcellular localization studies of MDDX28 using oligoclonal antibodies raised against the protein as well as its enhanced green fluorescence protein (EGFP) demonstrated that the protein is localized in the mitochondria and the nucleus. To our knowledge, MDDX28 is the first member of the RNA helicase described with this dual location. The nuclear localization of MDDX28 depended on active RNA polymerase II transcription, suggesting that the protein could be transported to and from the nucleus. This was confirmed further in an interspecies heterokaryon assay, in which MDDX28 was seen to translocate to the nucleus and mitochondria. The mitochondrial uptake of the MDDX28-EGFP-N1 fusion protein was inhibited by carbonyl cyanide p-(trichloromethoxy)phenylhydrazone. Our results indicate that MDDX28 can be transported between the mitochondria and the nucleus.

Published
2001
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16. Secondary structure prediction and in vitro accessibility of mRNA as tools in the selection of target sites for ribozymes.

Author

Amarzguioui, M, Brede, G, Babaie, E, Grotli, M, Sproat, B, and Prydz, H

Abstract

We have investigated the relative merits of two commonly used methods for target site selection for ribozymes: secondary structure prediction (MFold program) and in vitro accessibility assays. A total of eight methylated ribozymes with DNA arms were synthesized and analyzed in a transient co-transfection assay in HeLa cells. Residual expression levels ranging from 23 to 72% were obtained with anti-PSKH1 ribozymes compared to cells transfected with an irrelevant control ribozyme. Ribozyme efficacy depended on both ribozyme concentration and the steady state expression levels of the target mRNA. Allylated ribozymes against a subset of the target sites generally displayed poorer efficacy than their methylated counterparts. This effect appeared to be influenced by in vivo accessibility of the target site. Ribozymes designed on the basis of either selection method displayed a wide range of efficacies with no significant differences in the average activities of the two groups of ribozymes. While in vitro accessibility assays had limited predictive power, there was a significant correlation between certain features of the predicted secondary structure of the target sequence and the efficacy of the corresponding ribozyme. Specifically, ribozyme efficacy appeared to be positively correlated with the presence of short stem regions and helices of low stability within their target sequences. There were no correlations with predicted free energy or loop length.

Published
2000
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17. Expression of murine leukemia viruses in RFM mice with host versus graft disease after perinatal inoculation of (T6 X RFM)F1 lymphohemopoietic cells

Author

Cross, S S, Brede, G, Tucker, H S, Maloney, M, Montour, J L, and Hard, R C

Abstract

Host versus graft disease is the fatal syndrome of altered immunity that follows the perinatal inoculation of related F1 hybrid spleen cells to susceptible strains of inbred mice. The allogenic reaction results in severe depletion of T-lymphocytes, but causes hyperplasia and hypersecretion of B-cells. Among the long-term survivors of acute host versus graft reactions, there is a high incidence of nonthymic lymphomas associated with ecotropic murine leukemia virus that may be of donor F1 origin. The present studies were done to determine whether ecotropic murine leukemia virus played any role in the pathogenesis of acute host versus graft disease in RFM mice perinatally inoculated with (T6 X RFM)F1 spleen cells. In RFM/(T6 X RFM)F1 chimeras, N-tropic murine leukemia virus can be detected as early as 3 days. The progression of the disease was accompanied by increasing viral expression. The inoculation of N-tropic virus of F1 donor origin into RFM neonates failed to induce disease, although the virus proliferated. Detection of progressively rising titers of antibody to murine leukemia virus linked the virus to the development of hyperimmunoglobulinemia by virtue of its ability to serve as a replicating source of antigens. These and other studies provided evidence that the seemingly paradoxical appearance of hyperimmunoglobulinemia in T-cell-deficient mice with the host versus graft syndrome is due, at least in part, to the stimulation of presensitized F1 donor B-cells, which are not destroyed in the allogenic reaction, as are the T-cells. Another unusual finding was the detection of polytropic murine leukemia virus in 25-day-old RFM/(T6 X RFM)F1 chimeras. It is suggested that the allogenic host versus graft reaction favored the formation of recombinants.

Published
1983
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19. tRNA-Derived Fragments as Biomarkers in Bladder Cancer.

Author

Strømme O, Heck KA, Brede G, Lindholm HT, Otterlei M, and Arum CJ

Abstract

Bladder cancer (BC) diagnosis is reliant on cystoscopy, an invasive procedure associated with urinary tract infections. This has sparked interest in identifying noninvasive biomarkers in body fluids such as blood and urine. A source of biomarkers in these biofluids are extracellular vesicles (EVs), nanosized vesicles that contain a wide array of molecular cargo, including small noncoding RNA such as transfer RNA-derived fragments (tRF) and microRNA. Here, we performed small-RNA next-generation sequencing from EVs from urine and serum, as well as from serum supernatant. RNA was extracted from 15 non-cancer patients (NCPs) with benign findings in cystoscopy and 41 patients with non-muscle invasive BC. Urine and serum were collected before transurethral resection of bladder tumors (TUR-b) and at routine post-surgery check-ups. We compared levels of tRFs in pre-surgery samples to samples from NCPs and post-surgery check-ups. To further verify our findings, samples from 10 patients with stage T1 disease were resequenced. When comparing tRF expression in urine EVs between T1 stage BC patients and NCPs, 14 differentially expressed tRFs (DEtRFs) were identified. In serum supernatant, six DEtRFs were identified among stage T1 patients when comparing pre-surgery to post-surgery samples and four DEtRFs were found when comparing pre-surgery samples to NCPs. By performing a blast search, we found that sequences of DEtRFs aligned with genomic sequences pertaining to processes relevant to cancer development, such as enhancers, regulatory elements and CpG islands. Our findings display a number of tRFs that may hold potential as biomarkers for the diagnosis and recurrence-free survival of BC.

Published
2024
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20. Differentially Expressed Extracellular Vesicle-Contained microRNAs before and after Transurethral Resection of Bladder Tumors.

Author

Strømme O, Heck KA, Brede G, Lindholm HT, Otterlei M, and Arum CJ

Subjects
Aged, Aged, 80 and over, Apoptosis genetics, Biomarkers, Tumor blood, Biomarkers, Tumor urine, Cell Differentiation genetics, Female, Gene Ontology, Humans, Male, MicroRNAs blood, MicroRNAs urine, Middle Aged, Signal Transduction genetics, Urinary Bladder Neoplasms surgery, Biomarkers, Tumor genetics, Extracellular Vesicles genetics, Gene Expression Profiling methods, Gene Expression Regulation, Neoplastic, MicroRNAs genetics, Urinary Bladder Neoplasms genetics
Abstract

Bladder cancer (BC) is currently diagnosed and monitored by cystoscopy, a costly and invasive procedure. Potential biomarkers in urine, blood, and, more recently, extracellular vesicles (EVs), have been explored as non-invasive alternatives for diagnosis and surveillance of BC. EVs are nanovesicles secreted by most cell types containing diverse molecular cargo, including different types of small RNAs, such as microRNA (miRNA). In this study, we performed next-generation sequencing of EV-contained miRNA isolated from urine and serum of 41 patients with non-muscle invasive BC (27 stage Ta, 14 stage T1) and 15 non-cancer patients (NCP) with benign cystoscopy findings. MiRNA sequencing was also performed on serum supernatant samples for T1 patients. To identify potential BC-specific biomarkers, expression levels of miRNA in presurgery samples were compared to those at postsurgery check-ups, and to NCPs. Results showed that two miRNAs, urinary EV-contained miR-451a and miR-486-5p, were significantly upregulated in presurgery samples from T1 patients compared to postsurgery check-up samples. This was confirmed in a replica EV/RNA isolation and sequencing run of 10 T1 patients from the primary run; however, analyses revealed no differential expression of miRNAs in serum EVs, serum supernatant, or when comparing BC patients to NCPs. This is the first study to investigate EV-containing miRNA sequencing in pre- and postsurgery BC patient samples and our findings suggest that urinary EV-contained miR-451a and miR-486-5p may be potential biomarkers for recurrence-free survival of BC patients with stage T1 disease.

Published
2021
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21. Myeloma-derived extracellular vesicles mediate HGF/c-Met signaling in osteoblast-like cells.

Author

Strømme O, Psonka-Antonczyk KM, Stokke BT, Sundan A, Arum CJ, and Brede G

Subjects
Bone Neoplasms metabolism, Bone Neoplasms pathology, Cells, Cultured, Humans, Multiple Myeloma pathology, Osteoblasts cytology, Osteosarcoma pathology, Phosphorylation, Extracellular Vesicles metabolism, Hepatocyte Growth Factor metabolism, Multiple Myeloma metabolism, Osteoblasts metabolism, Osteosarcoma metabolism, Proteoglycans metabolism, Proto-Oncogene Proteins c-met metabolism
Abstract

Multiple myeloma is an incurable cancer of antibody-producing plasma cells. Hepatocyte growth factor (HGF), a cytokine aberrantly expressed in half of myeloma patients, is involved in myeloma pathogenesis by enhancing myeloma growth and invasiveness, and may play a role in myeloma bone disease by inhibiting osteoblastogenesis. In this study, we investigated whether extracellular vesicles (EVs) may play a role in HGF signaling between myeloma cells and osteoblast-like target cells. EVs from the HGF-positive cell line JJN-3 and the HGF-negative cell line INA-6, and from bone marrow plasma and primary human myeloma cells, were isolated using sequential centrifugation techniques and the presence of HGF on the EV-surface was investigated with ELISA. EVs from both cell lines were added to an established bioassay where HGF is known to induce interleukin-11 secretion in osteoblast-like cells. Our results show that HGF was bound to the surface of JJN-3-derived EVs, while INA-6-derived EVs were negative for HGF. Only JJN-3-derived EVs induced IL-11 secretion in osteoblast-like recipient cells. When osteoblast-like cells were preincubated with a specific HGF-receptor (c-Met) inhibitor, no induction of interleukin-11 was observed. Downstream c-Met phosphorylation was demonstrated by immunoblotting. EVs isolated from bone marrow plasma and primary myeloma cells were HGF-positive for a subset of myeloma patients. Taken together, this work shows for the first time that HGF bound on the surface of myeloma-derived EVs can effectuate HGF/c-Met signaling in osteoblast-like cells. Myeloma-derived EVs may play a role in myeloma bone disease by induction of the osteoclast-activating cytokine interleukin-11 in osteoblasts., (Copyright © 2019 Elsevier Inc. All rights reserved.)

Published
2019
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22. Photochemical Internalization of Peptide Antigens Provides a Novel Strategy to Realize Therapeutic Cancer Vaccination.

Author

Haug M, Brede G, Håkerud M, Nedberg AG, Gederaas OA, Flo TH, Edwards VT, Selbo PK, Høgset A, and Halaas Ø

Subjects
Animals, Antigen Presentation, Antigens, Neoplasm immunology, Cytotoxicity, Immunologic, Endocytosis, Humans, Injections, Intradermal, Mice, Neoplasms immunology, Peptides immunology, Photochemical Processes, CD8-Positive T-Lymphocytes immunology, Cancer Vaccines immunology, Immunotherapy methods, Neoplasms therapy, Vaccination methods
Abstract

Effective priming and activation of tumor-specific CD8+ cytotoxic T lymphocytes (CTLs) is crucial for realizing the potential of therapeutic cancer vaccination. This requires cytosolic antigens that feed into the MHC class I presentation pathway, which is not efficiently achieved with most current vaccination technologies. Photochemical internalization (PCI) provides an emerging technology to route endocytosed material to the cytosol of cells, based on light-induced disruption of endosomal membranes using a photosensitizing compound. Here, we investigated the potential of PCI as a novel, minimally invasive, and well-tolerated vaccination technology to induce priming of cancer-specific CTL responses to peptide antigens. We show that PCI effectively promotes delivery of peptide antigens to the cytosol of antigen-presenting cells (APCs) in vitro . This resulted in a 30-fold increase in MHC class I/peptide complex formation and surface presentation, and a subsequent 30- to 100-fold more efficient activation of antigen-specific CTLs compared to using the peptide alone. The effect was found to be highly dependent on the dose of the PCI treatment, where optimal doses promoted maturation of immature dendritic cells, thus also providing an adjuvant effect. The effect of PCI was confirmed in vivo by the successful induction of antigen-specific CTL responses to cancer antigens in C57BL/6 mice following intradermal peptide vaccination using PCI technology. We thus show new and strong evidence that PCI technology holds great potential as a novel strategy for improving the outcome of peptide vaccines aimed at triggering cancer-specific CD8+ CTL responses.

Published
2018
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23. Erythropoietin (EPO)-receptor signaling induces cell death of primary myeloma cells in vitro.

Author

Våtsveen TK, Sponaas AM, Tian E, Zhang Q, Misund K, Sundan A, Børset M, Waage A, and Brede G

Subjects
Bone Marrow pathology, Cell Survival drug effects, Erythropoietin pharmacology, Humans, Phosphorylation drug effects, Protein Kinases metabolism, RNA, Messenger blood, Receptors, Erythropoietin analysis, Receptors, Erythropoietin genetics, Signal Transduction physiology, Tumor Cells, Cultured, Cell Death, Multiple Myeloma pathology, Receptors, Erythropoietin physiology
Abstract

Background: Multiple myeloma is an incurable complex disease characterized by clonal proliferation of malignant plasma cells in a hypoxic bone marrow environment. Hypoxia-dependent erythropoietin (EPO)-receptor (EPOR) signaling is central in various cancers, but the relevance of EPOR signaling in multiple myeloma cells has not yet been thoroughly investigated., Methods: Myeloma cell lines and malignant plasma cells isolated from bone marrow of myeloma patients were used in this study. Transcript levels were analysed by quantitative PCR and cell surface levels of EPOR in primary cells by flow cytometry. Knockdown of EPOR by short interfering RNA was used to show specific EPOR signaling in the myeloma cell line INA-6. Flow cytometry was used to assess viability in primary cells treated with EPO in the presence and absence of neutralizing anti-EPOR antibodies. Gene expression data for total therapy 2 (TT2), total therapy 3A (TT3A) trials and APEX 039 and 040 were retrieved from NIH GEO omnibus and EBI ArrayExpress., Results: We show that the EPOR is expressed in myeloma cell lines and in primary myeloma cells both at the mRNA and protein level. Exposure to recombinant human EPO (rhEPO) reduced viability of INA-6 myeloma cell line and of primary myeloma cells. This effect could be partially reversed by neutralizing antibodies against EPOR. In INA-6 cells and primary myeloma cells, janus kinase 2 (JAK-2) and extracellular signal regulated kinase 1 and 2 (ERK-1/2) were phosphorylated by rhEPO treatment. Knockdown of EPOR expression in INA-6 cells reduced rhEPO-induced phospo-JAK-2 and phospho-ERK-1/2. Co-cultures of primary myeloma cells with bone marrow-derived stroma cells did not protect the myeloma cells from rhEPO-induced cell death. In four different clinical trials, survival data linked to gene expression analysis indicated that high levels of EPOR mRNA were associated with better survival., Conclusions: Our results demonstrate for the first time active EPOR signaling in malignant plasma cells. EPO-mediated EPOR signaling reduced the viability of myeloma cell lines and of malignant primary plasma cells in vitro. Our results encourage further studies to investigate the importance of EPO/EPOR in multiple myeloma progression and treatment., Trial Registration: [Trial registration number for Total Therapy (TT) 2: NCT00083551 and TT3: NCT00081939 ].

Published
2016
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24. A-kinase anchoring protein AKAP95 is a novel regulator of ribosomal RNA synthesis.

Author

Marstad A, Landsverk OJ, Strømme O, Otterlei M, Collas P, Sundan A, and Brede G

Subjects
A Kinase Anchor Proteins genetics, Cell Line, HEK293 Cells, Humans, A Kinase Anchor Proteins metabolism, RNA, Ribosomal biosynthesis
Abstract

The RNA polymerase I transcription apparatus acquires and integrates the combined information from multiple cellular signalling cascades to regulate ribosome production essential for cell growth and proliferation. In the present study, we show that a subpopulation of A-kinase anchoring protein 95 (AKAP95) targets the nucleolus during interphase and is involved in regulating rRNA production. We show that AKAP95 co-localizes with the nucleolar upstream binding factor, an essential rRNA transcription factor. Similar to other members of the C2 H2 -zinc finger family, we show, using systematic selection and evolution of ligands by exponential enrichment and in vitro binding analysis, that AKAP95 has a preference for GC-rich DNA in vitro, whereas fluorescence recovery after photobleaching analysis reveals AKAP95 to be a highly mobile protein that exhibits RNA polymerase I and II dependent nucleolar trafficking. In line with its GC-binding features, chromatin immunoprecipitation analysis revealed AKAP95 to be associated with ribosomal chromatin in vivo. Manipulation of AKAP95-expression in U2OS cells revealed a reciprocal relationship between the expression of AKAP95 and 47S rRNA. Taken together, our data indicate that AKAP95 is a novel nucleolus-associated protein with a regulatory role on rRNA production., (© 2015 Federation of European Biochemical Societies.)

Published
2016
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25. Human Breast Milk miRNA, Maternal Probiotic Supplementation and Atopic Dermatitis in Offspring.

Author

Simpson MR, Brede G, Johansen J, Johnsen R, Storrø O, Sætrom P, and Øien T

Subjects
Adult, Dietary Supplements, Female, Humans, Infant, Infant, Newborn, Male, MicroRNAs analysis, Perinatal Care, Pregnancy, Probiotics administration & dosage, Probiotics analysis, Dermatitis, Atopic prevention & control, MicroRNAs metabolism, Milk, Human metabolism, Prenatal Exposure Delayed Effects, Probiotics pharmacokinetics
Abstract

Background: Perinatal probiotic ingestion has been shown to prevent atopic dermatitis (AD) in infancy in a number of randomised trials. The Probiotics in the Prevention of Allergy among Children in Trondheim (ProPACT) trial involved a probiotic supplementation regime given solely to mothers in the perinatal period and demonstrated a ~40% relative risk reduction in the cumulative incidence of AD at 2 years of age. However, the mechanisms behind this effect are incompletely understood. Micro-RNAs (miRNA) are abundant in mammalian milk and may influence the developing gastrointestinal and immune systems of newborn infants. The objectives of this study were to describe the miRNA profile of human breast milk, and to investigate breast milk miRNAs as possible mediators of the observed preventative effect of probiotics., Methods: Small RNA sequencing was conducted on samples collected 3 months postpartum from 54 women participating in the ProPACT trial. Differential expression of miRNA was assessed for the probiotic vs placebo and AD vs non-AD groups. The results were further analysed using functional prediction techniques., Results: Human breast milk samples contain a relatively stable core group of highly expressed miRNAs, including miR-148a-3p, miR-22-3p, miR-30d-5p, let-7b-5p and miR-200a-3p. Functional analysis of these miRNAs revealed enrichment in a broad range of biological processes and molecular functions. Although several miRNAs were found to be differentially expressed on comparison of the probiotic vs placebo and AD vs non-AD groups, none had an acceptable false discovery rate and their biological significance in the development of AD is not immediately apparent from their predicted functional consequences., Conclusion: Whilst breast milk miRNAs have the potential to be active in a diverse range of tissues and biological process, individual miRNAs in breast milk 3 months postpartum are unlikely to play a major role in the prevention of atopic dermatitis in infancy by probiotics ingestion in the perinatal period., Trial Registration: ClinicalTrials.gov NCT00159523.

Published
2015
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26. Allelic mutations in noncoding genomic sequences construct novel transcription factor binding sites that promote gene overexpression.

Author

Tian E, Børset M, Sawyer JR, Brede G, Våtsveen TK, Hov H, Waage A, Barlogie B, Shaughnessy JD Jr, Epstein J, and Sundan A

Subjects
Binding Sites, Cell Line, Tumor, Hepatocyte Growth Factor genetics, Hepatocyte Growth Factor metabolism, Humans, Multiple Myeloma metabolism, Polymorphism, Single Nucleotide, Promoter Regions, Genetic, Alleles, Gene Expression Regulation, Neoplastic, Genome, Human, Multiple Myeloma genetics, Mutation, Transcription Factors metabolism
Abstract

The growth and survival factor hepatocyte growth factor (HGF) is expressed at high levels in multiple myeloma (MM) cells. We report here that elevated HGF transcription in MM was traced to DNA mutations in the promoter alleles of HGF. Sequence analysis revealed a previously undiscovered single-nucleotide polymorphism (SNP) and crucial single-nucleotide variants (SNVs) in the promoters of myeloma cells that produce large amounts of HGF. The allele-specific mutations functionally reassembled wild-type sequences into the motifs that affiliate with endogenous transcription factors NFKB (nuclear factor kappa-B), MZF1 (myeloid zinc finger 1), and NRF-2 (nuclear factor erythroid 2-related factor 2). In vitro, a mutant allele that gained novel NFKB-binding sites directly responded to transcriptional signaling induced by tumor necrosis factor alpha (TNFα) to promote high levels of luciferase reporter. Given the recent discovery by genome-wide sequencing (GWS) of numerous non-coding mutations in myeloma genomes, our data provide evidence that heterogeneous SNVs in the gene regulatory regions may frequently transform wild-type alleles into novel transcription factor binding properties to aberrantly interact with dysregulated transcriptional signals in MM and other cancer cells., (© 2015 Wiley Periodicals, Inc.)

Published
2015
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27. Involvement of the catalytic subunit of protein kinase A and of HA95 in pre-mRNA splicing.

Author

Kvissel AK, Ørstavik S, Eikvar S, Brede G, Jahnsen T, Collas P, Akusjärvi G, and Skålhegg BS

Subjects
A Kinase Anchor Proteins, Adaptor Proteins, Signal Transducing analysis, Animals, Catalytic Domain, Cell Line, Tumor, Cell Nucleus enzymology, Cyclic AMP pharmacology, Cyclic AMP-Dependent Protein Kinase Catalytic Subunits, Cyclic AMP-Dependent Protein Kinases analysis, Humans, Mice, Mice, Knockout, Phosphorylation, Adaptor Proteins, Signal Transducing metabolism, Cyclic AMP-Dependent Protein Kinases metabolism, RNA Precursors metabolism, RNA Splicing drug effects
Abstract

Protein kinase A (PKA) is a holoenzyme consisting of two catalytic (C) subunits bound to a regulatory (R) subunit dimer. Stimulation by cAMP dissociates the holoenzyme and causes translocation to the nucleus of a fraction of the C subunit. Apart from transcription regulation, little is known about the function of the C subunit in the nucleus. In the present report, we show that both Calpha and Cbeta are localized to spots in the mammalian nucleus. Double immunofluorescence analysis of splicing factor SC35 with the C subunit indicated that these spots are splicing factor compartments (SFCs). Using the E1A in vivo splicing assay, we found that catalytically active C subunits regulate alternative splicing and phosphorylate several members of the SR-protein family of splicing factors in vitro. Furthermore, nuclear C subunits co-localize with the C subunit-binding protein homologous to AKAP95, HA95. HA95 also regulates E1A alternative splicing in vivo, apparently through its N-terminal domain. Localization of the C subunit to SFCs and the E1A splicing pattern were unaffected by cAMP stimulation. Our findings demonstrate that the nuclear PKA C subunit co-locates with HA95 in SFCs and regulates pre-mRNA splicing, possibly through a cAMP-independent mechanism.

Published
2007
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28. Mutants of the protein serine kinase PSKH1 disassemble the Golgi apparatus.

Author

Brede G, Solheim J, Stang E, and Prydz H

Subjects
Acylation, Animals, COS Cells, Cell Membrane metabolism, Chlorocebus aethiops, Endosomes metabolism, Endosomes ultrastructure, Fatty Acids, Genetic Vectors, Golgi Apparatus ultrastructure, Humans, Intracellular Membranes metabolism, Microscopy, Electron, Protein Serine-Threonine Kinases metabolism, Protein Transport, Transfection, Transport Vesicles metabolism, Golgi Apparatus metabolism, Mutation, Protein Serine-Threonine Kinases genetics, Protein Serine-Threonine Kinases physiology
Abstract

We have dissected the molecular determinants involved in targeting the protein serine kinase PSKH1 to the endoplasmic reticulum (ER), the Golgi apparatus, and the plasma membrane (PM). Given this intracellular localization pattern, a potential role of PSKH1 in the secretory pathway was explored. The amino-terminal of PSKH1 revealed a striking similarity to the often acylated Src homology domain 4 (SH4)-harboring nonreceptor tyrosine kinases. Biochemical studies demonstrated that PSKH1 is myristoylated on glycine 2 and palmitoylated on cysteine 3. Dual amino-terminal acylation targets PSKH1 to Golgi as shown by colocalization with beta-COP and GM130, while nonpalmitoylated (myristoylated only) PSKH1 targets intracellular membranes colocalizing with protein disulphide isomerase (PDI, a marker for ER). Immunoelectron microscopy revealed that the dually acylated amino-terminal domain (in fusion with EGFP) was targeted to Golgi membranes as well as to the plasma membrane (PM), suggesting that the amino-terminal domain provides PSKH1 with membrane specificity dependent on its fatty acylation status. Subcellular fractionation by sucrose gradient analysis confirmed the impact of dual fatty acylation on endomembrane targeting, while cytosol and membrane fractioning revealed that myristoylation but not palmitoylation was required for general membrane association. A minimal region required for proper Golgi targeting of PSKH1 was identified within the first 29 amino acids. Expression of a PSKH1 mutant where the COOH-terminal kinase domain was swapped with green fluorescent protein and cysteine 3 was exchanged with serine resulted in disassembly of the Golgi apparatus as visualized by redistribution of beta-COP and GM130 to a diffuse cytoplasmic pattern, while leaving the tubulin skeleton intact. Our results suggest a structural and regulatory role of PSKH1 in maintenance of the Golgi apparatus, a key organelle within the secretory pathway.

Published
2003
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29. Y-chromosomal diversity in Europe is clinal and influenced primarily by geography, rather than by language.

Author

Rosser ZH, Zerjal T, Hurles ME, Adojaan M, Alavantic D, Amorim A, Amos W, Armenteros M, Arroyo E, Barbujani G, Beckman G, Beckman L, Bertranpetit J, Bosch E, Bradley DG, Brede G, Cooper G, Côrte-Real HB, de Knijff P, Decorte R, Dubrova YE, Evgrafov O, Gilissen A, Glisic S, Gölge M, Hill EW, Jeziorowska A, Kalaydjieva L, Kayser M, Kivisild T, Kravchenko SA, Krumina A, Kucinskas V, Lavinha J, Livshits LA, Malaspina P, Maria S, McElreavey K, Meitinger TA, Mikelsaar AV, Mitchell RJ, Nafa K, Nicholson J, Nørby S, Pandya A, Parik J, Patsalis PC, Pereira L, Peterlin B, Pielberg G, Prata MJ, Previderé C, Roewer L, Rootsi S, Rubinsztein DC, Saillard J, Santos FR, Stefanescu G, Sykes BC, Tolun A, Villems R, Tyler-Smith C, and Jobling MA

Subjects
Africa, Northern, Alleles, Emigration and Immigration, Europe, Gene Frequency genetics, Genetic Markers genetics, Haplotypes genetics, Humans, Linguistics, Male, Models, Genetic, Oceans and Seas, Phylogeny, Polymorphism, Genetic genetics, Genetic Variation genetics, Geography, Language, Y Chromosome genetics
Abstract

Clinal patterns of autosomal genetic diversity within Europe have been interpreted in previous studies in terms of a Neolithic demic diffusion model for the spread of agriculture; in contrast, studies using mtDNA have traced many founding lineages to the Paleolithic and have not shown strongly clinal variation. We have used 11 human Y-chromosomal biallelic polymorphisms, defining 10 haplogroups, to analyze a sample of 3,616 Y chromosomes belonging to 47 European and circum-European populations. Patterns of geographic differentiation are highly nonrandom, and, when they are assessed using spatial autocorrelation analysis, they show significant clines for five of six haplogroups analyzed. Clines for two haplogroups, representing 45% of the chromosomes, are continentwide and consistent with the demic diffusion hypothesis. Clines for three other haplogroups each have different foci and are more regionally restricted and are likely to reflect distinct population movements, including one from north of the Black Sea. Principal-components analysis suggests that populations are related primarily on the basis of geography, rather than on the basis of linguistic affinity. This is confirmed in Mantel tests, which show a strong and highly significant partial correlation between genetics and geography but a low, nonsignificant partial correlation between genetics and language. Genetic-barrier analysis also indicates the primacy of geography in the shaping of patterns of variation. These patterns retain a strong signal of expansion from the Near East but also suggest that the demographic history of Europe has been complex and influenced by other major population movements, as well as by linguistic and geographic heterogeneities and the effects of drift.

Published
2000
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30. Characterization of PSKH1, a novel human protein serine kinase with centrosomal, golgi, and nuclear localization.

Author

Brede G, Solheim J, Tröen G, and Prydz H

Subjects
Amino Acid Sequence, Base Sequence, Calcium-Calmodulin-Dependent Protein Kinase Type 1, Calcium-Calmodulin-Dependent Protein Kinases genetics, Cell Compartmentation, Cloning, Molecular, Humans, Male, Molecular Sequence Data, Nuclear Proteins genetics, Phosphorylation, Protein Sorting Signals, Protein Transport, Sequence Homology, Amino Acid, Serine metabolism, Testis enzymology, Tissue Distribution, Cell Nucleus enzymology, Centrosome enzymology, Golgi Apparatus enzymology, Protein Serine-Threonine Kinases genetics
Abstract

We report here the characterization of PSKH1, a novel human protein serine kinase with multiple intracellular localizations. The gene consists of three exons distributed over 35 kb of genomic DNA in region 16q22.1. The 3.4-kb cDNA predicts a protein of 424 amino acids with a calculated molecular mass of 48.1 kDa and pI of 9.6. PSKH1 is expressed in all tissues and cell lines tested as shown by Northern blots, with the highest level of abundance in testis. PSKH1 displays the highest level of similarity with rat CaM kinase I (50. 2%) over 259 amino acids in the conserved catalytic region, but lacks significant homology with proteins in the database outside the catalytic core. Polyclonal antibodies have been raised, and indirect immunofluorescence microscopy of untransfected COS-1 cells suggests that PSKH1 is localized in the Brefeldin A-sensitive Golgi compartment, at centrosomes, in the nucleus with a somewhat speckle-like presence, and more diffusely in the cytoplasm. The presence in the centrosome appears to be enhanced during osmotic stress. Immunoisolated PSKH1 does not phosphorylate any of the common kinase substrates in vitro, but autophosphorylates exclusively serines within its COOH-terminal region in an intermolecular fashion. Furthermore, autophosphorylation activity is repressed upon addition of Ca(2+)/CaM, suggesting that PSKH1 activity depends on Ca(2+) concentration in vivo., (Copyright 2000 Academic Press.)

Published
2000
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31. The gene cluster containing the LCAT gene is conserved between human and pig.

Author

Frengen E, Thomsen PD, Brede G, Solheim J, de Jong PJ, and Prydz H

Subjects
Animals, Base Sequence, Chromosomes, DNA, Complementary, Humans, In Situ Hybridization, Fluorescence, Molecular Sequence Data, Restriction Mapping, Swine, Chromosome Mapping, Conserved Sequence, Multigene Family, Phosphatidylcholine-Sterol O-Acyltransferase genetics
Abstract

A pooled DNA probe from P1 artificial chromosome clones (PACs) containing the human lecithin:cholesterol acyl transferase (LCAT) gene cluster was used in fluorescence in situ hybridization (FISH) experiments assigning the genes to pig chromosome 6p13. In addition, probes derived from the coding regions in the human gene cluster were used in long range mapping experiments to show that the overall structures of the human and porcine LCAT gene clusters are identical. Both the linear order and the close physical distance of five apparently unrelated genes have been maintained throughout 90 million years of divergent evolution between human and pig. The extremely dense clustering of the genes in the LCAT gene cluster suggests that this gene organization has biological significance. The conservation of the gene cluster between human and pig supports this suggestion.

Published
1997
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32. Cytogenetic studies of RFM mice which are susceptible to host versus graft disease following the perinatal inoculations of (T6 x RFM)F1 spleen cells and of T6T6 mice which are not.

Author

Hard RC Jr, Cross SS, Brede G, Montour JL, and Carter WH

Subjects
Animals, Crosses, Genetic, Female, Genetic Markers, Immune Tolerance, Kidney ultrastructure, Lymph Nodes ultrastructure, Male, Mice, Mice, Inbred DBA, Mice, Inbred Strains, Microscopy, Electron, Spleen transplantation, Spleen ultrastructure, T-Lymphocytes, H-2 Antigens genetics, Host vs Graft Reaction, Immunologic Deficiency Syndromes genetics
Published
1981
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