Your search keyword '"Ove Bruland"' showing total 63 results

1. Functional characterization of all‐trans retinoic acid‐induced differentiation factor (ATRAID)

Author

Roya Mehrasa, Ileana Cristea, Cecilie Bredrup, Eyvind Rødahl, and Ove Bruland

Subjects

ATRAID, endosomes, Golgi, isoform, N‐glycosylation, RAB11, Biology (General), QH301-705.5

Abstract

All‐trans retinoic acid‐induced differentiation (ATRAID) factor was first identified in HL60 cells. Several mRNA isoforms exist, but the respective proteins have not been fully characterized. In transfected cells expressing Myc‐Flag‐tagged ATRAID Isoform (Iso) A, B, and C, Iso C was found to be expressed at high levels, Iso A was found to be expressed at low levels due to rapid degradation, and the predicted protein expressed from Iso B was not detected. Iso C was present mainly in an N‐glycosylated form. In subcellular fractionation experiments, Iso C localized to the membranous and nuclear fractions, while immunofluorescence analysis revealed that Iso C is located close to the plasma membrane, mainly in cytoplasmic vesicles and in the Golgi area. We confirm that Iso C colocalizes to some extent with endosomal/lysosomal markers LAMP1 and LAMP2. Furthermore, we show that ATRAID co‐localizes with RAB11, a GTPase associated with recycling endosomes and implicated in regulating vesicular trafficking.

Published

2023

2. Xeno-free generation of human induced pluripotent stem cells from donor-matched fibroblasts isolated from dermal and oral tissues

Author

Hassan R. W. Ali, Salwa Suliman, Tarig Al-Hadi Osman, Manuel Carrasco, Ove Bruland, Daniela-Elena Costea, Helge Ræder, and Kamal Mustafa

Subjects

Platelet lysate, Fetal bovine serum, Fibroblasts, Xenogenic, Pluripotency, Medicine (General), R5-920, Biochemistry, QD415-436

Abstract

Abstract Background Induced pluripotent stem cells (iPS) can be generated from various somatic cells and can subsequently be differentiated to multiple cell types of the body. This makes them highly promising for cellular therapy in regenerative medicine. However, to facilitate their clinical use and to ensure safety, iPS culturing protocols must be compliant with good manufacturing practice guidelines and devoid of xenogenic products. Therefore, we aimed to compare the efficiency of using humanized culture conditions, specifically human platelet lysate to fetal bovine serum, for iPS generation from different sources, and to evaluate their stemness. Methods iPS were generated via a platelet lysate or fetal bovine serum-based culturing protocol from matched dermal, buccal and gingival human fibroblasts, isolated from healthy donors (n = 2) after informed consent, via episomal plasmid transfection. Pluripotency, genotype and phenotype of iPS, generated by both protocols, were then assessed by various methods. Results More attempts were generally required to successfully reprogram xeno-free fibroblasts to iPS, as compared to xenogenic cultured fibroblasts. Furthermore, oral fibroblasts generally required more attempts for successful iPS generation as opposed to dermal fibroblasts. Morphologically, all iPS generated from fibroblasts formed tight colonies surrounded by a reflective “whitish” outer rim, typical for iPS. They also expressed pluripotency markers at both gene (SOX2, OCT4, NANOG) and protein level (SOX2, OCT4). Upon stimulation, all iPS showed ability to differentiate into the three primary germ layers via expression of lineage-specific markers for mesoderm (MESP1, OSR1, HOPX), endoderm (GATA4) and ectoderm (PAX6, RAX). Genome analysis revealed several amplifications and deletions within the chromosomes of each iPS type. Conclusions The xeno-free protocol had a lower reprogramming efficiency compared to the standard xenogenic protocol. The oral fibroblasts generally proved to be more difficult to reprogram than dermal fibroblasts. Xeno-free dermal, buccal and gingival fibroblasts can successfully generate iPS with a comparable genotype/phenotype to their xenogenic counterparts.

Published

2023

3. Activity monitoring and patient-reported outcome measures in Myalgic Encephalomyelitis/Chronic Fatigue Syndrome patients

Author

Ingrid G. Rekeland, Kari Sørland, Ove Bruland, Kristin Risa, Kine Alme, Olav Dahl, Karl J. Tronstad, Olav Mella, and Øystein Fluge

Subjects

Medicine, Science

Abstract

Introduction Myalgic Encephalomyelitis/Chronic Fatigue Syndrome (ME/CFS) is a disease with no validated specific and sensitive biomarker, and no standard approved treatment. In this observational study with no intervention, participants used a Fitbit activity tracker. The aims were to explore natural symptom variation, feasibility of continuous activity monitoring, and to compare activity data with patient reported outcome measures (PROMs). Materials and methods In this pilot study, 27 patients with mild to severe ME/CFS, of mean age 42.3 years, used the Fitbit Charge 3 continuously for six months. Patients wore a SenseWear activity bracelet for 7 days at baseline, at 3 and 6 months. At baseline and follow-up they completed the Short Form 36 Health Survey (SF-36) and the DePaul Symptom Questionnaire–Short Form (DSQ-SF). Results The mean number of steps per day decreased with increasing ME/CFS severity; mild 5566, moderate 4991 and severe 1998. The day-by-day variation was mean 47% (range 25%–79%). Mean steps per day increased from the first to the second three-month period, 4341 vs 4781 steps, p = 0.022. The maximum differences in outcome measures between 4-week periods (highest vs lowest), were more evident in a group of eight patients with milder disease (baseline SF-36 PF > 50 or DSQ-SF < 55) as compared to 19 patients with higher symptom burden (SF-36 PF < 50 and DSQ-SF > 55), for SF-36 PF raw scores: 16.9 vs 3.4 points, and for steps per day: 958 versus 479 steps. The correlations between steps per day and self-reported SF-36 Physical function, SF-36 Social function, and DSQ-SF were significant. Fitbit recorded significantly higher number of steps than SenseWear. Resting heart rates were stable during six months. Conclusion Continuous activity registration with Fitbit Charge 3 trackers is feasible and useful in studies with ME/CFS patients to monitor steps and resting heart rate, in addition to self-reported outcome measures. Clinical trial registration Clinicaltrials.gov: NCT04195815.

Published

2022

4. GBA2 Mutations Cause a Marinesco-Sjögren-Like Syndrome: Genetic and Biochemical Studies.

Author

Kristoffer Haugarvoll, Stefan Johansson, Carlos E Rodriguez, Helge Boman, Bjørn Ivar Haukanes, Ove Bruland, Francisco Roque, Inge Jonassen, Maria Blomqvist, Wenche Telstad, Jan-Eric Månsson, Per Morten Knappskog, and Laurence A Bindoff

Subjects

Medicine, Science

Abstract

With the advent new sequencing technologies, we now have the tools to understand the phenotypic diversity and the common occurrence of phenocopies. We used these techniques to investigate two Norwegian families with an autosomal recessive cerebellar ataxia with cataracts and mental retardation.Single nucleotide polymorphism (SNP) chip analysis followed by Exome sequencing identified a 2 bp homozygous deletion in GBA2 in both families, c.1528_1529del [p.Met510Valfs*17]. Furthermore, we report the biochemical characterization of GBA2 in these patients. Our studies show that a reduced activity of GBA2 is sufficient to elevate the levels of glucosylceramide to similar levels as seen in Gaucher disease. Furthermore, leucocytes seem to be the proper enzyme source for in vitro analysis of GBA2 activity.We report GBA2 mutations causing a Marinesco-Sjögren-like syndrome in two Norwegian families. One of the families was originally diagnosed with Marinesco-Sjögren syndrome based on an autosomal recessive cerebellar ataxia with cataracts and mental retardation. Our findings highlight the phenotypic variability associated with GBA2 mutations, and suggest that patients with Marinesco-Sjögren-like syndromes should be tested for mutations in this gene.

Published

2017

5. Adenoviral Mediated Expression of BMP2 by Bone Marrow Stromal Cells Cultured in 3D Copolymer Scaffolds Enhances Bone Formation.

Author

Sunita Sharma, Dipak Sapkota, Ying Xue, Yang Sun, Anna Finne-Wistrand, Ove Bruland, and Kamal Mustafa

Subjects

Medicine, Science

Abstract

Selection of appropriate osteoinductive growth factors, suitable delivery method and proper supportive scaffold are critical for a successful outcome in bone tissue engineering using bone marrow stromal cells (BMSC). This study examined the molecular and functional effect of a combination of adenoviral mediated expression of bone morphogenetic protein-2 (BMP2) in BMSC and recently developed and characterized, biodegradable Poly(L-lactide-co-є-caprolactone){poly(LLA-co-CL)}scaffolds in osteogenic molecular changes and ectopic bone formation by using in vitro and in vivo approaches. Pathway-focused custom PCR array, validation using TaqMan based quantitative RT-PCR (qRT-PCR) and ALP staining showed significant up-regulation of several osteogenic and angiogenic molecules, including ALPL and RUNX2 in ad-BMP2 BMSC group grown in poly(LLA-co-CL) scaffolds both at 3 and 14 days. Micro CT and histological analyses of the subcutaneously implanted scaffolds in NOD/SCID mice revealed significantly increased radiopaque areas, percentage bone volume and formation of vital bone in ad-BMP2 scaffolds as compared to the control groups both at 2 and 8 weeks. The increased bone formation in the ad-BMP2 group in vivo was paralleled at the molecular level with concomitant over-expression of a number of osteogenic and angiogenic genes including ALPL, RUNX2, SPP1, ANGPT1. The increased bone formation in ad-BMP2 explants was not found to be associated with enhanced endochondral activity as evidenced by qRT-PCR (SOX9 and FGF2) and Safranin O staining. Taken together, combination of adenoviral mediated BMP-2 expression in BMSC grown in the newly developed poly(LLA-co-CL) scaffolds induced expression of osteogenic markers and enhanced bone formation in vivo.

Published

2016

6. Serum BAFF and APRIL Levels, T-Lymphocyte Subsets, and Immunoglobulins after B-Cell Depletion Using the Monoclonal Anti-CD20 Antibody Rituximab in Myalgic Encephalopathy/Chronic Fatigue Syndrome.

Author

Sigrid Lunde, Einar K Kristoffersen, Dipak Sapkota, Kristin Risa, Olav Dahl, Ove Bruland, Olav Mella, and Øystein Fluge

Subjects

Medicine, Science

Abstract

Myalgic Encephalopathy/Chronic Fatigue Syndrome (ME/CFS) is a disease of unknown etiology. We have previously suggested clinical benefit from B-cell depletion using the monoclonal anti-CD20 antibody rituximab in a randomized and placebo-controlled study. Prolonged responses were then demonstrated in an open-label phase-II study with maintenance rituximab treatment. Using blood samples from patients in the previous two clinical trials, we investigated quantitative changes in T-lymphocyte subsets, in immunoglobulins, and in serum levels of two B-cell regulating cytokines during follow-up. B-lymphocyte activating factor of the tumor necrosis family (BAFF) in baseline serum samples was elevated in 70 ME/CFS patients as compared to 56 healthy controls (p = 0.011). There were no significant differences in baseline serum BAFF levels between patients with mild, moderate, or severe ME/CFS, or between responders and non-responders to rituximab. A proliferation-inducing ligand (APRIL) serum levels were not significantly different in ME/CFS patients compared to healthy controls at baseline, and no changes in serum levels were seen during follow-up. Immunophenotyping of peripheral blood T-lymphocyte subsets and T-cell activation markers at multiple time points during follow-up showed no significant differences over time, between rituximab and placebo groups, or between responders and non-responders to rituximab. Baseline serum IgG levels were significantly lower in patients with subsequent response after rituximab therapy compared to non-responders (p = 0.03). In the maintenance study, slight but significant reductions in mean serum immunoglobulin levels were observed at 24 months compared to baseline; IgG 10.6-9.5 g/L, IgA 1.8-1.5 g/L, and IgM 0.97-0.70 g/L. Although no functional assays were performed, the lack of significant associations of T- and NK-cell subset numbers with B-cell depletion, as well as the lack of associations to clinical responses, suggest that B-cell regulatory effects on T-cell or NK-cell subsets are not the main mechanisms for the observed improvements in ME/CFS symptoms observed in the two previous trials. The modest increase in serum BAFF levels at baseline may indicate an activated B-lymphocyte system in a subgroup of ME/CFS patients.

Published

2016

7. B-Lymphocyte Depletion in Myalgic Encephalopathy/ Chronic Fatigue Syndrome. An Open-Label Phase II Study with Rituximab Maintenance Treatment.

Author

Øystein Fluge, Kristin Risa, Sigrid Lunde, Kine Alme, Ingrid Gurvin Rekeland, Dipak Sapkota, Einar Kleboe Kristoffersen, Kari Sørland, Ove Bruland, Olav Dahl, and Olav Mella

Subjects

Medicine, Science

Abstract

Myalgic Encephalopathy/Chronic Fatigue Syndrome (ME/CFS) is a disease of unknown etiology. We previously reported a pilot case series followed by a small, randomized, placebo-controlled phase II study, suggesting that B-cell depletion using the monoclonal anti-CD20 antibody rituximab can yield clinical benefit in ME/CFS.In this single-center, open-label, one-armed phase II study (NCT01156909), 29 patients were included for treatment with rituximab (500 mg/m2) two infusions two weeks apart, followed by maintenance rituximab infusions after 3, 6, 10 and 15 months, and with follow-up for 36 months.Major or moderate responses, predefined as lasting improvements in self-reported Fatigue score, were detected in 18 out of 29 patients (intention to treat). Clinically significant responses were seen in 18 out of 28 patients (64%) receiving rituximab maintenance treatment. For these 18 patients, the mean response durations within the 156 weeks study period were 105 weeks in 14 major responders, and 69 weeks in four moderate responders. At end of follow-up (36 months), 11 out of 18 responding patients were still in ongoing clinical remission. For major responders, the mean lag time from first rituximab infusion until start of clinical response was 23 weeks (range 8-66). Among the nine patients from the placebo group in the previous randomized study with no significant improvement during 12 months follow-up after saline infusions, six achieved a clinical response before 12 months after rituximab maintenance infusions in the present study. Two patients had an allergic reaction to rituximab and two had an episode of uncomplicated late-onset neutropenia. Eight patients experienced one or more transient symptom flares after rituximab infusions. There was no unexpected toxicity.In a subgroup of ME/CFS patients, prolonged B-cell depletion with rituximab maintenance infusions was associated with sustained clinical responses. The observed patterns of delayed responses and relapse after B-cell depletion and regeneration, a three times higher disease prevalence in women than in men, and a previously demonstrated increase in B-cell lymphoma risk for elderly ME/CFS patients, suggest that ME/CFS may be a variant of an autoimmune disease.ClinicalTrials.gov NCT01156909.

Published

2015

8. One-tube restriction enzyme digest and fluorescent labeling for restriction endonuclease fingerprinting single-strand conformational polymorphism

Author

Ove Bruland and Per Morten Knappskog

Subjects

Biology (General), QH301-705.5

Published

2004

9. S100A14 interacts with S100A16 and regulates its expression in human cancer cells.

Author

Dipak Sapkota, Daniela Elena Costea, Salah O Ibrahim, Anne C Johannessen, and Ove Bruland

Subjects

Medicine, Science

Abstract

Both S100A14 and S100A16 are members of the multifunctional S100 protein family. Formation of homo/heterodimers is considered to be one of the major mechanisms for S100 proteins to execute their diverse cellular functions. By employing a classical Yeast two hybrid (Y-2 H) screen, we identified S100A16 as the single interaction partner of S100A14. This interaction was verified by co-immunoprecipitation, double indirect immunofluorescence and double immunostaining in specimens of oral squamous cell carcinoma and normal oral mucosa. The functional significance of this interaction was examined by employing retroviral mediated over-expression and knock-down of these proteins in several cancer cell-lines. Over-expression and knock-down of S100A14 led to concomitant up- and down-regulation of S100A16 protein in the cell-lines examined. However, there was no up-regulation of S100A16 mRNA upon S100A14 over-expression, indicating that modulation of S100A16 expression was not due to enhanced transcriptional activity but possibly by post-transcriptional regulation. In contrary, over-expression of S100A16 was associated neither with the up-regulation of S100A14 mRNA nor its protein, suggesting a unidirectional regulation between S100A14 and S100A16. Cellular treatment with protein synthesis inhibitor cycloheximide demonstrated a time-dependent intracellular degradation of both S100A16 and S100A14 proteins. Additionally, regulation of S100A16 and S100A14 degradation was found to be independent of the classical proteasomal and lysosomal pathways of protein degradation. Further studies will therefore be necessary to understand the functional significance of this interaction and the mechanisms on how S100A14 is involved in the regulation of S100A16 expression.

Published

2013

10. Benefit from B-lymphocyte depletion using the anti-CD20 antibody rituximab in chronic fatigue syndrome. A double-blind and placebo-controlled study.

Author

Øystein Fluge, Ove Bruland, Kristin Risa, Anette Storstein, Einar K Kristoffersen, Dipak Sapkota, Halvor Næss, Olav Dahl, Harald Nyland, and Olav Mella

Subjects

Medicine, Science

Abstract

Chronic fatigue syndrome (CFS) is a disease of unknown aetiology. Major CFS symptom relief during cancer chemotherapy in a patient with synchronous CFS and lymphoma spurred a pilot study of B-lymphocyte depletion using the anti-CD20 antibody Rituximab, which demonstrated significant clinical response in three CFS patients.In this double-blind, placebo-controlled phase II study (NCT00848692), 30 CFS patients were randomised to either Rituximab 500 mg/m(2) or saline, given twice two weeks apart, with follow-up for 12 months. Xenotropic murine leukemia virus-related virus (XMRV) was not detected in any of the patients. The responses generally affected all CFS symptoms. Major or moderate overall response, defined as lasting improvements in self-reported Fatigue score during follow-up, was seen in 10 out of 15 patients (67%) in the Rituximab group and in two out of 15 patients (13%) in the Placebo group (p = 0.003). Mean response duration within the follow-up period for the 10 responders to Rituximab was 25 weeks (range 8-44). Four Rituximab patients had clinical response durations past the study period. General linear models for repeated measures of Fatigue scores during follow-up showed a significant interaction between time and intervention group (p = 0.018 for self-reported, and p = 0.024 for physician-assessed), with differences between the Rituximab and Placebo groups between 6-10 months after intervention. The primary end-point, defined as effect on self-reported Fatigue score 3 months after intervention, was negative. There were no serious adverse events. Two patients in the Rituximab group with pre-existing psoriasis experienced moderate psoriasis worsening.The delayed responses starting from 2-7 months after Rituximab treatment, in spite of rapid B-cell depletion, suggests that CFS is an autoimmune disease and may be consistent with the gradual elimination of autoantibodies preceding clinical responses. The present findings will impact future research efforts in CFS.ClinicalTrials.gov NCT00848692.

Published

2011

11. Xeno-free generation of human induced pluripotent stem cells from donor-matched fibroblasts isolated from dermal and oral tissues

Author

Hassan R.W. Ali, Salwa Suliman, Tarig Al-Hadi Osman, Manuel Carrasco, Ove Bruland, Daniela-Elena Costea, Helge Ræder, and Kamal Mustafa

Abstract

Background Induced pluripotent stem cells (iPS) can be generated from various somatic cells and can subsequently be differentiated to multiple cell types of the body. This makes them highly promising for cellular therapy in regenerative medicine. However, to facilitate their clinical use and to ensure safety, iPS culturing protocols must be compliant with good manufacturing practice guidelines, and devoid of xenogenic products. Therefore, we aimed to compare the efficiency of using humanized culture conditions, specifically human platelet lysate to fetal bovine serum, for iPS generation from different sources, and to evaluate their stemness. Methods iPS were generated via a platelet lysate or fetal bovine serum-based culturing protocol from matched dermal, buccal, and gingival human fibroblasts, isolated from healthy donors (n=2) after informed consent, via episomal plasmid transfection. Pluripotency, genotype, and phenotype of iPS, generated by both protocols, was then assessed by various methods. Results More attempts were generally required to successfully reprogram xeno-free fibroblasts to iPS, as compared to xenogenic cultured fibroblasts. Furthermore, oral fibroblasts generally required more attempts for successful iPS generation as opposed to dermal fibroblasts. Morphologically, all iPS generated from fibroblasts formed tight colonies surrounded by a reflective "whitish" outer rim, typical for iPS. They also expressed pluripotency markers at both gene (SOX2, OCT4, NANOG) and protein level (SOX2, OCT4). Upon stimulation, all iPS showed ability to differentiate into the three primary germ layers via expression of lineage specific markers for mesoderm (MESP1, OSR1, HOPX), endoderm (GATA4), and ectoderm (PAX6, RAX). Genome analysis revealed several amplifications and deletions within the chromosomes of each iPS cell line. Conclusions The xeno-free protocol had a lower reprogramming efficiency compared to the standard xenogenic protocol. The oral fibroblasts generally proved to be more difficult to reprogram than dermal fibroblasts. Xeno-free dermal, buccal, and gingival fibroblasts can successfully generate iPS with a comparable geno/phenotype to their xenogenic counterparts.

Published

2023

12. A Pellino-2 variant is associated with constitutive NLRP3 inflammasome activation in a family with ocular pterygium–digital keloid dysplasia

Author

Ileana Cristea, Hugo Abarca, Anne E. Christensen Mellgren, Milana Trubnykova, Roya Mehrasa, Dorien J. M. Peters, Gunnar Houge, Raoul C. M. Hennekam, Eyvind Rødahl, Ove Bruland, Cecilie Bredrup, General Paediatrics, and APH - Quality of Care

Subjects

PELI2, Structural Biology, Genetics, Biophysics, corneal vascularization, Cell Biology, pterygium, Molecular Biology, Biochemistry, NLRP3 inflammasome, keloids, OPDKD

Abstract

Ocular pterygium–digital keloid dysplasia (OPDKD) is a rare hereditary disease characterized by corneal ingrowth of vascularized conjunctival tissue early in life. Later, patients develop keloids on fingers and toes but are otherwise healthy. In a recently described family with OPDKD, we report the presence of a de novo c.770C > T, p.(Thr257Ile) variant in PELI2 in the affected individual. PELI2 encodes for the E3 ubiquitin ligase Pellino-2. In transgenic U87MG cells overexpressing Pellino-2 with the p.(Thr257Ile) amino acid substitution, constitutive activation of the NLRP3 inflammasome was observed. However, the Thr257Ile variant did not affect Pellino-2 intracellular localization, its binding to known interaction partners, nor its stability. Our findings indicate that constitutive autoactivation of the NLRP3 inflammasome contributes to the development of PELI2-associated OPDKD.

Published

2023

13. Pellino‐2 in nonimmune cells: novel interaction partners and intracellular localization

Author

Ove Bruland, Ingvild Aukrust, Ileana M. Cristea, Cecilie Bredrup, and Eyvind Rødahl

Subjects

Nigericin, Ubiquitin-Protein Ligases, Active Transport, Cell Nucleus, Biophysics, Biochemistry, chemistry.chemical_compound, Structural Biology, Two-Hybrid System Techniques, Genetics, medicine, Humans, Protein Interaction Maps, Molecular Biology, Cells, Cultured, Cell Nucleus, Innate immune system, biology, Chemistry, Kinase, Nuclear Proteins, Potassium channel blocker, Cell Biology, Fibroblasts, Cell biology, Ubiquitin ligase, HEK293 Cells, biology.protein, Tumor necrosis factor alpha, Nuclear localization sequence, Intracellular, Protein Binding, medicine.drug

Abstract

Pellino-2 is an E3 ubiquitin ligase that mediates intracellular signaling in innate immune pathways. Most studies of endogenous Pellino-2 have been performed in macrophages, but none in nonimmune cells. Using yeast two-hybrid screening and co-immunoprecipitation, we identified six novel interaction partners of Pellino-2, with various localizations: insulin receptor substrate 1, NIMA-related kinase 9, tumor necrosis factor receptor-associated factor 7, cyclin-F, roundabout homolog 1, and disheveled homolog 2. Pellino-2 showed cytoplasmic localization in a wide range of nonimmune cells under physiological potassium concentrations. Treatment with the potassium ionophore nigericin resulted in nuclear localization of Pellino-2, which was reversed by the potassium channel blocker tetraethylammonium. Live-cell imaging revealed intracellular migration of GFP-tagged Pellino-2. In summary, Pellino-2 interacts with proteins at different cellular locations, taking part in dynamic processes that change its intracellular localization influenced by potassium efflux. publishedVersion

Published

2021

14. K + regulates relocation of Pellino‐2 to the site of NLRP3 inflammasome activation in macrophages

Author

Ove Bruland, Cecilie Bredrup, Ileana M. Cristea, and Eyvind Rødahl

Subjects

Innate immune system, biology, Chemistry, Potassium, Biophysics, chemistry.chemical_element, Colocalization, Inflammasome, Cell Biology, Biochemistry, Potassium channel, Cell biology, Ubiquitin, Structural Biology, Genetics, biology.protein, medicine, Efflux, NLRP3 inflammasome activation, Molecular Biology, medicine.drug

Abstract

Pellino proteins are E3 ubiquitin ligases involved in the innate immune system. Recently, Pellino-2 was reported to modulate the activation of the mouse Nlrp3 inflammasome. We examined the intracellular localization of human Pellino-2 in THP1-derived macrophages during activation with LPS and ATP. We observed that Pellino-2 changed intracellular localization and colocalized with the inflammasome proteins NLRP3 and ASC late in the assembly of the inflammasome. Colocalization with NLRP3 and ASC was also seen in cells maintained in potassium-free medium. The colocalization and inflammasome activation were abrogated by several potassium channel inhibitors, supporting a role for potassium efflux in modulating intracellular localization of Pellino-2. The data suggest that Pellino-2 is essential for mediating the effect of potassium efflux on inflammasome activation. publishedVersion

Published

2021

15. The SH3PXD2A-HTRA1 fusion transcript is extremely rare in Norwegian sporadic vestibular schwannoma patients

Author

Peter Taule-Sivertsen, Per M. Knappskog, Ove Bruland, Eirik Bratland, Morten Lund-Johansen, and Aril Løge Håvik

Subjects

0301 basic medicine, Cancer Research, Oncogene Proteins, Fusion, Tumor suppressor gene, Neurosurgery, Biology, Schwannoma, medicine.disease_cause, Fusion gene, Gene product, 03 medical and health sciences, Vestibular schwannoma, 0302 clinical medicine, Genetics, medicine, Humans, Gene, Norway, Driver mutation, High-Temperature Requirement A Serine Peptidase 1, Neuroma, Acoustic, medicine.disease, Adaptor Proteins, Vesicular Transport, 030104 developmental biology, Neurology, Oncology, Fusion transcript, Tumorigenesis, HTRA1, Laboratory Investigation, Cancer research, Neurology (clinical), Carcinogenesis, Gene fusion, 030217 neurology & neurosurgery

Abstract

Introduction Vestibular schwannoma (VS) is a benign intracranial tumor in which the underlying genetics is largely uncertain, apart from mutations in the tumor suppressor gene NF2. Alternative tumorigenic mechanisms have been proposed, including a recurrent in-frame fusion transcript of the HTRA1 and SH3PXD2A genes. The gene product of the SH3PXD2A-HTRA1 fusion has been shown to promote proliferation, invasion and resistance to cell death in vitro and tumor growth in vivo. The aim of this study was to replicate the findings and to investigate the frequency of this fusion gene in another cohort of vestibular schwannoma patients. Methods The SH3PXD2A-HTRA1 transcript was synthesized in vitro using PCR and used as a positive control to assess the sensitivity of a real-time PCR assay. This real-time PCR assay was used to search for the presence of the fusion transcript in 121 Norwegian sporadic VS patients. Results The real-time PCR assay showed a high sensitivity and was able to detect as low as ~ 5 copies of the fusion transcript. Out of the 121 investigated tumors, only 1 harbored the SH3PXD2A-HTRA1 fusion. Conclusion Even though the SH3PXD2A-HTRA1 fusion has been shown to be a driver of tumorigenesis, our results suggest that it is a rare event in our VS patients. Further investigation is warranted in order to elucidate whether our results represent an extreme, and if the fusion is present also in other neoplasms.

Published

2021

16. K

Author

Ileana, Cristea, Ove, Bruland, Eyvind, Rødahl, and Cecilie, Bredrup

Subjects

Protein Transport, Inflammasomes, NLR Family, Pyrin Domain-Containing 3 Protein, Potassium, Humans, Macrophage Activation, Cell Line

Abstract

Pellino proteins are E3 ubiquitin ligases involved in the innate immune system. Recently, Pellino-2 was reported to modulate the activation of the mouse Nlrp3 inflammasome. We examined the intracellular localization of human Pellino-2 in THP1-derived macrophages during activation with LPS and ATP. We observed that Pellino-2 changed intracellular localization and colocalized with the inflammasome proteins NLRP3 and ASC late in the assembly of the inflammasome. Colocalization with NLRP3 and ASC was also seen in cells maintained in potassium-free medium. The colocalization and inflammasome activation were abrogated by several potassium channel inhibitors, supporting a role for potassium efflux in modulating intracellular localization of Pellino-2. The data suggest that Pellino-2 is essential for mediating the effect of potassium efflux on inflammasome activation.

Published

2021

17. Temperature-dependent autoactivation associated with clinical variability of PDGFRB Asn666 substitutions

Author

Deepak P. Edward, Kåre Steinar Tveit, Olav H. Haugen, Leen Abu Safieh, Frode Thu, Cecilie Bredrup, Raoul C.M. Hennekam, Eyvind Rødahl, Bjørn Tore Gjertsen, Ove Bruland, Gunnar Houge, Gunnar Høvding, Nils Bull, Emilio Di Maria, Ileana M. Cristea, General Paediatrics, and APH - Quality of Care

Subjects

0301 basic medicine, AcademicSubjects/SCI01140, Adult, Male, Adolescent, Limb Deformities, Congenital, Mutation, Missense, Connective tissue, PDGFRB, Biology, Pterygium, Receptor, Platelet-Derived Growth Factor beta, 03 medical and health sciences, Young Adult, 0302 clinical medicine, Keloid, Progeria, Genetics, medicine, Humans, STAT1, Phosphorylation, Child, Molecular Biology, Genetics (clinical), Acro-Osteolysis, Temperature, Infant, General Medicine, medicine.disease, Resorption, Tissue Degeneration, 030104 developmental biology, medicine.anatomical_structure, Phenotype, Amino Acid Substitution, Dysplasia, Child, Preschool, Cancer research, biology.protein, Skin Abnormalities, Female, General Article, Conjunctiva, 030217 neurology & neurosurgery

Abstract

Ocular pterygium-digital keloid dysplasia (OPDKD) presents in childhood with ingrowth of vascularized connective tissue on the cornea leading to severely reduced vision. Later the patients develop keloids on digits but are otherwise healthy. The overgrowth in OPDKD affects body parts that typically have lower temperature than 37°C. We present evidence that OPDKD is associated with a temperature sensitive, activating substitution, p.(Asn666Tyr), in PDGFRB. Phosphorylation levels of PDGFRB and downstream targets were higher in OPDKD fibroblasts at 37°C but were further greatly increased at the average corneal temperature of 32°C. This suggests that the substitution cause significant constitutive autoactivation mainly at lower temperature. In contrast, a different substitution in the same codon, p.(Asn666Ser), is associated with Penttinen type of premature aging syndrome. This devastating condition is characterized by widespread tissue degeneration, including pronounced chronic ulcers and osteolytic resorption in distal limbs. In Penttinen syndrome fibroblasts, equal and high levels of phosphorylated PDGFRB was present at both 32°C and 37°C. This indicates that this substitution causes severe constitutive autoactivation of PDGFRB regardless of temperature. In line with this, most downstream targets were not affected by lower temperature. However, STAT1, important for tissue wasting, did show further increased phosphorylation at 32°C. Temperature-dependent autoactivation offers an explanation to the strikingly different clinical outcomes of substitutions in the Asn666 codon of PDGFRB.

Published

2021

18. Gamma Knife Radiosurgery does not alter the copy number aberration profile in sporadic vestibular schwannoma

Author

Aril Løge Håvik, Per-Morten Knappskog, Morten Lund-Johansen, Ove Bruland, and Dhanushan Dhayalan

Subjects

Adult, Male, Oncology, Cancer Research, medicine.medical_specialty, DNA Copy Number Variations, Microarray, Neurosurgery, Gamma knife radiosurgery, Schwannoma, Radiosurgery, medicine.disease_cause, Malignancy, Vestibular schwannoma, Internal medicine, Genetics, Humans, Medicine, Aged, Aged, 80 and over, Vestibular system, Whole Genome Sequencing, business.industry, Radiotherapy Dosage, Neuroma, Acoustic, Intratumor genetic heterogeneity, Middle Aged, Prognosis, medicine.disease, Tumor Burden, Gamma Knife Radiosurgery, Neurology, Laboratory Investigation, Female, Neurology (clinical), Whole genome microarray, business, Carcinogenesis, Chromosome 22, Follow-Up Studies

Abstract

Introduction Ionizing radiation is a known etiologic factor in tumorigenesis and its role in inducing malignancy in the treatment of vestibular schwannoma has been debated. The purpose of this study was to identify a copy number aberration (CNA) profile or specific CNAs associated with radiation exposure which could either implicate an increased risk of malignancy or elucidate a mechanism of treatment resistance. Methods 55 sporadic VS, including 18 treated with Gamma Knife Radiosurgery (GKRS), were subjected to DNA whole-genome microarray and/or whole-exome sequencing. CNAs were called and statistical tests were performed to identify any association with radiation exposure. Hierarchical clustering was used to identify CNA profiles associated with radiation exposure. Results A median of 7 (0–58) CNAs were identified across the 55 VS. Chromosome 22 aberration was the only recurrent event. A median aberrant cell fraction of 0.59 (0.25–0.94) was observed, indicating several genetic clones in VS. No CNA or CNA profile was associated with GKRS. Conclusion GKRS is not associated with an increase in CNAs or alteration of the CNA profile in VS, lending support to its low risk. This also implies that there is no major issue with GKRS treatment failure being due to CNAs. In agreement with previous studies, chromosome 22 aberration is the only recurrent CNA. VS consist of several genetic clones, addressing the need for further studies on the composition of cells in this tumor.

Published

2020

19. A tyrosine kinase-activating variant Asn666Ser in PDGFRB causes a progeria-like condition in the severe end of Penttinen syndrome

Author

Tomasz Stokowy, Kåre Steinar Tveit, Gunnar Houge, Ove Bruland, Linda Xu, Dipak Sapkota, Vidar M. Steen, Eyvind Rødahl, Gunnar Høvding, Julie McGaughran, Ileana M. Cristea, Samuel Lee, and Cecilie Bredrup

Subjects

Adult, Male, 0301 basic medicine, Aging, Limb Deformities, Congenital, Mutation, Missense, Apoptosis, Protein Tyrosine Phosphatase, Non-Receptor Type 11, PDGFRB, Protein tyrosine phosphatase, Article, Receptor, Platelet-Derived Growth Factor beta, 03 medical and health sciences, Progeria, 0302 clinical medicine, Genetics, medicine, Humans, Genetic Predisposition to Disease, Protein Interaction Maps, Phosphorylation, Cockayne Syndrome, Protein kinase B, Genetics (clinical), Mitogen-Activated Protein Kinase 3, Acro-Osteolysis, biology, Chemistry, Autophosphorylation, Myofibromatosis, Protein-Tyrosine Kinases, medicine.disease, Phenotype, 030104 developmental biology, 030220 oncology & carcinogenesis, Imatinib Mesylate, biology.protein, Cancer research, Female, Tyrosine kinase, Platelet-derived growth factor receptor, HeLa Cells, Signal Transduction

Abstract

Missense variants located to the “molecular brake” in the tyrosine kinase hinge region of platelet-derived growth factor receptor-β, encoded by PFGFRB, can cause Penttinen-type (Val665Ala) and Penttinen-like (Asn666His) premature ageing syndromes, as well as infantile myofibromatosis (Asn666Lys and Pro660Thr). We have found the same de novo PDGFRB c.1997A>G p.(Asn666Ser) variants in two patients with lipodystrophy, acro-osteolysis and severely reduced vision due to corneal neovascularisation, reminiscent of a severe form of Penttinen syndrome with more pronounced connective tissue destruction. In line with this phenotype, patient skin fibroblasts were prone to apoptosis. Both in patient fibroblasts and stably transduced HeLa and HEK293 cells, autophosphorylation of PDGFRβ was observed, as well as increased phosphorylation of downstream signalling proteins such as STAT1, PLCγ1, PTPN11/SHP2-Tyr580 and AKT. Phosphorylation of MAPK3 (ERK1) and PTPN11/SHP2-Tyr542 appeared unaffected. This suggests that this missense change not only weakens tyrosine kinase autoinhibition, but also influences substrate binding, as both PTPN11 tyrosines (Tyr542 and Tyr580) usually are phosphorylated upon PDGFR activation. Imatinib was a strong inhibitor of phosphorylation of all these targets, suggesting an option for precision medicine based treatment.

Published

2018

20. Activating mutations in discoidin domain receptor 2 cause Warburg‐Cinotti syndrome

Author

Linda Zi Yan Xu, Katja Kloth, Leslie G. Biesecker, Elisa Cinotti, Thomas N. Darling, Ove Bruland, Gunnar Houge, Emilio Di Maria, Christian Kubisch, Hanne Jensen, Jennifer J. Johnston, Laryssa A. Huryn, Lisbeth Tranebjærg, Julie C. Sapp, Ileana M. Cristea, Eyvind Rødahl, and Cecilie Bredrup

Subjects

Ophthalmology, Chemistry, General Medicine, Receptor, Discoidin domain, Cell biology

Published

2019

21. Upregulated PDK4 expression is a sensitive marker of increased fatty acid oxidation

Author

Linn I. Hodneland, Nils Gunnar Løvsletten, Rolf K. Berge, Kjetil Berge, Nils Halberg, Ina Katrine Nitschke Pettersen, Hege Wergedahl, Bodil Bjørndal, Lena Hansen, Xiao-Zheng Liu, Ove Bruland, Gro V. Røsland, Øystein Fluge, Sissel E. Dyrstad, Arild C. Rustan, Hanan Ashrafi, Deusdedit Tusubira, and Karl Johan Tronstad

Subjects

Male, 0301 basic medicine, Mitochondrion, peroxisome proliferator-activated receptor (ppar), metabolic flexibility, chemistry.chemical_compound, 0302 clinical medicine, Metabolic flexibility, cell metabolism, Glycolysis, Beta oxidation, fatty acid oxidation, chemistry.chemical_classification, Fatty Acids, Tetradecylthioacetic acid, Peroxisome, Up-Regulation, Mitochondria, mitochondria, Biochemistry, Organ Specificity, Fatty acid oxidation, Pyruvate dehydrogenase kinase, biomarker, Molecular Medicine, Oxidation-Reduction, VDP::Matematikk og Naturvitenskap: 400::Basale biofag: 470::Cellebiologi: 471, PDK4, Sulfides, Gene Expression Regulation, Enzymologic, Mitochondrial Proteins, 03 medical and health sciences, pyruvate dehydrogenase kinase, Metabolic regulation, Animals, Humans, Rats, Wistar, Molecular Biology, Cell metabolism, Pyruvate Dehydrogenase Acetyl-Transferring Kinase, Fatty acid, Cell Biology, Biomarker, Rats, 030104 developmental biology, chemistry, Mitochondrial biogenesis, Peroxisome proliferator-activated receptor (PPAR), metabolic regulation, Biomarkers, 030217 neurology & neurosurgery, HeLa Cells

Abstract

Fatty acid oxidation is a central fueling pathway for mitochondrial ATP production. Regulation occurs through multiple nutrient- and energy-sensitive molecular mechanisms. We explored if upregulated mRNA expression of the mitochondrial enzyme pyruvate dehydrogenase kinase 4 (PDK4) may be used as a surrogate marker of increased mitochondrial fatty acid oxidation, by indicating an overall shift from glucose to fatty acids as the preferred oxidation fuel. The association between fatty acid oxidation and PDK4 expression was studied in different contexts of metabolic adaption. In rats treated with the modified fatty acid tetradecylthioacetic acid (TTA), Pdk4 was upregulated simultaneously with fatty acid oxidation genes in liver and heart, whereas muscle and white adipose tissue remained unaffected. In MDA-MB-231 cells, fatty acid oxidation increased nearly threefold upon peroxisome proliferator-activated receptor α (PPARα, PPARA) overexpression, and four-fold upon TTA-treatment. PDK4 expression was highly increased under these conditions. Further, overexpression of PDK4 caused increased fatty acid oxidation in these cells. Pharmacological activators of PPARα and AMPK had minor effects, while the mTOR inhibitor rapamycin potentiated the effect of TTA. There were minor changes in mitochondrial respiration, glycolytic function, and mitochondrial biogenesis under conditions of increased fatty acid oxidation. TTA was found to act as a mild uncoupler, which is likely to contribute to the metabolic effects. Repeated experiments with HeLa cells supported these findings. In summary, PDK4 upregulation implies an overarching metabolic shift towards increased utilization of fatty acids as energy fuel, and thus constitutes a sensitive marker of enhanced fatty acid oxidation. publishedVersion

Published

2019

22. Recurrent, Activating Variants in the Receptor Tyrosine Kinase DDR2 Cause Warburg-Cinotti Syndrome

Author

Hanne Jensen, Christian Kubisch, Eyvind Rødahl, Lisbeth Tranebjærg, Leslie G. Biesecker, Katja Kloth, Thomas N. Darling, Linda Xu, Laryssa A. Huryn, Julie C. Sapp, Elisa Cinotti, Cecilie Bredrup, Jennifer J. Johnston, Ileana M. Cristea, Ove Bruland, Gunnar Houge, and Emilio Di Maria

Subjects

Adult, 0301 basic medicine, chronic skin ulcers, lipodystrophy, medicine.drug_class, acro-osteolysis, keloid formation, Biology, contractures, corneal neovascularization, DDR2, Genetics, Genetics (clinical), Receptor tyrosine kinase, 03 medical and health sciences, Discoidin Domain Receptor 2, 0302 clinical medicine, Report, medicine, Humans, Amino Acid Sequence, Preschool, Child, Connective Tissue Diseases, Receptor, Protein Kinase Inhibitors, Kinase, Autophosphorylation, Receptor Protein-Tyrosine Kinases, Fibroblasts, Middle Aged, Protein kinase inhibitor, Child, Preschool, Collagen, Female, Sequence Alignment, Signal Transduction, Dasatinib, 030104 developmental biology, 030220 oncology & carcinogenesis, Cancer research, biology.protein, Phosphorylation, Discoidin domain, medicine.drug

Abstract

We have investigated a distinct disorder with progressive corneal neovascularization, keloid formation, chronic skin ulcers, wasting of subcutaneous tissue, flexion contractures of the fingers, and acro-osteolysis. In six affected individuals from four families, we found one of two recurrent variants in discoidin domain receptor tyrosine kinase 2 (DDR2): c.1829T>C (p.Leu610Pro) or c.2219A>G (p.Tyr740Cys). DDR2 encodes a collagen-responsive receptor tyrosine kinase that regulates connective-tissue formation. In three of the families, affected individuals comprise singleton adult individuals, and parental samples were not available for verification of the de novo occurrence of the DDR2 variants. In the fourth family, a mother and two of her children were affected, and the c.2219A>G missense variant was proven to be de novo in the mother. Phosphorylation of DDR2 was increased in fibroblasts from affected individuals, suggesting reduced receptor autoinhibition and ligand-independent kinase activation. Evidence for activation of other growth-regulatory signaling pathways was not found. Finally, we found that the protein kinase inhibitor dasatinib prevented DDR2 autophosphorylation in fibroblasts, suggesting an approach to treatment. We propose this progressive, fibrotic condition should be designated as Warburg-Cinotti syndrome.

Published

2018

23. B-Lymphocyte Depletion in Patients With Myalgic Encephalomyelitis/Chronic Fatigue Syndrome

Author

Solvang Ah, Merethe Eide Gotaas, Kine Alme, Ingrid Herder, Katarina Lien, Kristin Risa, Lonar Ae, Kari Sørland, Kvammen Ø, Martinsen Ss, Bohnen Lmlj, Gya Aes, Christoph Schäfer, Hanne Thürmer, Olav Mella, Irini Ktoridou-Valen, Ove Bruland, Jörg Aßmus, Katarzyna A. Baranowska, Olav Dahl, Ingrid Gurvin Rekeland, Petter C. Borchgrevink, and Øystein Fluge

Subjects

Adult, Male, medicine.medical_specialty, Placebo-controlled study, Placebo, Severity of Illness Index, 01 natural sciences, Lymphocyte Depletion, 03 medical and health sciences, Antineoplastic Agents, Immunological, 0302 clinical medicine, Double-Blind Method, Multicenter trial, Internal medicine, Severity of illness, Internal Medicine, Chronic fatigue syndrome, medicine, Humans, 030212 general & internal medicine, 0101 mathematics, Infusions, Intravenous, B-Lymphocytes, Fatigue Syndrome, Chronic, business.industry, Surrogate endpoint, 010102 general mathematics, Repeated measures design, General Medicine, medicine.disease, Female, Rituximab, business, medicine.drug

Abstract

Background Previous phase 2 trials indicated benefit from B-lymphocyte depletion in myalgic encephalomyelitis/chronic fatigue syndrome (ME/CFS). Objective To evaluate the effect of the monoclonal anti-CD20 antibody rituximab versus placebo in patients with ME/CFS. Design Randomized, placebo-controlled, double-blind, multicenter trial. (ClinicalTrials.gov: NCT02229942). Setting 4 university hospitals and 1 general hospital in Norway. Patients 151 patients aged 18 to 65 years who had ME/CFS according to Canadian consensus criteria and had had the disease for 2 to 15 years. Intervention Treatment induction with 2 infusions of rituximab, 500 mg/m2 of body surface area, 2 weeks apart, followed by 4 maintenance infusions with a fixed dose of 500 mg at 3, 6, 9, and 12 months (n = 77), or placebo (n = 74). Measurements Primary outcomes were overall response rate (fatigue score ≥4.5 for ≥8 consecutive weeks) and repeated measurements of fatigue score over 24 months. Secondary outcomes included repeated measurements of self-reported function over 24 months, components of the Short Form-36 Health Survey and Fatigue Severity Scale over 24 months, and changes from baseline to 18 months in these measures and physical activity level. Between-group differences in outcome measures over time were assessed by general linear models for repeated measures. Results Overall response rates were 35.1% in the placebo group and 26.0% in the rituximab group (difference, 9.2 percentage points [95% CI, -5.5 to 23.3 percentage points]; P = 0.22). The treatment groups did not differ in fatigue score over 24 months (difference in average score, 0.02 [CI, -0.27 to 0.31]; P = 0.80) or any of the secondary end points. Twenty patients (26.0%) in the rituximab group and 14 (18.9%) in the placebo group had serious adverse events. Limitation Self-reported primary outcome measures and possible recall bias. Conclusion B-cell depletion using several infusions of rituximab over 12 months was not associated with clinical improvement in patients with ME/CFS. Primary Funding Source The Norwegian Research Council, Norwegian Regional Health Trusts, Kavli Trust, MEandYou Foundation, and Norwegian ME Association.

Published

2019

24. Expression of DSG1 and DSC1 are prognostic markers in anal carcinoma patients

Author

Olav Dahl, A. Skarstein, Heike Immervoll, Mette Pernille Myklebust, Ove Bruland, Øystein Fluge, and Lise Balteskard

Subjects

Male, Cancer Research, Pathology, medicine.medical_specialty, Anal Carcinoma, Mitomycin, Biology, Disease-Free Survival, DSG1, DSC1, Carcinoma, medicine, Humans, Molecular Diagnostics, Lymph node, Aged, anal carcinoma and survival, Desmocollins, Univariate analysis, Cadherin, Desmoglein 1, E-cadherin, Anal Region, Middle Aged, Anus Neoplasms, Cadherins, Prognosis, medicine.disease, Combined Modality Therapy, Staining, medicine.anatomical_structure, Oncology, Carcinoma, Squamous Cell, Immunohistochemistry, Female, Fluorouracil

Abstract

Background: Our purpose was to investigate if dysregulation of cell adhesion molecules could be linked to prognosis in squamous cell carcinomas (SCCs) of the anal region. Methods: Protein expression of desmoglein-1 (DSG1), desmocollin-1 (DSC1) and E-cadherin was studied by immunohistochemistry in a cohort of 53 anal carcinoma patients treated by radiation alone or combined with 5-fluorouracil and mitomycin C. Results: Univariate analyses identified, among others, negative membranous DSG1 staining (P=0.009), negative cytoplasmic DSC1 staining (P=0.012) and negative DSG1 (membranous)+negative DSC1 (cytoplasmic) staining (P=0.004) to be associated with improved cancer-specific survival (CSS). On multivariate analyses positive DSG1 (membranous)+DSC1 (cytoplasmic) staining (HR 6.95, P=0.044), large tumour size and lymph node metastases (HR 6.44, P=0.004) and radiation without chemotherapy (HR 6.73 P=0.004) were associated with worse CSS. On univariate analysis, improved disease-free survival was associated with negative membranous staining of DSG1 (P=0.047), and negative DSG1 (membranous)+negative DSC1 (cytoplasmic) staining (P=0.025), among others. Conclusion: Membrane negativity for DSG1 and cytoplasmic negativity for DSC1 are favourable markers for CSS in SCCs of the anal region.

Published

2012

25. Expression profile of the S100 gene family members in oral squamous cell carcinomas

Author

Osman A-Aziz Elgindi, Dipak Sapkota, Salah O. Ibrahim, Endre N. Vasstrand, Ove Bruland, Hala Bakeer, and Olav E. Bøe

Subjects

Cancer Research, Pathology, medicine.medical_specialty, Cancer, Biology, medicine.disease, medicine.disease_cause, Pathology and Forensic Medicine, S100A8, Pathogenesis, Reverse transcription polymerase chain reaction, stomatognathic diseases, Real-time polymerase chain reaction, Otorhinolaryngology, medicine, Cancer research, Periodontics, Gene family, Oral Surgery, Carcinogenesis, Gene

Abstract

Background: Several of the S100 gene members have been reported to be differentially expressed in many human pathological conditions, in particular, the malignancies. Identification and quantification of the differentially expressed S100 gene members in oral squamous cell carcinoma (OSCC) might facilitate their use as potential diagnostic and/or prognostic markers or targets for therapy. Methods: we examined the expression profile of 16 members of the S100 gene family at the mRNA level by semiquantitative reverse transcription-polymerase chain reaction (sRT-PCR) in 27 cases of OSCCs/their pair-wised normal controls obtained from Sudanese patients, and confirmed the sRT-PCR results by performing quantitative real time-polymerase chain reaction (qRT-PCR) for 6 of the 16 genes examined. Results: With sRT-PCR, 4 (25%; S100A4, S100A6, S100A8, S100A14) out of the 16 S100 gene members examined were found to be significantly down-regulated (P

Published

2008

26. Adenoviral Mediated Expression of BMP2 by Bone Marrow Stromal Cells Cultured in 3D Copolymer Scaffolds Enhances Bone Formation

Author

Kamal Mustafa, Yang Sun, Ove Bruland, Anna Finne-Wistrand, Ying Xue, Dipak Sapkota, and Sunita Sharma

Subjects

0301 basic medicine, Pathology, Polymers, Physiology, Organogenesis, lcsh:Medicine, Bone Morphogenetic Protein 2, Gene Expression, Artificial Gene Amplification and Extension, 02 engineering and technology, Mice, SCID, Ossification, Cardiovascular Physiology, Polymerase Chain Reaction, Mice, Endocrinology, Mice, Inbred NOD, Teknik och teknologier, Medicine and Health Sciences, lcsh:Science, Cells, Cultured, Staining, Multidisciplinary, ALPL, 021001 nanoscience & nanotechnology, medicine.anatomical_structure, Engineering and Technology, Bone Remodeling, medicine.symptom, 0210 nano-technology, Research Article, medicine.medical_specialty, Stromal cell, Genetic Vectors, Research and Analysis Methods, Bone morphogenetic protein 2, Adenoviridae, 03 medical and health sciences, Extraction techniques, In vivo, Growth Factors, medicine, Genetics, Animals, Humans, Molecular Biology Techniques, Endochondral ossification, Cytoplasmic Staining, Molecular Biology, Bone Development, Endocrine Physiology, lcsh:R, Mesenchymal stem cell, Biology and Life Sciences, Mesenchymal Stem Cells, Molecular biology, RNA extraction, 030104 developmental biology, HEK293 Cells, Specimen Preparation and Treatment, lcsh:Q, Safranin Staining, Bone marrow, Angiogenesis, Physiological Processes, Organism Development, Developmental Biology

Abstract

Selection of appropriate osteoinductive growth factors, suitable delivery method and proper supportive scaffold are critical for a successful outcome in bone tissue engineering using bone marrow stromal cells (BMSC). This study examined the molecular and functional effect of a combination of adenoviral mediated expression of bone morphogenetic protein-2 (BMP2) in BMSC and recently developed and characterized, biodegradable Poly(L-lactideco-epsilon-caprolactone){poly(LLA-co-CL)} scaffolds in osteogenic molecular changes and ectopic bone formation by using in vitro and in vivo approaches. Pathway-focused custom PCR array, validation using TaqMan based quantitative RT-PCR (qRT-PCR) and ALP staining showed significant up-regulation of several osteogenic and angiogenic molecules, including ALPL and RUNX2 in ad-BMP2 BMSC group grown in poly(LLA-co-CL) scaffolds both at 3 and 14 days. Micro CT and histological analyses of the subcutaneously implanted scaffolds in NOD/SCID mice revealed significantly increased radiopaque areas, percentage bone volume and formation of vital bone in ad-BMP2 scaffolds as compared to the control groups both at 2 and 8 weeks. The increased bone formation in the ad-BMP2 group in vivo was paralleled at the molecular level with concomitant over-expression of a number of osteogenic and angiogenic genes including ALPL, RUNX2, SPP1, ANGPT1. The increased bone formation in ad-BMP2 explants was not found to be associated with enhanced endochondral activity as evidenced by qRT-PCR (SOX9 and FGF2) and Safranin O staining. Taken together, combination of adenoviral mediated BMP-2 expression in BMSC grown in the newly developed poly(LLA-co-CL) scaffolds induced expression of osteogenic markers and enhanced bone formation in vivo. QC 20160319

Published

2015

27. S100A16 promotes differentiation and contributes to a less aggressive tumor phenotype in oral squamous cell carcinoma

Author

Muy-Teck Teh, Tarig Al-Hadi Osman, Himalaya Parajuli, Anne Christine Johannessen, Daniela Elena Costea, Ove Bruland, and Dipak Sapkota

Subjects

Adult, Male, Cancer Research, Pathology, medicine.medical_specialty, MMP1, Biopsy, Cellular differentiation, Genetic Vectors, Real-Time Polymerase Chain Reaction, medicine.disease_cause, Mice, Genetics, Animals, Humans, Medicine, Neoplasm Invasiveness, Aged, Cell Proliferation, Aged, 80 and over, Mouth neoplasm, business.industry, Cell growth, S100 Proteins, Mouth Mucosa, Middle Aged, stomatognathic diseases, Phenotype, Retroviridae, Real-time polymerase chain reaction, Oncology, Models, Animal, Carcinoma, Squamous Cell, Cancer research, Heterografts, Immunohistochemistry, Female, Mouth Neoplasms, Stem cell, business, Carcinogenesis, Research Article

Abstract

Background Altered expression of S100A16 has been reported in human cancers, but its biological role in tumorigenesis is not fully understood. This study aimed to investigate the clinical significance and functional role of S100A16 in oral squamous cell carcinoma (OSCC) suppression. Methods S100A16 mRNA and/or protein levels were examined by quantitative RT-PCR and immunohistochemistry in whole- and laser microdissected-specimens of normal human oral mucosa (NHOM, n = 65), oral dysplastic lesions (ODL, n = 21), OSCCs (n = 132) and positive cervical nodes (n = 17). S100A16 protein expression in OSCC was examined for correlations with clinicopathological variables and patient survival. S100A16 was over-expressed and knocked-down in OSCC-derived (CaLH3 and H357) cells by employing retroviral constructs to investigate its effects on cell proliferation, sphere formation and three dimensional (3D)-organotypic invasive abilities in vitro and tumorigenesis in a mouse xenograft model. Results Both S100A16 mRNA and protein levels were found to be progressively down-regulated from NHOM to ODL and OSCC. Low S100A16 protein levels in OSCC significantly correlated with reduced 10-year overall survival and poor tumor differentiation. Analysis of two external OSCC microarray datasets showed a positive correlation between the mRNA expression levels of S100A16 and keratinocyte differentiation markers. CaLH3 and H357 cell fractions enriched for differentiated cells either by lack of adherence to collagen IV or FACS sorting for low p75NTR expression expressed significantly higher S100A16 mRNA levels than the subpopulations enriched for less differentiated cells. Corroborating these findings, retroviral mediated S100A16 over-expression and knock-down in CaLH3 and H357 cells led to respective up- and down-regulation of differentiation markers. In vitro functional studies showed significant reduction in cell proliferation, sphere formation and 3D-invasive abilities of CaLH3 and H357 cells upon S100A16 over-expression. These functional effects were associated with concomitant down-regulation of self-renewal (Bmi-1 and Oct 4A) and invasion related (MMP1 and MMP9) molecules. S100A16 over-expression also suppressed tumorigenesis of H357 cells in a mouse xenograft model and the resulting tumor xenografts displayed features/expression of increased differentiation and reduced proliferation/self-renewal. Conclusions These results indicate that S100A16 is a differentiation promoting protein and might function as a tumor suppressor in OSCC. Electronic supplementary material The online version of this article (doi:10.1186/s12885-015-1622-1) contains supplementary material, which is available to authorized users.

Published

2015

28. B-Lymphocyte Depletion in Myalgic Encephalopathy/ Chronic Fatigue Syndrome. An Open-Label Phase II Study with Rituximab Maintenance Treatment

Author

Einar Kleboe Kristoffersen, Olav Mella, Øystein Fluge, Dipak Sapkota, Sigrid Lunde, Ingrid Gurvin Rekeland, Olav Dahl, Kari Sørland, Kristin Risa, Ove Bruland, and Kine Alme

Subjects

myalgia, Adult, Male, medicine.medical_specialty, Adolescent, Encephalopathy, Phases of clinical research, lcsh:Medicine, Neutropenia, Lymphocyte Depletion, law.invention, Randomized controlled trial, law, Internal medicine, medicine, Chronic fatigue syndrome, Humans, Immunologic Factors, lcsh:Science, Aged, B-Lymphocytes, Multidisciplinary, Intention-to-treat analysis, Fatigue Syndrome, Chronic, business.industry, lcsh:R, Middle Aged, medicine.disease, Immunology, Rituximab, Female, lcsh:Q, medicine.symptom, business, medicine.drug, Research Article

Abstract

Background Myalgic Encephalopathy/Chronic Fatigue Syndrome (ME/CFS) is a disease of unknown etiology. We previously reported a pilot case series followed by a small, randomized, placebo-controlled phase II study, suggesting that B-cell depletion using the monoclonal anti-CD20 antibody rituximab can yield clinical benefit in ME/CFS. Methods In this single-center, open-label, one-armed phase II study (NCT01156909), 29 patients were included for treatment with rituximab (500 mg/m2) two infusions two weeks apart, followed by maintenance rituximab infusions after 3, 6, 10 and 15 months, and with follow-up for 36 months. Findings Major or moderate responses, predefined as lasting improvements in self-reported Fatigue score, were detected in 18 out of 29 patients (intention to treat). Clinically significant responses were seen in 18 out of 28 patients (64%) receiving rituximab maintenance treatment. For these 18 patients, the mean response durations within the 156 weeks study period were 105 weeks in 14 major responders, and 69 weeks in four moderate responders. At end of follow-up (36 months), 11 out of 18 responding patients were still in ongoing clinical remission. For major responders, the mean lag time from first rituximab infusion until start of clinical response was 23 weeks (range 8–66). Among the nine patients from the placebo group in the previous randomized study with no significant improvement during 12 months follow-up after saline infusions, six achieved a clinical response before 12 months after rituximab maintenance infusions in the present study. Two patients had an allergic reaction to rituximab and two had an episode of uncomplicated late-onset neutropenia. Eight patients experienced one or more transient symptom flares after rituximab infusions. There was no unexpected toxicity. Conclusion In a subgroup of ME/CFS patients, prolonged B-cell depletion with rituximab maintenance infusions was associated with sustained clinical responses. The observed patterns of delayed responses and relapse after B-cell depletion and regeneration, a three times higher disease prevalence in women than in men, and a previously demonstrated increase in B-cell lymphoma risk for elderly ME/CFS patients, suggest that ME/CFS may be a variant of an autoimmune disease. Trial registration ClinicalTrials.gov NCT01156909

Published

2015

29. RACK1 regulates Ki-Ras-mediated signaling and morphological transformation of NIH 3T3 cells

Author

Ove Bruland, Line M. Myklebust, Garry P. Nolan, Ken Roger Rosendal, Bodil Bjørndal, Johan R. Lillehaug, Frøydis D. Myromslien, and James B. Lorens

Subjects

MAPK/ERK pathway, Cancer Research, Molecular Sequence Data, Receptors for Activated C Kinase, PKC alpha, 3T3 cells, Proto-Oncogene Proteins p21(ras), Mice, medicine, Animals, Amino Acid Sequence, Extracellular Signal-Regulated MAP Kinases, Protein Kinase C, Cellular localization, Protein kinase C, Gene Library, Sequence Deletion, biology, Tumor Suppressor Proteins, Neuropeptides, Molecular biology, Actins, Cell Transformation, Neoplastic, medicine.anatomical_structure, Oncology, Mitogen-activated protein kinase, NIH 3T3 Cells, biology.protein, Signal transduction, Signal Transduction

Abstract

Activating Ras mutations are involved in a significant fraction of human tumors. A suppressor screen using a retroviral mouse fibroblast cDNA library was performed to identify novel factors in Ras-mediated transformation. We identified a novel potent inhibitor of Ras-mediated morphological transformation encoded by a truncated version of the receptor for activated C-kinase (RACK1). The truncated protein, designated RACK1DeltaWD1, lacked the N-terminal 49 amino acids encoding the first of the 7 WD40 repeats in RACK1. RACK1DeltaWD1 expression restored contact inhibition, stress fiber formation and reduced ERK phosphorylation in Ki-Ras transformed NIH 3T3 cells. We demonstrate that truncated RACK1 is involved in complexes consisting of wild-type RACK1 and protein kinase C isoforms alpha, betaI and delta, compromising the transduction of an activated Ras signal to the Raf-MEK-ERK pathway. The cellular localization of RACK1DeltaWD1 differed from wtRACK1, indicating that signaling complexes containing the truncated version of RACK1 are incorrectly localized. Notably, 12-O-tetradecanoyl-13-phorbol acetate (TPA) mediated intracellular translocation of RACK1-interacting PKC alpha and delta was abrogated in RACK1DeltaWD1-expressing cells. Our data support a model where RACK1 acts as a key factor in Ki-Ras-mediated morphological transformation.

Published

2006

30. Gene Expression in Poorly Differentiated Papillary Thyroid Carcinomas

Author

Jan Erik Varhaug, Lars A. Akslen, Johan R. Lillehaug, Φystein Fluge, and Ove Bruland

Subjects

Adult, Male, Proto-Oncogene Proteins B-raf, DNA, Complementary, endocrine system diseases, Endocrinology, Diabetes and Metabolism, Cellular differentiation, DNA Mutational Analysis, Extracellular matrix protein 1, Endocrinology, Downregulation and upregulation, Cell Movement, Dock10, Humans, RNA, Messenger, Thyroid Neoplasms, education, In Situ Hybridization, Phylogeny, Aged, Oligonucleotide Array Sequence Analysis, education.field_of_study, biology, Reverse Transcriptase Polymerase Chain Reaction, Cadherin, Cell Differentiation, Middle Aged, Cadherins, Immunohistochemistry, Molecular biology, Carcinoma, Papillary, Extracellular Matrix, Up-Regulation, Gene Expression Regulation, Neoplastic, Fibronectin, Genes, ras, Phenotype, Tumor progression, Mutation, biology.protein, Female, PAX8

Abstract

We used cDNA microarrays to study gene expression in fresh frozen papillary thyroid carcinoma (PTC) specimens. Seven clinically aggressive carcinomas were included, comprising poorly differentiated PTC and tumors with extensive local invasion or synchronous distant metastases. Ten differentiated (classic) papillary thyroid carcinomas (PTC) and non-neoplastic thyroid tissues were also investigated. TaqMan quantitative reverse transcriptase-polymerase chain reaction (RT-PCR), in situ hybridization, and immunohistochemistry verified the differential gene expression. The B-Raf gene was mutated with a T-->A transversion at nucleotide 1799 (V600E) in 8 of 10 differentiated PTC, and in 4 of 7 aggressive carcinomas. Among genes markedly and equally over-expressed in carcinomas of both the aggressive and classic PtC groups, compared to normal thyroid tissue, were CBP/p300 transactivator (CItED1), fibronectin, growth/differentiation factor 15, potassium inwardly rectifying channel KCNJ2, glutaminyl peptide cyclotransferase, WNT7A, and dipeptidyl peptidase IV. A marked upregulation in carcinomas of P-cadherin mRNA and protein concomitant with E-cadherin downregulation, indicates a possible P-E cadherin "switch" in PTC. The growth factor homologue Nel-like 2, dual specificity phosphatase 5, the serine protease kallikrein 10, and also the tight junction genes claudin 1 and claudin 16, were upregulated in classic PTC but not in aggressive tumors, which may be consistent with altered cell polarity in the dedifferentiated PtC. The aggressive, poorly differentiated PtC group was specifically characterized by marked upregulation of several genes related to cell proliferation such as cell division cycle 2 (CDC2), CDC7, kinesin-like 5, ubiquitin conjugating enzyme E2C, and topoisomerase IIalpha, and by upregulation of genes encoding extracellular matrix proteins such as seprase, extracellular matrix protein 1, and several collagens. These aggressive tumors were also characterized by overexpression of the integrin ligand periostin, and in some biopsies also of osteopontin and of the upstream Rac-regulator dedicator of cytokinesis 10 (DOCK10). These data are interpreted to be consistent with altered cell motility, extracellular matrix remodeling and increased cell proliferation, as important processes in PTC tumor progression.

Published

2006

31. S100A16 Functions as a Tumor Suppressor Protein in Oral Squamous Cell Carcinoma

Author

Tarig Al-Hadi Osman, Ove Bruland, Daniela Elena Costea, Himalaya Parajuli, Dipak Sapkota, Muy-Teck Teh, and A.C. Johannessen

Subjects

Oncology, Cancer Research, medicine.medical_specialty, Radiation, business.industry, law.invention, law, Internal medicine, medicine, Suppressor, Radiology, Nuclear Medicine and imaging, Basal cell, business

Published

2016

32. Participation of phospholipase D and α/β-protein kinase C in growth factor-induced signalling in C3H10T1/2 fibroblasts

Author

M. Vorland, Ove Bruland, Holm Holmsen, Johan R. Lillehaug, Bodil Bjørndal, and Vidar A.T. Thorsen

Subjects

MAPK/ERK pathway, Platelet-derived growth factor, Swine, Phosphatidic Acids, Glycerophospholipids, Biology, Cell Line, Mice, chemistry.chemical_compound, 1-Butanol, Epidermal growth factor, Phospholipase D, Animals, RNA, Messenger, Enzyme Inhibitors, Growth Substances, Molecular Biology, Protein Kinase C, Protein kinase C, Platelet-Derived Growth Factor, Mice, Inbred C3H, Mitogen-Activated Protein Kinase 3, Epidermal Growth Factor, Kinase, PLD2, Receptor for activated C kinase 1, Cell Biology, Fibroblasts, Molecular biology, Cell biology, Enzyme Activation, chemistry, Tetradecanoylphorbol Acetate, lipids (amino acids, peptides, and proteins), Mitogen-Activated Protein Kinases, Peptides, Proto-Oncogene Proteins c-fos, Signal Transduction

Abstract

We have studied phospholipase D (PLD) activation in relation to protein kinase C (PKC) and the involvement of PLD in extracellularly regulated kinase 1 (MAPK) (ERK1) activation and c-fos mRNA expression in C3H/10T1/2 (Cl8) fibroblasts. In these cells, the PLD activity was significantly increased by porcine platelet-derived growth factor (PDGF-BB), phorbol 12-myristate 13-acetate (PMA), and epidermal growth factor (EGF). PLD activation by PDGF-BB and PMA, but not EGF, was inhibited in Cl8 cells expressing the HAbetaC2-1 peptide (Cl8 HAbetaC2-1 cells), with a sequence (betaC2-1) shown to bind receptor for activated C kinase 1 (RACK1) and inhibit c-PKC-mediated cell functions [Science 268 (1995) 247]. A role of alpha-PKC in PLD activation is further underscored by co-immunoprecipitation of alpha-PKC with PLD1 and PLD2 in non-stimulated as well as PMA- and PDGF-BB-stimulated Cl8 cells. However, only PKC in PLD1 precipitates was activated by these agonists, while the PKC in the PLD2 precipitates was constitutively activated. The c-fos mRNA levels in Cl8 cells increased more than 30-fold in response to either PDGF-BB, EGF, or PMA. Approximately 60% inhibition of this increase in c-fos mRNA levels was observed in Cl8 HAbetaC2-1 cells. Formation of phosphatidylbutanol (PtdBut) at the expense of phosphatidic acid (PtdH) in the presence of n-butanol inhibited ERK1 activation and c-fos mRNA expression in PDGF-BB-treated Cl8 cells. ERK activation by PMA was unaffected by n-butanol in Cl8 cells but almost abolished by n-butanol in Cl8 HAbetaC2-1 cells, showing that ERK activation by PMA is heavily dependent on PKC and PLD1. In contrast, ERK activation by EGF in both cell types was not sensitive to n-butanol. These results indicate (1) a role of a functional interaction between the RACK1 scaffolding protein and a alphaPKC-PLD complex for achieving full PLD activity in PDGF-BB- and PMA-stimulated Cl8 cells; (2) PLD-mediated PtdH formation is needed for optimal ERK1 activation by PDGF-BB and maximal increase in c-fos mRNA expression. These findings place PLD as an important component in PDGF-BB- and PMA-stimulated intracellular signalling leading to gene activation in Cl8 cells, while EGF does not require PLD.

Published

2003

33. Haplotype Analysis of Norwegian and Swedish Patients with Acute Intermittent Porphyria (AIP): Extreme Haplotype Heterogeneity for the Mutation R116W

Author

Ylva Floderus, Øyvind Skadberg, Ove Bruland, Jaran Apold, Sverre Sandberg, and Kjersti Tjensvoll

Subjects

Porphobilinogen deaminase, Hydroxymethylbilane Synthase, Clinical Biochemistry, SNP, L238P, Single-nucleotide polymorphism, Norwegian, Biology, Polymorphism, Single Nucleotide, porphyria, microsatellites, Gene Frequency, Genetics, medicine, acute intermittent porphyria, Humans, AIP, V215E, Molecular Biology, Allele frequency, Polymorphism, Single-Stranded Conformational, Acute intermittent porphyria, Sweden, lcsh:R5-920, Norway, Biochemistry (medical), Haplotype, General Medicine, HMBS, medicine.disease, haplotyping, Founder Effect, language.human_language, PBGD, Haplotypes, Porphyria, Acute Intermittent, Mutation, genetic markers, language, Other, lcsh:Medicine (General), Microsatellite Repeats, Founder effect

Abstract

Acute intermittent porphyria (AIP), the most common of the acute porphyrias, is caused by mutations in the gene encoding hydroxymethylbilane synthase (HMBS) also called porphobilinogen deaminase (PBGD). The mutation spectrum in the HMBS gene is characterized by a majority of family specific mutations. Among the exceptions are R116W and W198X, with high prevalence in both the Dutch and Swedish populations. These two mutations were also detected in unrelated Norwegian patients. Thus, Norwegian and Swedish patients were haplotyped using closely linked flanking microsatellites and intragenic single nucleotide polymorphisms (SNPs) to see if the high frequency of these two mutations is due to a founder effect. Twelve intragenic SNPs were determined by a method based on fluorescent restriction enzyme fingerprinting single-strand conformation polymorphism (F-REF-SSCP).W198X occurred exclusively on one haplotype in both Norwegian and Swedish patients, showing that it has originated from a common gene source. In contrast, R116W was found on three different haplotypes in three Norwegian families, and in five Swedish families on four or five haplotypes. This extreme haplotype heterogeneity indicates that R116W is a recurrent mutation, maybe explained by the high mutability of CpG dinucleotides. This can also explain why it is the only AIP mutation reported to occur in seven different populations (Norway, Sweden, Finland, Netherlands, France, Spain and South Africa).

Published

2003

34. NATH, a novel gene overexpressed in papillary thyroid carcinomas

Author

Lars A. Akslen, Jan Erik Varhaug, Johan R. Lillehaug, Ove Bruland, and Øystein Fluge

Subjects

Cancer Research, Time Factors, Nath, endocrine system diseases, Blotting, Western, Molecular Sequence Data, In situ hybridization, Biology, Transfection, Thyroid carcinoma, Acetyltransferases, Complementary DNA, Genetics, medicine, Animals, Humans, Amino Acid Sequence, N-Terminal Acetyltransferase E, RNA, Messenger, Thyroid Neoplasms, Northern blot, Cloning, Molecular, Molecular Biology, In Situ Hybridization, N-Terminal Acetyltransferase A, Messenger RNA, Base Sequence, Reverse Transcriptase Polymerase Chain Reaction, cDNA library, Thyroid, Molecular biology, Carcinoma, Papillary, Neoplasm Proteins, Gene Expression Regulation, Neoplastic, medicine.anatomical_structure, COS Cells, Cell Division

Abstract

In this study a replica cDNA screening (RCS) approach to identify genes differentially expressed in papillary thyroid carcinomas (PTC) was used, as compared to non-neoplastic thyroid tissues. RCS is based on hybridization of radioactively labeled cDNA probes made from the biopsies to replica membranes with 15 000 clones from a PTC cDNA library. Among the genes overexpressed in PTC, and especially in clinically aggressive tumors with histologic evidence of poorly differentiated or undifferentiated areas, a novel gene named NATH was found. NATH has two mRNA species, 4.6 and 5.8 kb, both harboring the same open reading frame encoding a putative protein of 866 amino acids. The NATH protein is homologous to yeast N-acetyltransferase (NAT)1 and to mouse NARG1 (mNAT1) and contains four tetratricopeptide repeat (TPR) domains, suggesting that NATH may be part of a multiprotein complex. Overlapping RT-PCR fragments from several PTC biopsies confirmed the NATH mRNA sequence. Northern blots, semiquantitative RT-PCR experiments, TaqMan real-time RT-PCR experiments, and in situ hybridization verified the overexpression of NATH mRNA localized to tumor cells in PTC biopsies. NATH was expressed at a low level in most human adult tissues, including the normal thyroid gland. Increased NATH expression was seen especially in a Burkitt lymphoma cell line and in adult human testis. Recombinant in vitro expression showed that NATH protein was located mainly in the cytoplasm, and was present as a single protein band of the expected 105 kDa molecular weight. Heterologous expression of NATH in the papillary carcinoma cell line (NPA) and 293 cells did not alter the cellular proliferation rate. The biological function of NATH remains to be elucidated, but the overexpression in classic PTC and especially in poorly differentiated or undifferentiated components may indicate a function in the progression of papillary thyroid carcinomas.

Published

2002

35. GBA2 Mutations Cause a Marinesco-Sjögren-Like Syndrome: Genetic and Biochemical Studies

Author

Wenche Telstad, Kristoffer Haugarvoll, Stefan Johansson, Helge Boman, Laurence A. Bindoff, Per M. Knappskog, Inge Jonassen, Ove Bruland, Bjørn Ivar Haukanes, Francisco S. Roque, Jan-Eric Månsson, Carlos E Rodriguez, and Maria Blomqvist

Subjects

Male, 0301 basic medicine, lcsh:Medicine, Pathology and Laboratory Medicine, White Blood Cells, 0302 clinical medicine, Animal Cells, Red Blood Cells, Medicine and Health Sciences, lcsh:Science, Child, Exome sequencing, Spinocerebellar Degenerations, Genetics, Movement Disorders, Multidisciplinary, beta-Glucosidase, Homozygote, Ophthalmic Procedures, Neurodegenerative Diseases, Cataract Surgery, Autosomal recessive cerebellar ataxia, Inherited Metabolic Disorders, Middle Aged, Pedigree, Neurology, Genetic Diseases, Child, Preschool, Glucosylceramidase, Female, Cellular Types, Research Article, Cerebellar Ataxia, Immune Cells, Immunology, Surgical and Invasive Medical Procedures, Single-nucleotide polymorphism, Biology, 03 medical and health sciences, Signs and Symptoms, Autosomal Recessive Diseases, Cataracts, Diagnostic Medicine, medicine, Humans, SNP, Gene, Aged, Clinical Genetics, Phenocopy, Blood Cells, lcsh:R, Biology and Life Sciences, Cell Biology, medicine.disease, Ophthalmology, 030104 developmental biology, Lens Disorders, Metabolic Disorders, Mutation, lcsh:Q, Atrophy, Gaucher's Disease, 030217 neurology & neurosurgery

Abstract

Background: With the advent new sequencing technologies, we now have the tools to understand the phenotypic diversity and the common occurrence of phenocopies. We used these techniques to investigate two Norwegian families with an autosomal recessive cerebellar ataxia with cataracts and mental retardation. Methods and Results: Single nucleotide polymorphism (SNP) chip analysis followed by Exome sequencing identified a 2 bp homozygous deletion in GBA2 in both families, c.1528_1529del [p.Met510Valfs*17]. Furthermore, we report the biochemical characterization of GBA2 in these patients. Our studies show that a reduced activity of GBA2 is sufficient to elevate the levels of glucosylceramide to similar levels as seen in Gaucher disease. Furthermore, leucocytes seem to be the proper enzyme source for in vitro analysis of GBA2 activity. Conclusions: We report GBA2 mutations causing a Marinesco-Sjögren-like syndrome in two Norwegian families. One of the families was originally diagnosed with Marinesco-Sjögren syndrome based on an autosomal recessive cerebellar ataxia with cataracts and mental retardation. Our findings highlight the phenotypic variability associated with GBA2 mutations, and suggest that patients with Marinesco-Sjögren-like syndromes should be tested for mutations in this gene. publishedVersion

Published

2017

36. STUB1 mutations in autosomal recessive ataxias – evidence for mutation-specific clinical heterogeneity

Author

Ketil Heimdal, Ove Bruland, Lise Bjørkhaug, Per M. Knappskog, Bjørn Ivar Haukanes, Ingvild Aukrust, Jens Bollerslev, Torunn Fiskerstrand, Einar Gude, Mònica Sánchez-Guixé, Sigrid Erdal, Stefan Johansson, Jeanette Koht, Helge Boman, Anne Kjersti Erichsen, Chantal M. E. Tallaksen, and Greg Eigner Jablonski

Subjects

Adult, Male, Ataxia, HSC70, Ubiquitin-Protein Ligases, Nonsense mutation, Mutation, Missense, Genes, Recessive, Biology, medicine.disease_cause, Young Adult, Heat shock protein, medicine, Humans, Missense mutation, Genetics(clinical), Pharmacology (medical), E3-ubiquitin ligase, Genetics (clinical), Exome sequencing, STUB1, Genetics, Medicine(all), Mutation, CHIP, Research, Hypogonadism, Homozygote, ARCA, General Medicine, Magnetic Resonance Imaging, Molecular biology, Hsp70, Female, medicine.symptom

Abstract

Background A subset of hereditary cerebellar ataxias is inherited as autosomal recessive traits (ARCAs). Classification of recessive ataxias due to phenotypic differences in the cerebellum and cerebellar structures is constantly evolving due to new identified disease genes. Recently, reports have linked mutations in genes involved in ubiquitination (RNF216, OTUD4, STUB1) to ARCA with hypogonadism. Methods and results With a combination of homozygozity mapping and exome sequencing, we identified three mutations in STUB1 in two families with ARCA and cognitive impairment; a homozygous missense variant (c.194A > G, p.Asn65Ser) that segregated in three affected siblings, and a missense change (c.82G > A, p.Glu28Lys) which was inherited in trans with a nonsense mutation (c.430A > T, p.Lys144Ter) in another patient. STUB1 encodes CHIP (C-terminus of Heat shock protein 70 – Interacting Protein), a dual function protein with a role in ubiquitination as a co-chaperone with heat shock proteins, and as an E3 ligase. We show that the p.Asn65Ser substitution impairs CHIP’s ability to ubiquitinate HSC70 in vitro, despite being able to self-ubiquitinate. These results are consistent with previous studies highlighting this as a critical residue for the interaction between CHIP and its co-chaperones. Furthermore, we show that the levels of CHIP are strongly reduced in vivo in patients’ fibroblasts compared to controls. Conclusions These results suggest that STUB1 mutations might cause disease by impacting not only the E3 ligase function, but also its protein interaction properties and protein amount. Whether the clinical heterogeneity seen in STUB1 ARCA can be related to the location of the mutations remains to be understood, but interestingly, all siblings with the p.Asn65Ser substitution showed a marked appearance of accelerated aging not previously described in STUB1 related ARCA, none display hormonal aberrations/clinical hypogonadism while some affected family members had diabetes, alopecia, uveitis and ulcerative colitis, further refining the spectrum of STUB1 related disease. Electronic supplementary material The online version of this article (doi:10.1186/s13023-014-0146-0) contains supplementary material, which is available to authorized users.

Published

2014

37. Accurate determination of the number of CAG repeats in the Huntington disease gene using a sequence-specific internal DNA standard

Author

Helge Boman, Per M. Knappskog, E. Almqvist, Y P Goldberg, Ove Bruland, and Michael R. Hayden

Subjects

Genetics, Biology, Molecular biology, law.invention, DNA sequencer, chemistry.chemical_compound, chemistry, law, Huntingtin Protein, Allele, Repeated sequence, Polyacrylamide gel electrophoresis, Gene, Genetics (clinical), Polymerase chain reaction, DNA

Abstract

We have developed a sequence-specific internal DNA size standard for the accurate determination of the number of CAG repeats in the Huntington disease (HD) gene by cloning key fragments (between 15 and 64 CAG repeats) of the HD gene. These fragments, pooled to produce a sequence-specific DNA ladder, enabled us to observe the true number of CAG repeats directly, with no need for calculations. Comparison of the calculated numbers of CAG repeats in the HD gene using this sequence-specific DNA standard with a commercially available standard (GENESCAN-500 TAMRA) showed that the latter underestimated the number of CAG repeats by three when analyzed by capillary electrophoresis on the ABI 310 Genetic Analyzer (POP4 polymer). In contrast, the use of the same standard overestimated the number of CAG repeats by one when the samples were analyzed by denaturing polyacrylamide electrophoresis on ABI 377 DNA Sequencer (6% denaturing polyacrylamide gel). This suggests that our sequence-specific standard provides greater accuracy for the determination of the true number of CAG repeats in the HD gene than commercially available standards. The sequence-specific standard can be radioactively labeled and successfully replace conventional DNA size standards when analyzing polymerase chain reaction (PCR)-amplified HD alleles by denaturing polyacrylamide electrophoresis.

Published

1999

38. [Untitled]

Author

Johan R. Lillehaug, Holm Holmsen, Vidar A.T. Thorsen, and Ove Bruland

Subjects

Phospholipase D, PLD2, Clinical Biochemistry, Cell Biology, General Medicine, 12-O-Tetradecanoylphorbol-13-acetate, chemistry.chemical_compound, chemistry, Biochemistry, Phosphatidylcholine, Choline, lipids (amino acids, peptides, and proteins), CDP-choline pathway, Choline transport, Molecular Biology, Protein kinase C

Abstract

We have shown that 12-O-tetradecanoylphorbol 13-acetate (TPA) increases protein kinase C (PKC)-mediated choline transport, incorporation of choline into phosphatidylcholine (PtdCho) and PtdCho degradation by phospholipase D (PLD) in C3H10T1/2 Cl 8 cells. Dual prelabeling experiment using [3H]/[14C]choline indicated that intracellular choline generated from the PLD reaction was not directly recycled to PtdCho synthesis within the cell, and that a large fraction of the choline was transported out of the TPA-treated cells. In contrast, medium derived choline was preferably channeled to PtdCho synthesis. These results indicate that in TPA-treated cells, the choline derived from the PKC-mediated increased PLD activity and the choline newly taken up by the cell behave as two distinctly different metabolic pools.

Published

1998

39. PKU mutation (D143G) associated with an apparent high residual enzyme activity: Expression of a kinetic variant form of phenylalanine hydroxylase in three different systems

Author

Torgeir Flatmark, Per M. Knappskog, Aurora Martinez, Ove Bruland, Jaran Apold, and Hans Geir Eiken

Subjects

Phenylalanine hydroxylase, Recombinant Fusion Proteins, Glycine, Kidney, Polymerase Chain Reaction, Cell Line, Hydroxylation, chemistry.chemical_compound, Phenylketonurias, medicine, Escherichia coli, Genetics, Humans, Enzyme kinetics, Enzyme inducer, Cloning, Molecular, Genetics (clinical), chemistry.chemical_classification, Aspartic Acid, biology, Genetic Variation, Phenylalanine Hydroxylase, Tetrahydrobiopterin, Exons, Fusion protein, Molecular biology, Enzyme assay, Kinetics, Enzyme, chemistry, Biochemistry, biology.protein, Mutagenesis, Site-Directed, medicine.drug

Abstract

We have used three complementary in vitro systems to express the human phenylalanine hydroxylase (PAH) gene at high levels. Recombinant PAH was expressed in Escherichia coli (as a fusion protein), in human kidney cells and in a cell-free in vitro transcription-translation system. These systems were used to characterize a novel kinetic variant form (D143G) of the enzyme. The recombinant D143G mutant enzyme had the same physicochemical properties as the wild-type PAH and was stable when expressed in eukaryotic cells. Enzyme activity studies of the D143G mutant enzyme, produced in the three expression systems, revealed a kinetic variant form with reduced affinity for L-Phe (about 2.4.fold increase in the SOe5 value) as well as reduced affinity for tetrahydrobiopterin (BH,) (about 2.fold increase in the apparent K,,,). At standard assay conditions (1 mM L-Phe, 75 WM BH,) the residual activity of the mutant enzyme was high and variable (52%, 33%, and 102%) when analysed in the three different systems. The high residual activities of the mutant enzyme obtained at these conditions were not in agreement with the classical PKU phenotype found in a patient compound heterozygous for the termination mutation G272X and the novel D 143G mutation. However, when the D143G mutant enzyme was assayed at lower concentrations of L-Phe (100-300 pM) and BH, (10 pM) the residual activities were compatible with severely reduced hydroxylation of L-Phe and the classical PKU phenotype. 0 1996 Wiley-Liss, Inc.

Published

1996

40. Evidence for anticipation in Beckwith-Wiedemann syndrome

Author

Mia Appelbäck, I. Karen Temple, Ove Bruland, Deborah J G Mackay, Karin Buiting, Siren Berland, Gunnar Houge, and Jasmin Beygo

Subjects

Male, Beckwith-Wiedemann Syndrome, Adolescent, Medizin, Beckwith–Wiedemann syndrome, Biology, Article, Medical genetics: 714 [VDP], Medisinsk genetikk: 714 [VDP], symbols.namesake, Genomic Imprinting, Insulin-Like Growth Factor II, Genetics, medicine, Humans, Imprinting (psychology), Allele, Child, Genetics (clinical), Alleles, Sanger sequencing, Maternal Transmission, Binding Sites, H19, Chromosomes, Human, Pair 11, IGF2, Methylation, DNA Methylation, medicine.disease, DNA methylation, Genomic Structural Variation, Mutation, symbols, anticipation, Female, RNA, Long Noncoding, imprinting, Genomic imprinting, Octamer Transcription Factor-3

Abstract

Classical Beckwith–Wiedemann syndrome (BWS) was diagnosed in two sisters and their male cousin. The children’s mothers and a third sister were tall statured (178, 185 and 187 cm) and one had mild BWS features as a child. Their parents had average heights of 173 cm (mother) and 180 cm (father). This second generation tall stature and third generation BWS correlated with increased methylation of the maternal H19/IGF2-locus. The results were obtained by bisulphite treatment and subclone Sanger sequencing or next generation sequencing to quantitate the degree of CpG-methylation on three locations: the H19 promoter region and two CTCF binding sites in the H19 imprinting control region (ICR1), specifically in ICR1 repeats B1 and B7. Upon ICR1 copy number analysis and sequencing, the same maternal point variant NCBI36:11:g.1979595T>C that had been described previously as a cause of BWS in three brothers, was found. As expected, this point variant was on the paternal allele in the non-affected grandmother. This nucleotide variant has been shown to affect OCTamer-binding transcription factor-4 (OCT4) binding, which may be necessary for maintaining the unmethylated state of the maternal allele. Our data extend these findings by showing that the OCT4 binding site mutation caused incomplete switching from paternal to maternal ICR1 methylation imprint, and that upon further maternal transmission, methylation of the incompletely demethylated variant ICR1 allele was further increased. This suggests that maternal and paternal ICR1 alleles are treated differentially in the female germline, and only the paternal allele appears to be capable of demethylation. publishedVersion

Published

2012

41. Disruption of a long distance regulatory region upstream of SOX9 in isolated disorders of sex development

Author

Audrey Labalme, Vincent R. Harley, Delphine Mallet, Atle Brendehaug, Gunnar Houge, Christopher T. Gordon, Sabina Benko, Ove Bruland, Stanislas Lyonnet, Anders Molven, Damien Sanlaville, Frédéric Huet, Yves Morel, Patrick Callier, Laurence Faivre, Rajini Sreenivasan, Michel David, Valérie Malan, Frédérique Dijoud, Sophie Thomas, Christel Thauvin-Robinet, Arnold Munnich, Jeanne Amiel, and Marc Nicolino

Subjects

Male, endocrine system, Gonad, 46, XX Disorders of Sex Development, DNA Copy Number Variations, Locus (genetics), SOX9, Biology, Regulatory Sequences, Nucleic Acid, Gene Duplication, Genetics, medicine, Humans, Disorders of sex development, Copy-number variation, Enhancer, Child, Genetics (clinical), Alleles, Gonadal Dysgenesis, 46,XY, Comparative Genomic Hybridization, Chromosome Mapping, Infant, SOX9 Transcription Factor, Sex reversal, medicine.disease, Sex-Determining Region Y Protein, Pedigree, Testis determining factor, medicine.anatomical_structure, Haplotypes, embryonic structures, Female, Gonadoblastoma

Abstract

Background The early gonad is bipotential and can differentiate into either a testis or an ovary. In XY embryos, the SRY gene triggers testicular differentiation and subsequent male development via its action on a single gene, SOX9 . The supporting cell lineage of the bipotential gonad will differentiate as testicular Sertoli cells if SOX9 is expressed and conversely will differentiate as ovarian granulosa cells when SOX9 expression is switched off. Results Through copy number variation mapping this study identified duplications upstream of the SOX9 gene in three families with an isolated 46,XX disorder of sex development (DSD) and an overlapping deletion in one family with two probands with an isolated 46,XY DSD. The region of overlap between these genomic alterations, and previously reported deletions and duplications at the SOX9 locus associated with syndromic and isolated cases of 46,XX and 46,XY DSD, reveal a minimal non-coding 78 kb sex determining region located in a gene desert 517–595 kb upstream of the SOX9 promoter. Conclusions These data indicate that a non-coding regulatory region critical for gonadal SOX9 expression and subsequent normal sex development is located far upstream of the SOX9 promoter. Its copy number variations are the genetic basis of isolated 46,XX and 46,XY DSDs of variable severity (ranging from mild to complete sex reversal). It is proposed that this region contains a gonad specific SOX9 transcriptional enhancer(s), the gain or loss of which results in genomic imbalance sufficient to activate or inactivate SOX9 gonadal expression in a tissue specific manner, switch sex determination, and result in isolated DSD.

Published

2011

42. S100A14 inhibits proliferation of oral carcinoma derived cells through G1-arrest

Author

Daniela Elena Costea, Endre N. Vasstrand, Salah O. Ibrahim, Ove Bruland, Dipak Sapkota, Magnus Blø, and James B. Lorens

Subjects

Cyclin-Dependent Kinase Inhibitor p21, Cancer Research, Cell cycle checkpoint, Cell, Blotting, Western, Biology, medicine.disease_cause, Small hairpin RNA, Cell Line, Tumor, medicine, Gene silencing, Humans, RNA, Messenger, RNA, Small Interfering, Cyclin-Dependent Kinase Inhibitor Proteins, Mouth neoplasm, Cell growth, Calcium-Binding Proteins, G1 Phase, Cell Cycle Checkpoints, stomatognathic diseases, medicine.anatomical_structure, Oncology, Cancer research, Carcinoma, Squamous Cell, Mouth Neoplasms, Oral Surgery, Tumor Suppressor Protein p53, Carcinogenesis, Cyclin-dependent kinase inhibitor protein

Abstract

Altered expression of S100A14 has been reported in various human cancers including oral squamous cell carcinomas (OSCCs). Its biological functions in carcinogenesis, however, are largely unknown. This study aimed to investigate the functional role of S100A14 in tumor cell proliferation and its possible functional association with p53. S100A14 protein was found to be gradually down-regulated during the transition from normal to dysplastic and carcinoma cells in an in vitro human OSCC progression model. When over-expressed by employing retroviral expression vector, S100A14 inhibited proliferation of CaLH3 and OSCC1, OSCC cell-lines harboring wild type (wt) p53, by inducing G1-arrest. This G1-arrest correlated with up-regulation of p21 both in the CaLH3 and OSCC1 cell-lines. shRNA mediated silencing of p53 led to partial suppression of p21 in S100A14 over-expressing CaLH3 cells, indicating that p21 up-regulation was, at least, partly dependent on p53. We further demonstrated that nuclear accumulation of p53 occurred with over-expression of S100A14 in CaLH3 cells. Our data suggest a novel role of S100A14 in OSCC cell proliferation by inducing G1-arrest and also indicate a functional link between S100A14 and the tumor suppressor protein p53.

Published

2011

43. Benefit from B-lymphocyte depletion using the anti-CD20 antibody rituximab in chronic fatigue syndrome. A double-blind and placebo-controlled study

Author

Anette Storstein, Dipak Sapkota, Einar K. Kristoffersen, Ove Bruland, Kristin Risa, Olav Dahl, Øystein Fluge, Olav Mella, Harald Nyland, and Halvor Naess

Subjects

Male, B Cells, Anatomy and Physiology, Placebo-controlled study, lcsh:Medicine, Autoimmunity, Polymerase Chain Reaction, law.invention, Placebos, Antibodies, Monoclonal, Murine-Derived, Medical disciplines: 700::Clinical medical disciplines: 750::Oncology: 762 [VDP], Randomized controlled trial, law, Immune Physiology, Medicine, lcsh:Science, Psychiatry, B-Lymphocytes, Multidisciplinary, Fatigue Syndrome, Chronic, Clinical Pharmacology, Middle Aged, Clinical Laboratory Sciences, Treatment Outcome, Mental Health, Rituximab, Female, Immunotherapy, medicine.drug, Research Article, Adult, medicine.medical_specialty, Drugs and Devices, Clinical Research Design, Immune Cells, Medical disciplines: 700::Clinical medical disciplines: 750 [VDP], Immunology, Immunopathology, Placebo, Lymphocyte Depletion, Antibodies, Autoimmune Diseases, Immunomodulation, Double-Blind Method, Rheumatology, Diagnostic Medicine, Internal medicine, Psoriasis, Chronic fatigue syndrome, Humans, Clinical Trials, Adverse effect, Biology, business.industry, lcsh:R, Immunity, Repeated measures design, medicine.disease, Antigens, CD20, Therapies, Clinical Immunology, lcsh:Q, business

Abstract

Background Chronic fatigue syndrome (CFS) is a disease of unknown aetiology. Major CFS symptom relief during cancer chemotherapy in a patient with synchronous CFS and lymphoma spurred a pilot study of B-lymphocyte depletion using the anti-CD20 antibody Rituximab, which demonstrated significant clinical response in three CFS patients. Methods and Findings In this double-blind, placebo-controlled phase II study (NCT00848692), 30 CFS patients were randomised to either Rituximab 500 mg/m2 or saline, given twice two weeks apart, with follow-up for 12 months. Xenotropic murine leukemia virus-related virus (XMRV) was not detected in any of the patients. The responses generally affected all CFS symptoms. Major or moderate overall response, defined as lasting improvements in self-reported Fatigue score during follow-up, was seen in 10 out of 15 patients (67%) in the Rituximab group and in two out of 15 patients (13%) in the Placebo group (p = 0.003). Mean response duration within the follow-up period for the 10 responders to Rituximab was 25 weeks (range 8–44). Four Rituximab patients had clinical response durations past the study period. General linear models for repeated measures of Fatigue scores during follow-up showed a significant interaction between time and intervention group (p = 0.018 for self-reported, and p = 0.024 for physician-assessed), with differences between the Rituximab and Placebo groups between 6–10 months after intervention. The primary end-point, defined as effect on self-reported Fatigue score 3 months after intervention, was negative. There were no serious adverse events. Two patients in the Rituximab group with pre-existing psoriasis experienced moderate psoriasis worsening. Conclusion The delayed responses starting from 2–7 months after Rituximab treatment, in spite of rapid B-cell depletion, suggests that CFS is an autoimmune disease and may be consistent with the gradual elimination of autoantibodies preceding clinical responses. The present findings will impact future research efforts in CFS. Trial registration ClinicalTrials.gov NCT00848692

Published

2011

44. S100A14 regulates the invasive potential of oral squamous cell carcinoma derived cell-lines in vitro by modulating expression of matrix metalloproteinases, MMP1 and MMP9

Author

Salah O. Ibrahim, Hallvard Haugen, Endre N. Vasstrand, Ove Bruland, Daniela Elena Costea, and Dipak Sapkota

Subjects

Cancer Research, Pathology, medicine.medical_specialty, MMP1, Cell, Down-Regulation, Biology, MMP9, Downregulation and upregulation, Cell Line, Tumor, medicine, Humans, Neoplasm Invasiveness, RNA, Messenger, Gene knockdown, Matrigel Invasion Assay, Calcium-Binding Proteins, Immunohistochemistry, Neoplasm Proteins, stomatognathic diseases, medicine.anatomical_structure, Oncology, Matrix Metalloproteinase 9, Cell culture, Cancer research, Carcinoma, Squamous Cell, Mouth Neoplasms, Matrix Metalloproteinase 1

Abstract

Despite the differential expression of S100A14 (a newly identified S100 member) in various human cancers including oral squamous cell carcinomas (OSCCs), its biological role in tumour invasion has not been characterised. The aim of this study was thus to investigate the possible role of S100A14 in OSCC cell invasion. Using immunohistochemistry in normal (n=13), dysplastic (n=10) and OSCC (n=16) archival tissues, S100A14 protein was found to be down-regulated/lost with concomitant membrane to cytoplasmic translocation in OSCCs, especially in the invading tumour islands. These expression data were corroborated by profiling S100A14 mRNA expression using quantitative RT-PCR (qRT-PCR) in an in vitro human OSCC progression model consisting of cell-lines derived from normal (n=3), dysplastic (n=3) and OSCC (n=8) tissues. Employing in vitro Matrigel invasion assay, we demonstrated that retroviral vector mediated over-expression of S100A14 resulted in significant decrease in the invasive potential of OSCC derived CaLH3 and H357 cell-lines whereas siRNA mediated knockdown resulted in significant increase in the invasive potential of CaLH3 cell-line. Pathway focused PCR array and validation using qRT-PCR revealed that S100A14 over-expression was associated with down-regulation of MMP1 and MMP9 mRNAs in both CaLH3 and H357 cell-lines. Further, S100A14 over-expression was found to be associated with suppression of MMP9 gelatinolytic activity in CaLH3 cell-line. Additionally, an inverse correlation between mRNA expression levels of MMP1 and MMP9 with S100A14 was found in 19 cases of OSCCs. Collectively, these data provide the first evidence for a role of S100A14 protein in regulation of OSCC cell invasion by modulating expression of MMP1 and MMP9.

Published

2010

45. Decorin accumulation contributes to the stromal opacities found in congenital stromal corneal dystrophy

Author

Eyvind Rødahl, Cecilie Bredrup, Per M. Knappskog, Barbara P. Palka, Robert D. Young, Jan Haavik, Espen Stang, and Ove Bruland

Subjects

Stromal cell, Indoles, Decorin, Immunoelectron microscopy, Corneal Stroma, Blotting, Western, Immunoblotting, Gene Expression, Kidney, Transfection, Corneal Opacity, Cornea, Gene expression, medicine, Organometallic Compounds, Humans, RNA, Messenger, Microscopy, Immunoelectron, Cells, Cultured, Corneal Dystrophies, Hereditary, Staining and Labeling, Chemistry, Reverse Transcriptase Polymerase Chain Reaction, Fibroblasts, medicine.disease, Molecular biology, In vitro, carbohydrates (lipids), Blot, medicine.anatomical_structure, Chromatography, Gel, Congenital stromal corneal dystrophy, Plasmids

Abstract

Purpose Congenital stromal corneal dystrophy (CSCD) is characterized by stromal opacities that morphologically are seen as interlamellar layers of amorphous substance with small filaments, the nature of which has hitherto been unknown. CSCD is associated with truncating mutations in the decorin gene (DCN). To understand the molecular basis for the corneal opacities we analyzed the expression of decorin in this disease, both at the morphologic and the molecular level. Methods Corneal specimens were examined after contrast enhancement with cuprolinic blue and by immunoelectron microscopy. Decorin protein from corneal tissue and keratocyte culture was studied by immunoblot analysis before and after O- and N-deglycosylation. The relative level of DCN mRNA expression was examined using Q-RT-PCR, and cDNA was sequenced. Recombinant wild-type and truncated decorin transiently expressed in HEK293 cells were analyzed by gel filtration and immunoblotting. Results The areas of interlamellar filaments were stained by cuprolinic blue. Immunoelectron microscopy using decorin antibodies revealed intense labeling of these areas. Both wild-type and truncated decorin protein was expressed in corneal tissue and keratocytes of affected persons. When decorin expressed in HEK293 cells was examined by gel filtration, the truncated decorin eluted as high molecular weight aggregates. Conclusions Accumulation of decorin was found in the interlamellar areas of amorphous substance. The truncated decorin is present in CSCD corneas, and there is evidence it may aggregate in vitro. Thus, decorin accumulation appears to contribute to the stromal opacities that are characteristic of CSCD.

Published

2010

46. Kinetics study on markers of the immune system by gene expression profiling of an in vivo heated tumor

Author

Øystein Fluge, Erling Dahl Borkamo, Ove Bruland, and Olav Dahl

Subjects

Hyperthermia, Cancer Research, Pathology, medicine.medical_specialty, Microarray, Physiology, CD14, Gene Expression, Biology, Immune system, Physiology (medical), Intensive care, Glioma, Neoplasms, Gene expression, medicine, Animals, Gene Expression Profiling, Hyperthermia, Induced, medicine.disease, Microarray Analysis, Rats, Gene expression profiling, Immune System, Cancer research, Biomarkers

Abstract

To analyze effects of hyperthermia on immune cells within tumors.Subcutaneously implanted rat gliomas were treated with water-bath hyperthermia for one hour at day zero (HT) (intratumoral temperature of 43 degrees C), low-dose metronomic cyclophosphamide (CTX) 35 mg/kg three times a week for two weeks, both HT and CTX (CTX-HT(0)), or saline. Tumors harvested at day 1, 7, 14 and 21 were analyzed for changes in gene expression by microarrays, focusing on genes expressed in immune cells. Microarray analyses and real-time RT-PCR were previously performed on tumors harvested day zero at 0, 45, 90 and 180 minutes after end of treatment. Gene expression kinetics of selected genes were analyzed in all tumors by quantitative real-time RT-PCR (qPCR) to validate the results of the microarrays.Previous microarray analyses have indicated a suppression of gene expression in immune cells within tumors by hyperthermia the first three hours after treatment. qPCR analyses of CD14, CD36, Klrd1 (CD94), Tlr2 and Lrp1 confirmed these results. Global mRNA screen revealed no hyperthermia-induced changes in gene expression of immune cells at day 1, 7, 14 and 21. qPCR analyses of CD14, CD36, Klrd1 (CD94), Tlr2 and Lrp1 confirmed the results of the microarrays, i.e. none of these were differentially expressed after the first day, with the exception of Lrp1 which displayed elevated mRNA levels.The suppression in gene expression of a range of immune cells within tumors treated with hyperthermia at 43 degrees C is a transient phenomenon.

Published

2009

47. cDNA microarray analysis of serially sampled cervical cancer specimens from patients treated with thermochemoradiotherapy

Author

Baard-Christian Schem, Erling Dahl Borkamo, Olav Mella, Øystein Fluge, Ove Bruland, and Olav Dahl

Subjects

Adult, Cancer Research, Pathology, medicine.medical_specialty, Time Factors, Microarray, Biopsy, Alpha interferon, Uterine Cervical Neoplasms, Antineoplastic Agents, Cervix Uteri, medicine.disease_cause, Gene expression, Gene duplication, medicine, Humans, Radiology, Nuclear Medicine and imaging, Interferon alfa, Aged, Oligonucleotide Array Sequence Analysis, Receptors, Interferon, Radiation, Microarray analysis techniques, business.industry, Norway, Tumor Necrosis Factor-alpha, NF-kappa B, Interferon-alpha, Radiotherapy Dosage, Hyperthermia, Induced, Interferon-beta, Middle Aged, Combined Modality Therapy, Neoplasm Proteins, Oncology, Cancer research, Carcinoma, Squamous Cell, Female, DNA microarray, Cisplatin, Carcinogenesis, business, medicine.drug

Abstract

Purpose To elucidate changes in gene expression after treatment with regional thermochemoradiotherapy in locally advanced squamous cell cervical cancer. Methods and Materials Tru-Cut biopsy specimens were serially collected from 16 patients. Microarray gene expression levels before and 24 h after the first and second trimodality treatment sessions were compared. Pathway and network analyses were conducted by use of Ingenuity Pathways Analysis (IPA; Ingenuity Systems, Redwood City, CA). Single gene expressions were analyzed by quantitative real-time reverse transcription–polymerase chain reaction. Results We detected 53 annotated genes that were differentially expressed after trimodality treatment. Central in the three top networks detected by IPA were interferon alfa, interferon beta, and interferon gamma receptor; nuclear factor κB; and tumor necrosis factor, respectively. These genes encode proteins that are important in regulation cell signaling, proliferation, gene expression, and immune stimulation. Biological processes over-represented among the 53 genes were fibrosis, tumorigenesis, and immune response. Conclusions Microarrays showed minor changes in gene expression after thermochemoradiotherapy in locally advanced cervical cancer. We detected 53 differentially expressed genes, mainly involved in fibrosis, tumorigenesis, and immune response. A limitation with the use of serial biopsy specimens was low quality of ribonucleic acid from tumors that respond to highly effective therapy. Another “key limitation” is timing of the post-treatment biopsy, because 24 h may be too late to adequately assess the impact of hyperthermia on gene expression.

Published

2009

48. Expression profile of the S100 gene family members in oral squamous cell carcinomas

Author

Dipak, Sapkota, Ove, Bruland, Olav E, Bøe, Hala, Bakeer, Osman A A, Elgindi, Endre N, Vasstrand, and Salah O, Ibrahim

Subjects

Adult, Aged, 80 and over, Male, Tobacco, Smokeless, Reverse Transcriptase Polymerase Chain Reaction, Gene Expression Profiling, S100 Proteins, Down-Regulation, Middle Aged, Gene Expression Regulation, Neoplastic, Sudan, Young Adult, Biomarkers, Tumor, Carcinoma, Squamous Cell, Humans, Female, Mouth Neoplasms, Aged

Abstract

Several of the S100 gene members have been reported to be differentially expressed in many human pathological conditions, in particular, the malignancies. Identification and quantification of the differentially expressed S100 gene members in oral squamous cell carcinoma (OSCC) might facilitate their use as potential diagnostic and/or prognostic markers or targets for therapy.we examined the expression profile of 16 members of the S100 gene family at the mRNA level by semiquantitative reverse transcription-polymerase chain reaction (sRT-PCR) in 27 cases of OSCCs/their pair-wised normal controls obtained from Sudanese patients, and confirmed the sRT-PCR results by performing quantitative real time-polymerase chain reaction (qRT-PCR) for 6 of the 16 genes examined.With sRT-PCR, 4 (25%; S100A4, S100A6, S100A8, S100A14) out of the 16 S100 gene members examined were found to be significantly down-regulated (P0.05) in the tumors compared to the normal controls. None of the S100 gene members examined were found to be significantly up-regulated in the tumors. qRT-PCR results confirmed the significant down-regulation of the S100A4, S100A6, and S100A14 genes in the tumors examined.S100 gene family members might play an important role in the pathogenesis of the OSCCs examined. Findings of the present work warrant in-depth studies of the S100 gene family members, in particular, the S100A4, S100A6, S100A8, and S100A14 to further understand their possible role(s) in OSCC tumorigenesis.

Published

2008

49. Global gene expression analyses reveal changes in biological processes after hyperthermia in a rat glioma model

Author

Olav Dahl, Øystein Fluge, Erling Dahl Borkamo, and Ove Bruland

Subjects

Cancer Research, Pathology, medicine.medical_specialty, Cell signaling, Microarray, Physiology, Apoptosis, Biology, In vivo, Physiology (medical), Glioma, Intensive care, Cell Line, Tumor, Gene expression, medicine, Animals, Transcription factor, Gene, Heat-Shock Proteins, Oligonucleotide Array Sequence Analysis, Neovascularization, Pathologic, Reverse Transcriptase Polymerase Chain Reaction, Immunity, Proteins, Hyperthermia, Induced, medicine.disease, Molecular biology, Rats, Gene Expression Regulation, Neoplastic, Neoplasm Transplantation, Transcription Factors

Abstract

To elucidate the thermal impact on biological processes the first three hours after hyperthermia (HT).Tumor samples from BT(4)An rat tumors were transplanted subcutaneously to the right hind foot of BD IX rats, treated with local water-bath HT (mean tumor temperature of 43 degrees C) for one hour, and analyzed for changes in global gene expression the first three hours after treatment with HT. Samples from a corresponding in vitro experiment were also analyzed. Differentially expressed genes in vivo were mapped to a gene ontology (GO) database in search for biological processes overrepresented after treatment with HT. Selected genes were verified using Taqman quantitative RT-PCR.1213 genes were differentially expressed after HT treatment in vivo. Processes overrepresented by GO mapping could be sorted into 10 main functional groups; apoptosis, transcription, immune system, blood vessels, metabolism/protein modifications, differentiation, cell signaling, response to stimulus, transport and cytoskeleton. We detected reduced mRNA levels of a wide range of T-cell, natural killer cell and antigen presenting cell-related genes after HT.To our best knowledge, this is the first global microarray analysis of a malignant tumor treated with HT in vivo. We highlight biological processes affected by HT. RNA expression profiles also indicate a rapid suppression of the immune system within tumors by local HT.

Published

2008

50. Gene expression reveals two distinct groups of anal carcinomas with clinical implications

Author

A. Skarstein, Ove Bruland, Heike Immervoll, Øystein Fluge, Lise Balteskard, Mette Pernille Myklebust, and Olav Dahl

Subjects

Cancer Research, Candidate gene, Tumor suppressor gene, anal cancer, Papillomavirus E7 Proteins, Protein Array Analysis, Gene Expression, Cell Cycle Proteins, Biology, CDKN2A, Gene expression, medicine, gene expression profiling, Anal cancer, Humans, RNA, Messenger, human papillomavirus, Gene, Molecular Diagnostics, In Situ Hybridization, Oligonucleotide Array Sequence Analysis, MCM7, Human papillomavirus 16, Genes, p16, Nuclear Proteins, Oncogene Proteins, Viral, Viral Load, medicine.disease, Anus Neoplasms, Minichromosome Maintenance Complex Component 7, Molecular biology, Gene expression profiling, DNA-Binding Proteins, Real-time polymerase chain reaction, Oncology, Cancer research, CDKN2A (p16), microarray

Abstract

Human papillomavirus (HPV) is a major aetiological agent in anal carcinomas. We here present a study of global gene expression using microarray hybridisation in a collection of anal carcinoma biopsies. Quantitative PCR was used to verify expression of selected genes. All biopsies contained integrated DNA of human papillomavirus subtype 16 (HPV16) and expressed HPV16 E7 mRNA. No other subspecies of HPV were detected in these 13 biopsies as assessed by PCR amplification and DNA sequencing. Unsupervised cluster analysis, based on global mRNA expression, divided the tumour biopsies into two distinct groups. Cluster analysis based on a number of high-risk HPV and/or E2F-regulated genes reproduced this biopsy grouping, suggesting that integrated HPV16 substantially influenced global gene expression in approximately half the biopsies studied. The levels of HPV16 E7 mRNA were significantly different between the two groups, but with considerable overlap. Thus, influence on global gene expression could not be absolutely ascribed to the expression level of HPV16. To investigate whether this distinction in gene expression had prognostic impact, we studied protein expression in an independent cohort of 55 anal carcinomas not included in the microarray study of two differentially expressed candidate genes, minichromosome maintenance complex component 7 (MCM7) and cyclin-dependent kinase inhibitor 2A (CDKN2A or p16). HPV status was assessed by in situ hybridisation. There was a significant association between in situ staining for HPV E7 mRNA and immunostaining for CDKN2A (p16) and MCM7 protein. CDKN2A (p16) mRNA was found significantly differentially expressed between the two tumour groups. However, cluster analysis on genes directly regulated by CDKN2A (p16) could not reproduce this split of biopsies into two groups, suggesting that the transcriptional regulatory activity of CDKN2A in these biopsies is inhibited. Furthermore, protein expression of CDKN2A (p16) could not be associated with survival. MCM7 is directly regulated by E2F and induced by HPV, and its mRNA was found differentially expressed between the two tumour groups. High level of MCM7 protein was found to be associated with both improved relapse-free survival (RFS, P=0.02) and cancer-specific survival (CSS, P=0.03) in anal cancer patients treated with radiation with or without additional chemotherapy.

Published

2008