Your search keyword '"Steen HB"' showing total 118 results

1. Proliferation and apoptosis in malignant and normal cells in B-cell non-Hodgkin's lymphomas

Author

Stokke, T, primary, Holte, H, additional, Smedshammer, L, additional, Smeland, EB, additional, Kaalhus, O, additional, and Steen, HB, additional

Published

1998

2. Anti-tumour activity of photodynamic therapy in combination with mitomycin C in nude mice with human colon adenocarcinoma

Author

Ma, LW, primary, Moan, J, additional, Steen, HB, additional, and Iani, V, additional

Published

1995

3. Excitation of Tryptophan in Solution during Irradiation with X-Rays and UV Light between 77°K and 300°K

Author

Steen Hb

Subjects

Radiation, Ethylene, Biophysics, Analytical chemistry, Tryptophan, Phosphor, Photochemistry, Fluorescence, chemistry.chemical_compound, chemistry, Radiology, Nuclear Medicine and imaging, Irradiation, Luminescence, Phosphorescence, Excitation

Abstract

The temperature dependence of the yields of the x-ray-induced fluorescence and phosphorescence of tryptophan in ethylene glycol-water solution, between 77°K and 300°K, was found to be quite different from that observed upon excitation with non-ionizing UV light. Thus, while the quantum yields of the fluorescence and phosphorescence, induced by 270-nm UV light, were independent of the temperature up to about 220°K and 140°K, respectively, the yields of the x-ray-induced emissions decreased by more than a factor of two within the same ranges of temperature. For both types of irradiation, the phosphorescence-to-fluorescence ratio remained constant up to 140°K, being 3.6 for x-rays and 0.46 for UV light. However, the marked drop in this ratio observed, in both cases, around 160°K was much more pronounced for x-irradiation. The temperature dependence of the phosphorescence decay time was identical for the two types of irradiation. The difference between the results obtained with x-rays and UV light was attribu...

Published

1970

4. A stochastic model of cancer initiation including a bystander effect.

Author

Østby I, Øyehaug L, and Steen HB

Subjects

Cell Transformation, Neoplastic genetics, Computer Simulation, Humans, Leukoplakia, Oral genetics, Leukoplakia, Oral pathology, Mutation, Stochastic Processes, Bystander Effect, Cell Transformation, Neoplastic pathology, Leukoplakia, Oral etiology, Models, Biological

Abstract

A stochastic model of cancer initiation is considered. The model is used to evaluate whether a bystander effect may be important in the pre-malignant and malignant stages of carcinogenesis, and furthermore, on the basis of epidemiological data, to estimate the mutation rates of genes involved in the development of oral leukoplakias. The bystander effect is defined here as the capability of oncogenic mutations to increase the mutation probability of neighbouring (bystander) cells, thus leading potentially to a cascade of neighbouring mutated and neoplastic cells as a pre-stage in the development to leukoplakias and cancer. We find that incidence data for oral cancer are indeed in accordance with a significant bystander effect, operating either alone or in combination with genomic instability in the early stages of carcinogenesis, i.e. the development of neoplasia. Simulations performed gave a picture of how mutations and neoplasia may spread in a tissue, to form characteristic leukoplakias with a core of neoplastic cells. The model also showed that the probability of finding at least one neoplastic cell in the tissue after a given number of years is more sensitive to changes in genomic instability within the cell itself than to changes in a bystander effect. Based on epidemiological data we also calculate the maximum number of oncogenic genes that may be involved in the bystander effect and development of genomic instability. Even if capable of explaining the initial development of oncogenic mutations towards neoplastic cells, the bystander model could not reproduce the observed incidence rates of leukoplakia without assuming a carcinogen mutation probability per cell per year of neoplastic cells practically equal to one. This means that the bystander effect, to be of substantial importance in the final development of neoplastic cells towards leukoplakias, requires a very significant increase in mutation probabilities for bystanders to neoplastic cells. Alternatively, additional mechanisms such as abnormal cell differentiation and uncontrolled proliferation and apoptotis in the neoplastic stage may be of major importance during the development to cancerization.

Published

2006

5. Automated counting of mammalian cell colonies by means of a flat bed scanner and image processing.

Author

Dahle J, Kakar M, Steen HB, and Kaalhus O

Subjects

Algorithms, Animals, Cell Line, Cricetinae, Fibroblasts cytology, Software, Colony Count, Microbial methods, Computers, Image Processing, Computer-Assisted methods

Abstract

Background: Clonogenic assays are used frequently to measure the cell killing and mutagenic effects of radiation and other agents. Clonogenic assays carried out manually are tedious and time-consuming and involve a significant element of subjectivity. However, several commercial automatic colony counters are available. Based on CCD video imaging and image analysis they are relatively expensive and can analyze only one petri dish at a time., Method: We have developed a cheaper and more efficient device, which employs a flat bed scanner to image 12 60-mm petri dishes at a time. Two major problems in automated colony counting are the clustering of colonies and edge effects. By using standard image analysis and implementing an inflection point algorithm, these problems were greatly diminished. The resulting system was compared with two manual colony counts, as well as with automated counts with the Oxford Optronix ColCount colony counter for cell lines V79 and HaCaT., Results: Comparisons assuming the manual counts to be correct showed that our automatic counter was slightly more accurate than the commercial unit., Conclusions: As a whole, our automated colony counter performed significantly better than the commercial unit with regard to processing time, cost and accuracy.

Published

2004

6. Flow cytometer for measurement of the light scattering of viral and other submicroscopic particles.

Author

Steen HB

Subjects

Animals, Flow Cytometry instrumentation, Lasers, Light, Microspheres, Photometry, Scattering, Radiation, Viruses ultrastructure, Flow Cytometry methods, Viruses chemistry

Abstract

Background: Light scattering is an essential parameter in flow cytometry, facilitating functions such as size measurement, discrimination of cell types on the basis of shape and morphology, detection of fluorescence-negative cells, and gating of fluorescence measurements. Light scattering measurement of viruses is generally not feasible with current flow cytometers due to their small size. The problem is aggravated by the fact that the light scattering of particles in this size range (< 200 nm) falls off with roughly the sixth power of their linear dimensions., Methods: A new optical layout using darkfield illumination and detection has been developed. A 532-nm laser was used for excitation, and scattered light was collected with large aperture optics., Results: Light scattering histograms of polymer particles with diameters of 70-300 nm were recorded without gating by other parameters. By extrapolation, a detection limit of about 50 nm was obtained. Different species of virus with sizes of approximately 100 nm also were recorded., Conclusions: Flow cytometric light scattering measurement of submicroscopic particles, in a size range that includes many viral species, is now feasible. The results indicate that it may be practically impossible to measure by flow cytometry the light scattering of particles smaller than 40 nm., (Copyright 2004 Wiley-Liss, Inc.)

Published

2004

7. A sample injection device for flow cytometers.

Author

Steen HB

Subjects

Pressure, Reproducibility of Results, Flow Cytometry instrumentation

Abstract

Background: The sample injection systems of flow cytometers employ either a pressure differential between the sample vial and the sheath fluid reservoir or volumetric injection of the sample from a syringe. The pressure differential method facilitates rapid and efficient flushing to eliminate carryover between samples, but does not allow accurate determination of the rate of sample flow and cell concentration. Volumetric injection, which comprises a valve for switching the sample flow, facilitates highly accurate measurement of the cell concentration, but requires a less efficient and more time-consuming flushing procedure., Methods: Applying a removable syringe, which connects to the inlet of the sample tubing via a tight sealing, we eliminate the valve and obtain efficient flushing while maintaining the advantage of volumetric sample injection., Results: This device gives highly constant sample flow rates strictly proportional to syringe velocity over the range 0.2-50 microl/min with a settling time of about 2 sec., Conclusion: This device has the same precision as the conventional sample injection system, whereas the speed and efficiency of flushing are improved greatly., (Copyright 2002 Wiley-Liss, Inc.)

Published

2002

8. Dye exclusion artifact in flow cytometers.

Author

Steen HB and Stokke T

Subjects

Animals, Diffusion Chambers, Culture instrumentation, Diffusion Chambers, Culture methods, Diffusion Chambers, Culture standards, Flow Cytometry instrumentation, Humans, Artifacts, Flow Cytometry methods, Fluorescent Dyes

Abstract

Background: Cells exclude their own volume of dye solution in the sample flow which carries them through the flow chamber of the flow cytometer, thereby affecting the otherwise constant signal arising from the fluorescence of this solution. Under certain conditions, this phenomenon may significantly influence the fluorescence signal of the cells., Materials and Methods: Using the slit scan technique, we studied this phenomenon as observed for monodisperse polystyrene particles in fluorescein solution., Results: The measurements show that dye solution accumulates just in front of the particle and just behind it, with a relative void in between. This phenomenon is most likely caused by the rapid constriction of the flow as it enters the orifice of the nozzle or flow chamber, giving rise to a pulse of fluorescence which adds to that of the particle or cell itself. The magnitude of this artifact depends on the design and dimensions of the nozzle/flow chamber as well as on the rate of sample flow., Conclusions: The dye exclusion artifact may affect measurements of cells when they are in a dye solution having a fluorescence per unit volume which is significant compared to that of the cells, especially at low sample flow rates., (Copyright 2002 Wiley-Liss, Inc.)

Published

2002

9. Loss of chromosome 11q21-23.1 and 17p and gain of chromosome 6p are independent prognostic indicators in B-cell non-Hodgkin's lymphoma.

Author

Stokke T, DeAngelis P, Smedshammer L, Galteland E, Steen HB, Smeland EB, Delabie J, and Holte H

Subjects

Adult, Aged, Aged, 80 and over, Chromosome Aberrations, Chromosomes, Human, Pair 11 ultrastructure, Chromosomes, Human, Pair 17 ultrastructure, Chromosomes, Human, Pair 6 ultrastructure, DNA, Neoplasm genetics, Female, Flow Cytometry, Humans, Life Tables, Lymphoma, B-Cell classification, Lymphoma, B-Cell mortality, Lymphoma, B-Cell pathology, Male, Middle Aged, Nucleic Acid Hybridization, Prognosis, Retrospective Studies, Risk, Risk Factors, S Phase, Survival Analysis, Translocation, Genetic, Chromosome Deletion, Chromosomes, Human, Pair 11 genetics, Chromosomes, Human, Pair 17 genetics, Chromosomes, Human, Pair 6 genetics, Lymphoma, B-Cell genetics

Abstract

Comparative genomic hybridization (CGH) was employed to study chromosomal aberrations in relation to cell proliferation, apoptosis, and patient survival in 94 cases of B-cell non-Hodgkin's lymphoma diagnosed between 1983 and 1993. Eighty cases had aberrations by CGH. Chromosomal regions 1p21-31.1 (10%), 6cen-q24 (12%), 8p (11%), 9p21-ter (14%), 11q21-23.1 (11%), 13q13-21.1 (12%), and 17p (15%) were frequently lost. Gains were found at 3q21-ter (22%), 6p (11%), 7p (12%), 8q23-ter (13%), 12cen-q15 (17%), 17q24-ter (13%), and 18q13.3-21 (20%). A high number of aberrations (> or = 4, 33 cases) was associated (P < or = 0.001) with the mantle cell and diffuse large B-cell lymphoma subtypes, a high fraction of tumour cells in S phase, and short survival (RR (relative risk) = 3.7). Loss of 1p21-31.1, 8p, 9p21-ter, 11q21-23.1, and 13q13-21.1 were associated with mantle cell lymphoma (P < or = 0.03), while gain of 6p and 12cen-q15 were more frequent in diffuse large B-cell and small lymphocytic lymphoma, respectively (P = 0.04). Loss of 8p and 17p, and gain of 3q21-ter, 6p, 7p, and 8q23-ter were associated with a high S phase fraction (P < or = 0.03), but none of the aberrations were associated with tumour apoptotic fraction (P > or = 0.13). The most important prognostic CGH parameters (P < 0.001) were losses of 11q21-23.1 (RR = 3.8) and 17p (RR = 4.4), and gain of 6p (RR = 4.2). The latter parameters and IPI were the only ones with independent prognostic value (RR = 10, 5.0, 6.7, and 3.7, respectively; P < 0.001) when assessed together with lymphoma sub-type, primary versus relapse cases, treatment, B symptoms, S phase fraction, and presence of BCL1 and BCL2 translocations. A combined CGH/IPI binary parameter had high prognostic value for patients receiving different treatments, with various lymphoma sub-types, and for primary as well as relapse cases.

Published

2001

10. Flow cytometers for characterization of microorganisms.

Author

Steen HB

Subjects

Cell Cycle, Cell Separation instrumentation, Equipment Design, Fluorescent Dyes, Lasers, Light, Models, Statistical, Reproducibility of Results, Scattering, Radiation, Bacteria cytology, Cell Separation methods, Flow Cytometry instrumentation, Flow Cytometry methods

Abstract

The measurement of microbes is an increasingly important application in flow cytometry. The small size of these organisms can create special difficulties for instruments designed to analyze much larger eukaryotic cells. This unit describes the problems encountered in making microbiological measurements, the instrument requirements, and some approaches that can be taken to optimize the instrument. This material is essential background for the protocols found in chapter 11, Microbiological Applications.

Published

2001

11. Bystander effects in cell death induced by photodynamic treatment UVA radiation and inhibitors of ATP synthesis.

Author

Dahle J, Angell-Petersen E, Steen HB, and Moan J

Subjects

Algorithms, Animals, Carbonyl Cyanide m-Chlorophenyl Hydrazone toxicity, Cell Communication, Cell Death drug effects, Cell Death radiation effects, Cells, Cultured, Deoxyglucose toxicity, Disease Models, Animal, Dogs, Kidney anatomy & histology, Kidney drug effects, Kidney radiation effects, Photochemistry, Adenosine Triphosphate metabolism, Cell Death physiology, Dihematoporphyrin Ether toxicity, Photosensitizing Agents toxicity, Ultraviolet Rays adverse effects

Abstract

Confluent layers of MDCK II cells were treated with four different photosensitizers (a purified version of hematoporphyrin derivative [Photofrin], tetra(3-hydroxyphenyl)porphine [3-THPP], meso-tetra(4-sulphonatophenyl)porphine [TPPS4] and ALA-induced Protoporphyrin IX) and irradiated with blue light, with UVA without exogenous photosensitizers, or incubated with the metabolic inhibitors carbonyl cyanide m-chlorophenylhydrazone and 2-deoxy-D-glucose. Necrotic and apoptotic cells were detected about 4 h later by fluorescence microscopy. Dead cells appeared in distinct clusters in the confluent layers. The number of dead cells in these clusters was determined by manual counting and image analysis. Forty-one of the 43 experimental distributions of dead cells in clusters were found to be significantly different from a Monte Carlo simulation of the distribution of independently inactivated cells. However, a Monte Carlo simulation model, assuming that each dead cell increased the probability of inactivation of adjacent cells, fitted 34 of the 43 observed distributions of dead cells in clusters, indicating a significant bystander effect for all the investigated treatments. The bystander-effect model parameter, defined as a cell's increase in probability of dying when it has dead neighbors, was significantly lower for 3-THPP-PDT and TPPS4-PDT than for Photofrin-PDT, ALA-PDT and treatment with metabolic inhibitors.

Published

2001

12. Intracellular localisation of hypericin in human glioblastoma and carcinoma cell lines.

Author

Uzdensky AB, Ma LW, Iani V, Hjortland GO, Steen HB, and Moan J

Subjects

Anthracenes, Colonic Neoplasms, Female, Humans, Tumor Cells, Cultured, Uterine Cervical Neoplasms, Adenocarcinoma metabolism, Carcinoma in Situ metabolism, Glioblastoma metabolism, Perylene analogs & derivatives, Perylene pharmacokinetics, Radiation-Sensitizing Agents pharmacokinetics

Abstract

Hypericin, a natural polycyclic quinone extracted from Hypericum perforatum, has been recently shown to be a powerful sensitiser for photodynamic therapy (PDT). However, its intracellular localisation remains unclear and contradictory. In the present work we compared the intracellular localisation of hypericin in three cultured cell lines (adenocarcinoma cells WiDr, carcinoma cells NHIK 3025 and glioblastoma cells D54Mg) with the distribution of fluorescent probes specific to lysosomes (LysoTracker Blue DND-22), mitochondria (MitoTracker Green FM) and endoplasmic reticulum (ERTracker Blue-White DPX). It was shown that the hypericin staining pattern was different compared to the intracellular distribution of mitochondria or lysosomes. Hypericin was concentrated in the perinucleolar cytoplasmic area mainly on one side of the nucleus--the region rich in endoplasmic reticulum and Golgi. Sometimes nuclear envelope was also stained. Plasma membrane was not stained but the dye was often accumulated in the intercellular space between the tightly contacting WiDr cells in colonies. Hypericin concentrations of 10 microM or less were not toxic for WiDr cells in the dark. Orange light (lambda max approximately 600 nm; 6 mW/cm2) killed the cells stained with 1 microM hypericin with LD50 approximately 1 J/cm2.

Published

2001

13. Flow cytometric monitoring of bacterial susceptibility to antibiotics.

Author

Walberg M and Steen HB

Subjects

Anti-Bacterial Agents pharmacokinetics, Bacteria growth & development, Bacteria metabolism, Cell Wall metabolism, DNA, Bacterial metabolism, Humans, Microbial Sensitivity Tests, Time Factors, Anti-Bacterial Agents pharmacology, Bacteria drug effects, Flow Cytometry methods, Fluorescent Dyes metabolism

Published

2001

14. Staining and measurement of DNA in bacteria.

Author

Steen HB

Subjects

Bacteria metabolism, Cell Wall metabolism, DNA, Bacterial chemistry, Enzyme Inhibitors pharmacology, Ethanol chemistry, Ethidium metabolism, Fixatives chemistry, Flow Cytometry instrumentation, Flow Cytometry standards, Fluorescent Dyes metabolism, Plicamycin metabolism, Rifampin pharmacology, Bacteria chemistry, DNA, Bacterial analysis, Flow Cytometry methods, Staining and Labeling methods

Published

2001

15. The origin of oncogenic mutations: where is the primary damage?

Author

Steen HB

Subjects

Animals, Humans, Neoplasms epidemiology, Neoplasms genetics, Cell Transformation, Neoplastic genetics, Models, Biological, Mutation, Oncogenes genetics

Abstract

Cancer is generally believed to arise from a single cell which has become 'initiated' by mutation of a few crucial genes, caused by random 'hits' in its DNA, a 'hit' being an error in DNA replication or a reaction of the DNA with free radicals or other chemical species of exogenous or endogenous origin. It is not obvious how the epidemiological data on cancer incidence can be interpreted within the framework of this paradigm. For example, it cannot account quantitatively for the age dependence of cancer incidence, or for the fact that the incidence of cancer in people with hereditary mutations in tumour suppressor genes is much lower than expected, or for the observation that while in some types of cancer, like colon and pancreas, certain highly oncogenic mutations, such as that of TP53, are prevalent, there is no significant increase in the incidence of these cancers in people who carry the mutations by heredity. It is argued here that although mutations in such genes appear to be of crucial importance in carcinogenesis they may not be the rate limiting events in common cancer. The epidemiological data are consistent with the hypothesis that the rate limiting processes involve large numbers of cells. Conceivably, the mutations directly underlying neoplastic transformation may be the result of a local collapse in the system of intercellular processes on which the stability of the normal genotype and phenotype depends, and thereby trigger a cascade of mutations, among them the highly oncogenic ones. This local collapse may be due to mutations of many different genes in many cells as well as to other factors affecting the integrity of tissue.

Published

2000

16. Flow cytometry of bacteria: glimpses from the past with a view to the future.

Author

Steen HB

Subjects

Escherichia coli growth & development, Forecasting, History, 20th Century, Humans, Bacteria growth & development, Bacteriological Techniques history, Bacteriological Techniques trends, Flow Cytometry history, Flow Cytometry trends

Abstract

Measurement of bacteria and other microorganisms at the level of single cells has progressed enormously over the last couple of decades. Up to the late 1970s, there were no other means than microscopy for observation of single microorganisms, making any type of measurement very cumbersome and tedious, at best. Today, we measure several parameters simultaneously with a precision of a few per cent, and at a rate of 1000 cells per second. The first papers on the use of flow cytometry to measure bacteria appeared only in 1977, although the method had proved highly successful in studies of mammalian cells for almost a decade. There were several reasons for this relatively late introduction, including technical limitations, problems with adequate staining, and, not least, the human factor. Today, flow cytometry has a wide range of microbiological applications, ranging from studies of the bacterial cell cycle and many other cellular characteristics to assessment of antibiotic susceptibility of clinical samples, and monitoring of bacteria and other microorganisms in anything from sewage to sea water. Still, the potential of flow cytometry in microbiology is far from fully utilised. Better instruments and new stains will provide new opportunities to understand, control and exploit this vital part of the biosphere.

Published

2000

17. Gap junctional intercellular communication is not a major mediator in the bystander effect in photodynamic treatment of MDCK II cells.

Author

Dahle J, Mikalsen SO, Rivedal E, and Steen HB

Subjects

Animals, Cell Death drug effects, Cell Death radiation effects, Cell Line drug effects, Cell Line radiation effects, Dieldrin pharmacology, Dihematoporphyrin Ether radiation effects, Dogs, Epithelial Cells radiation effects, Gap Junctions drug effects, Kidney, Monte Carlo Method, Oxidative Stress, Phosphorylation drug effects, Phosphorylation radiation effects, Photochemistry, Protein Processing, Post-Translational drug effects, Protein Processing, Post-Translational radiation effects, Cell Communication drug effects, Computer Simulation, Dihematoporphyrin Ether pharmacology, Epithelial Cells drug effects, Gap Junctions physiology, Models, Biological, Photochemotherapy, Photosensitizing Agents pharmacology

Abstract

Photodynamic treatment (PDT) of confluent MDCK II cells resulted in a noticeable clustering of dead cells, consistent with a significant bystander effect. Likewise, PDT of cells in microcolonies resulted in an overabundance of microcolonies that had responded to the treatment as a single unit, that is, in which either all or no cells were dead. Confluent MDCK II cells appeared to communicate via gap junction channels, while cells in microcolonies did not. Monte Carlo simulation models were fitted to the distributions of dead cells in confluent monolayers and in microcolonies. The simulations showed that the degree of the bystander effect was higher in microcolonies than in confluent cells, suggesting that gap junction communication may be involved in the bystander effect. However, when the gap junction hypothesis was tested by treatment of microcolonies with 30 microM dieldrin, an inhibitor of gap junctional intercellular communication, there was no reduction of the bystander effect, indicating that this effect was not mediated by gap junctional intercellular communication. PDT influenced phosphorylation of tyrosine residues in several proteins in the cells. Protein phosphorylation is important in cellular signaling pathways and may be involved in the bystander effect, for example by influencing the mode of cell death.

Published

2000

18. The bystander effect in photodynamic inactivation of cells.

Author

Dahle J, Bagdonas S, Kaalhus O, Olsen G, Steen HB, and Moan J

Subjects

Animals, Cell Communication, Cell Line pathology, Dihematoporphyrin Ether pharmacology, Dogs, Dose-Response Relationship, Drug, Flow Cytometry, Fluorescent Antibody Technique, Light, Necrosis, Photochemotherapy, Apoptosis, Cell Line drug effects, Porphyrins pharmacology, Radiation-Sensitizing Agents pharmacology

Abstract

Treatment of MDCK II cells with the lipophilic photosensitizer tetra(3-hydroxyphenyl)porphyrin and light was found to induce a rapid apoptotic response in a large fraction of the cells. Furthermore, the distribution of apoptotic cells in microcolonies of eight cells was found to be different from the binomial distribution, indicating that the cells are not inactivated independently, but that a bystander effect is involved in cell killing by photodynamic treatment. The observation of a bystander effect disagrees with the common view that cells are inactivated only by direct damage and indicates that communication between cells in a colony plays a role in photosensitized induction of apoptosis. The degree of bystander effect was higher for cells dying by necrosis than for cell dying by apoptosis.

Published

2000

19. Oncogenic aberrations in the p53 pathway are associated with a high S phase fraction and poor patient survival in B-cell Non-Hodgkin's lymphoma.

Author

Stokke T, Galteland E, Holte H, Smedshammer L, Suo Z, Smeland EB, Børresen-Dale AL, DeAngelis P, and Steen HB

Subjects

Adult, Aged, Aged, 80 and over, Alleles, Antineoplastic Combined Chemotherapy Protocols therapeutic use, Apoptosis genetics, Exons, Female, Gene Deletion, Gene Expression, Humans, In Situ Hybridization, Fluorescence, Lymphoma, B-Cell drug therapy, Lymphoma, B-Cell pathology, Male, Middle Aged, Mutation, Missense, Phenotype, Point Mutation, Prognosis, Retrospective Studies, Survival Analysis, Treatment Outcome, Tumor Suppressor Protein p53 biosynthesis, Tumor Suppressor Protein p53 genetics, Tumor Suppressor Protein p53 physiology, Genes, p53 genetics, Lymphoma, B-Cell genetics, S Phase genetics

Abstract

The implications of aberrations in the p53 pathway for induction of apoptosis and regulation of S phase entry, and for patient survival, were investigated in 83 B-cell Non-Hodgkin's lymphomas. Eight cases had missense mutations in exons 5, 7, 8 and 9 as revealed by constant denaturant gel electrophoresis and sequencing. Fifteen cases had lost 1 TP53 allele as revealed by fluorescent in situ hybridization and comparative genomic hybridization. Ten cases expressed high levels of p53 as assessed by immunoblotting and immunohistochemistry. S phase fractions were higher, apoptotic fractions were the same and survival times were shorter in all aberration groups compared with the cases with no TP53/p53 aberrations. Since many tumors had more than one TP53/p53 aberration, the tumors were divided into groups with the following characteristics: no TP53/p53 aberrations; loss of one TP53 allele only (9 cases), TP53 point mutation (8 cases), high-level p53 expression and no TP53 mutation (3 cases). Tumors from the 3 latter groups had higher median S phase fractions (5%, 7.6%, and 5%, respectively, p<0.02) than the cases without any aberrations (1.1%), and survival time for these patients was much shorter (relative risks of 5.9, 8.9, and 6.6, respectively, p<0.003). Apoptotic fractions were similar in all these groups (p=0.09). Multivariate analysis showed that the presence of TP53/p53 aberrations is a strong and independent prognostic parameter in B-cell Non-Hodgkin's lymphoma., (Copyright 2000 Wiley-Liss, Inc.)

Published

2000

20. Photodynamic therapy of superficial basal cell carcinoma with 5-aminolevulinic acid with dimethylsulfoxide and ethylendiaminetetraacetic acid: a comparison of two light sources.

Author

Soler AM, Angell-Petersen E, Warloe T, Tausjø J, Steen HB, Moan J, and Giercksky KE

Subjects

Female, Humans, Male, Middle Aged, Aminolevulinic Acid therapeutic use, Carcinoma, Basal Cell drug therapy, Dimethyl Sulfoxide therapeutic use, Edetic Acid therapeutic use, Light, Photochemotherapy adverse effects, Skin Neoplasms drug therapy

Abstract

The aim of this prospective randomized study was to compare the clinical and cosmetic outcome of superficial basal cell carcinomas (BCC), using either laser or broadband halogen light, in photodynamic therapy with topical 5-aminolevulinic acid (ALA). A total of 83 patients with 245 superficial BCC were included in the study. Standard treatment involved 15 min of local pretreatment with 99% dimethylsulfoxide (DMSO) before topical application of 20% ALA with DMSO (2%) and ethylendiaminetetraacetic acid (2%) as cofactors for 3 h before light exposure with either laser or a broadband lamp (BL). A complete response was achieved in 95 lesions (86%) in the laser group and 110 lesions (82%) in the BL group 6 months after treatment. Of these, 80 lesions (84%) in the laser group and 101 lesions (92%) in the lamp group were independently evaluated to have an excellent or good cosmetic post-treatment score. No serious adverse events were reported. This study shows that there is no statistical significant difference in cure the rate (P = 0.49) and the cosmetic outcome (P = 0.075) with topical application of a modified ALA-cream between light exposure from a simple BL with continuous spectrum (570-740 nm) or from a red-light laser (monochromatic 630 nm). Cost and safety are further elements in favor of the BL in this setting.

Published

2000

21. A new alpha-particle irradiator with absolute dosimetric determination.

Author

Soyland C, Hassfjell SP, and Steen HB

Subjects

Air, Beta Particles, Bismuth, Cells, Cultured radiation effects, Equipment Design, Humans, Lead Radioisotopes, Linear Energy Transfer, Lung cytology, Lung radiation effects, Polyethylene Terephthalates radiation effects, Radiation Protection methods, Radiometry methods, Spectrum Analysis, Thorium, Alpha Particles, Cell Culture Techniques instrumentation, Cells radiation effects, Radiometry instrumentation

Abstract

A new experimental setup for uniform alpha-particle irradiation of cells in vitro is described. The alpha-particle irradiator is based on a radioactive (212)Pb/(212)Bi source. In the experimental setup proposed, cells are grown directly on a polylysine-coated track-etch material that forms the base of custom-made cell dishes. Alpha-particle irradiation is done through the base of the dish. Immediately prior to irradiation, the cell dish is scanned under a microscope, and images of cells with the corresponding coordinates are saved. After irradiation and after the biological end point under study has been determined, the cell dish is etched to develop alpha-particle tracks in the dish base. A microscope image series of alpha-particle track images is obtained by accurately revisiting every original (preirradiation) cell position in the track-etched dish. The number of alpha-particle traversals of each individual cell is scored by mapping images of alpha-particle tracks onto the images of cells recorded prior to irradiation. The uncertainty of the alpha-particle hit determination is 0.9 microm. The procedure described thus presents a method for radiobiological experiments with absolute, rather than statistical, cell dosimetry.

Published

2000

22. The mode of cell death induced by photodynamic treatment depends on cell density.

Author

Dahle J, Steen HB, and Moan J

Subjects

Animals, Apoptosis drug effects, Apoptosis physiology, Cell Count, Cell Death drug effects, Cell Line, Dogs, Kidney cytology, Kidney drug effects, Porphyrins toxicity, Radiation-Sensitizing Agents toxicity, Cell Death physiology, Photochemotherapy methods

Abstract

Madison Darby canine kidney II (MDCK II) cells were seeded out at two different densities and incubated with 125 micrograms/mL of the photosensitizer meso-tetra(4-sulfonatophenyl)porphine (TPPS4) for 18 h, washed and irradiated with blue light. Four hours later the cells were studied by fluorescence microscopy. Apoptotic cells were detected by virtue of the distinct condensation and fragmentation of chromatin, and necrotic cells were detected by uptake of propidium iodide. In addition apoptosis was measured by the TdT assay. The fraction of apoptotic cells and the fraction of necrotic cells were determined for both cell densities at various levels of survival. With < 55% total cell death the apoptotic fraction was significantly higher for cells in confluent monolayers than for cells growing in microcolonies at equitoxic doses. Confluent cells were 2.9 times more sensitive than cells in microcolonies partly due to a 1.5 times higher uptake of TPPS4 in monolayer cells. The difference in mode of cell death for the different cell densities was not related to any observable difference in subcellular localization pattern of TPPS4 at equitoxic doses of photodynamic treatment.

Published

1999

23. Uptake kinetics of nucleic acid targeting dyes in S. aureus, E. faecalis and B. cereus: a flow cytometric study.

Author

Walberg M, Gaustad P, and Steen HB

Subjects

Bacillus cereus growth & development, Bacillus cereus metabolism, Cold Temperature, Enterococcus faecalis growth & development, Enterococcus faecalis metabolism, Kinetics, Nucleic Acids metabolism, Staphylococcus aureus growth & development, Staphylococcus aureus metabolism, Flow Cytometry methods, Fluorescent Dyes metabolism, Gram-Positive Bacteria metabolism

Abstract

For flow cytometry-based detection as well as susceptibility testing and counting, staining of the bacterial cells is essential. In an attempt to develop rapid preparatory procedures for nucleic acid staining of wild type Gram positive bacteria, the uptake of fluorescent dyes in viable S. aureus, E. faecalis, and B. cereus cells was studied by flow cytometry under conditions intended to block probe efflux and increase cell wall permeability. The aim of the study was to develop procedures which allow rapid nucleic acid staining independent of fixation, since ethanol fixation is time-consuming and may mask phenomena associated with viability and lead to uncontrolled loss and aggregation of cells. The dye uptake was measured repeatedly after treating cells with metabolic inhibitors in order to block probe efflux, or cold shock (0 degree C) to increase permeability. The probes used were mithramycin (Mi), ethidium bromide (EB), DAPI, Hoechst 33342 and Hoechst 33258. None of the procedures facilitated uptake of the dyes to a level similar to that obtained in fixed control cells in all of the species. After metabolic inhibition of B. cereus cells, DAPI and Hoechst fluorescence increased to a level similar to or above that found in fixed cells, indicating that the uptake of these dyes is limited by energy-dependent efflux. A similar increase of DAPI fluorescence was observed after cold shock suggesting the uptake of this dye to be limited also by permeability in B. cereus. The Mi and EB fluorescence increased to the level of the fixed control cells under all conditions tested, suggesting free probe influx in this species. Generally, probe uptake in S. aureus and E. faecalis was lower than in B. cereus cells, and no permeabilizing effect of cold shock was observed. In some experiments the fluorescence exceeded that of ethanol fixed control cells, indicating that the fixation may cause conformational changes in DNA.

Published

1999

24. Propidium iodide quenches the fluorescence of TdT-incorporated FITC-labeled dUTP in apoptotic cells.

Author

Stokke T, Solberg K, DeAngelis P, and Steen HB

Subjects

Flow Cytometry methods, Fluorescence, HL-60 Cells, Humans, Apoptosis, DNA Nucleotidylexotransferase metabolism, Deoxyuracil Nucleotides metabolism, Fluorescein-5-isothiocyanate, Fluorescent Dyes, Propidium

Abstract

Apoptotic cells with frequent DNA strand breaks may be detected by tagging with directly or indirectly labeled nucleotides incorporated by the use of terminal deoxynucleotidyl transferase (TdT). Propidium iodide (PI) is typically added for the simultaneous assessment of DNA content. PI was found to quench the specific in situ FITC-fluorescence of apoptotic cells which were labeled by TdT with FITC-conjugated dUTP, biotin-dUTP followed by streptavidin-FITC, or digoxigenin-dUTP followed by FITC-labeled anti-digoxigenin antibodies as measured by flow cytometry. The effect was concentration-dependent, with 50% quenching occurring at 0.8 microg/ml, 1.5 microg/ml, and 5 microg/ml PI, respectively, at approximately 1 x 10(6) cells/ml. Spectrofluorimetry in solution revealed that 15 microg/ml PI was required to quench 50% of the fluorescence of ss FITC-labeled poly(dU)35. In contrast, the fluorescence of ds FITC-labeled poly(dU)35-poly(dA) was quenched to 50% at 3 microg/ml PI. The maximum of the fluorescence excitation spectrum of PI shifted from 490 nm to 535 nm upon binding to ds DNA as well as ss poly(dU)35, and the fluorescence yield of PI at 610 nm increased, but the binding required 10-fold higher concentrations of poly(dU)35 as compared to ds DNA. The spectroscopic properties of PI are therefore similar whether bound to poly(dU) or to double-stranded DNA, but the binding to poly(dU) is much weaker. The observed quenching in situ therefore cannot be explained by direct binding of PI to the poly(dU) tails synthesized by TdT in situ in apoptotic cells, but may rather be due to radiationless energy transfer from FITC to PI bound to double-stranded DNA close to the nicks where TdT is known to start polymerization.

Published

1998

25. Protoporphyrin IX accumulation in cells treated with 5-aminolevulinic acid: dependence on cell density, cell size and cell cycle.

Author

Moan J, Bech O, Gaullier JM, Stokke T, Steen HB, Ma LW, and Berg K

Subjects

Adenocarcinoma metabolism, Adenocarcinoma pathology, Animals, Cell Line drug effects, Colonic Neoplasms metabolism, Colonic Neoplasms pathology, Cricetinae, Cricetulus, Fibroblasts drug effects, Fibroblasts metabolism, Fibroblasts pathology, Humans, Tumor Cells, Cultured drug effects, Aminolevulinic Acid pharmacology, Cell Communication, Cell Count, Cell Cycle, Protoporphyrins biosynthesis

Abstract

Human colon adenocarcinoma cells (WiDr) and Chinese hamster lung fibroblasts cells (V79) were incubated with different concentrations of 5-aminolevulinic acid (ALA), and the production of protoporphyrin IX (PpIX) was studied using several techniques. The amount of PpIX produced per cell increased with increasing ALA concentration according to different kinetics for the 2 cell lines. For both cell lines a cell density dependency of the PpIX synthesis was observed. For saturating ALA concentrations, 2-3 times more PpIX was produced per cell at a density of 5 x 10(4) than at a density of 5 x 10(3) cells/cm2. The photosensitivity of cells appeared to increase even more than the PpIX content, indicating a cooperative effect in inactivation. The PpIX production rate increased with cell size and was about 1.9 times higher for cells in the G2 + M phase than for cells in the G1 phase of the cell cycle. Neither cell size nor cell cycle distribution were significantly dependent on cell density.

Published

1998

26. Rapid discrimination of bacterial species with different ampicillin susceptibility levels by means of flow cytometry.

Author

Walberg M, Gaustad P, and Steen HB

Subjects

Escherichia coli isolation & purification, Fluorescence, Klebsiella pneumoniae isolation & purification, Microbial Sensitivity Tests methods, Scattering, Radiation, Ampicillin Resistance, Escherichia coli drug effects, Flow Cytometry methods, Klebsiella pneumoniae drug effects

Abstract

An in vitro model for flow cytometric detection of heterogeneous drug response in exponentially growing Escherichia coli and Klebsiella pneumoniae was studied to evaluate the potential of this technology for rapid antibiotic susceptibility testing in polymicrobial samples. The cells, which exhibited 80-fold difference in in ampicillin susceptibility, were cultivated in the presence of ampicillin at a concentration equaling 1 MIC of the low-susceptibility strain (E. coli). Prior to flow cytometric analysis, the cells were fixed in 70% ethanol and stained with a DNA-specific dye. After 1 h of ampicillin incubation, the light scattering and fluorescence intensities of the susceptible cells increased 4.3-fold and 5-fold, respectively, but remained about constant for the resistant cells. The corresponding cell number increase for the resistant and the susceptible cells was 9.4 and 1.7, respectively. The two strains could be distinguished in the histograms on the basis of their light scattering and fluorescence intensities and by cell number. With an incubation of up to 3 h, the light scattering and fluorescence intensities of the susceptible cells grew stronger, at the expense of cell number. By combination of histograms, the discrimination of different cell populations could be improved. The results demonstrate the ability of flow cytometry to discriminate between species in heterogeneous cultures and suggest the potential of the technique for rapid assessment of bacterial susceptibility. However, the present results are preliminary, and the application to biological liquids and clinical samples has to be demonstrated further.

Published

1997

27. Uncoupling of the order of the S and M phases: effects of staurosporine on human cell cycle kinases.

Author

Stokke T, Smedshammer L, Jonassen TS, Blomhoff HK, Skarstad K, and Steen HB

Subjects

Cell Cycle drug effects, Cell Division drug effects, Cell Nucleus drug effects, Cells, Cultured, DNA analysis, DNA metabolism, Fibroblasts drug effects, Genes, p53, Humans, Meiosis, Mitosis drug effects, Models, Biological, Neoplasms metabolism, Polyploidy, Retinoblastoma enzymology, Retinoblastoma Protein genetics, Retinoblastoma Protein metabolism, S Phase drug effects, Tumor Cells, Cultured, Fibroblasts cytology, Fibroblasts enzymology, Protein Kinases metabolism, Staurosporine pharmacology

Abstract

The protein kinase inhibitor staurosporine (SSP) was employed to study the involvement of kinases in human cell cycle progression. Thirty to 100 ng/ml SSP blocks entry into S phase and M phase. Lack of entry into S phase is due to impaired activity of the retinoblastoma protein kinase. The requirement for any of the SSP-sensitive kinases for cell cycle progression can be abrogated in tumour cells. Therefore, these kinases act in a checkpoint network negatively controlling the initiation of S phase, M phase and cytokinesis, rather than being inherent parts of a substrate-product chain required for the initiation of the cell cycle phases. As a consequence of the lack of certain checkpoint effectors, tumour cells may endoreduplicate or binucleate in the presence of SSP. The latter processes, as well as meiosis, are naturally occurring in specialized cell types, leading to the idea that this checkpoint network controls the order of the cell cycle phases in normal cells. A model is presented where the cell cycle is envisioned as two independently running cycles, the S and the M cycle, which are controlled by intra and intercycledependent checkpoints in human somatic cells. The model accounts for the dependency of S and M phase initiation on the successful completion of the previous M and S phase, respectively, as well as entry into a resting state.

Published

1997

28. Cooperative effects of photodynamic treatment of cells in microcolonies.

Author

Dahle J, Kaalhus O, Moan J, and Steen HB

Subjects

Animals, Bromodeoxyuridine metabolism, CHO Cells, Cell Line, Cricetinae, DNA Nucleotidylexotransferase analysis, DNA Nucleotidylexotransferase metabolism, Dogs, Microscopy, Fluorescence, Models, Biological, Probability, S Phase physiology, Cell Communication, Cell Death, Hematoporphyrin Derivative pharmacology, Light, Photosensitizing Agents pharmacology

Abstract

Microcolonies of 2-8 Madison-Darby canine kidney cells (MDCK II) and Chinese hamster lung fibroblasts (V79) cells were incubated with the photosensitizer Photofrin and exposed to light, and the resulting number of dead cells per colony was determined. The distribution of this number was found to be incompatible with the assumption that cells are inactivated independently. The experimental distributions were significantly different from the binomial distribution expected from this assumption, but in accordance with a model in which an inactivated cell can inactivate adjacent cells with a certain probability. These findings are contrary to the common view that damage caused by radiation is limited to the cell in which the primary damage takes place. Our findings clearly indicate some kind of cooperativity between cells treated with Photofrin and light.

Published

1997

29. Rapid assessment of ceftazidime, ciprofloxacin, and gentamicin susceptibility in exponentially-growing E. coli cells by means of flow cytometry.

Author

Walberg M, Gaustad P, and Steen HB

Subjects

Colony Count, Microbial, Escherichia coli growth & development, Ethidium chemistry, Fluorescent Dyes chemistry, Microbial Sensitivity Tests, Anti-Bacterial Agents pharmacology, Ceftazidime pharmacology, Ciprofloxacin pharmacology, Escherichia coli drug effects, Flow Cytometry methods, Gentamicins pharmacology

Abstract

Exponentially growing E. coli cells were cultivated in the presence of ceftazidime, ciprofloxacin, and gentamicin in concentrations ranging from 0.5-8 minimal inhibitory concentration (MIC), permeabilized by means of cold shock in EDTA/azide, and stained with the DNA-specific dye combination of ethidium bromide and mithramycin before the fluorescence, light scattering, and cell number were measured flow-cytometrically. In order to evaluate the applicability of the cold-shock procedure, cells were also permeabillized by 70% ethanol. Permeabilization by cold shock, which eliminates washing of the cells, reduced the preparation time to <5 min. A statistically significant increase in light scattering and fluorescence, i.e., cell size and DNA content, could be detected already after 30 min of ceftazidime and ciprofloxacin exposure, even at sub-MIC concentrations. The results obtained with these drugs with cold-shock permeabilization were similar to those seen with ethanol fixation. For gentamicin-treated cells, however, a majority of the cells lost their fluorescence after cold shock. In gentamicin-treated cells fixed in ethanol, there was no consistent effect on either light scattering or fluorescence; however, we observed a substantial fragmentation and leakage of DNA in such cells. The cell proliferation was completely inhibited within 30 min of gentamicin incubation. For all three drugs, loss of light scattering and DNA were associated with cellular disintegration, i.e., reduced viability. The present results demonstrate that effects of ceftazidime, ciprofloxacin, and gentamicin on E. coli can be detected by flow cytometry within 1 h from the beginning of drug exposure to the completed measurement.

Published

1997

30. Build-up of esterified aminolevulinic-acid-derivative-induced porphyrin fluorescence in normal mouse skin.

Author

Peng Q, Moan J, Warloe T, Iani V, Steen HB, Bjørseth A, and Nesland JM

Subjects

Aminolevulinic Acid analogs & derivatives, Animals, Esterification, Female, Fluorescence, Mice, Mice, Inbred BALB C, Mice, Nude, Aminolevulinic Acid metabolism, Porphyrins metabolism, Skin metabolism

Published

1996

31. Rapid flow cytometric assessment of mecillinam and ampicillin bacterial susceptibility.

Author

Walberg M, Gaustad P, and Steen HB

Subjects

Cell Division drug effects, DNA, Bacterial chemistry, DNA, Bacterial drug effects, Escherichia coli cytology, Escherichia coli drug effects, Escherichia coli genetics, Fluorescence, Time Factors, Amdinocillin pharmacology, Ampicillin pharmacology, Flow Cytometry methods, Microbial Sensitivity Tests methods

Abstract

The effects of antibiotics on Escherichia coli during exponential growth in liquid medium were monitored by flow cytometry measuring cellular DNA content and cell size of individual cells in large numbers as well as cell counts. A statistically significant increase in cellular DNA as well as size was recorded after 20 and 40 min of incubation with the MIC of ampicillin and mecillinam, respectively. The optical density (OD600nm) of treated cultures continued to increase for at least 80 minutes, showing that the increase in cellular DNA and size reflected continued growth and elongation of cells coupled with inhibition of cell division, the latter being confirmed by the cell counting. Since fixation, staining and flow-cytometric analysis can be carried out within a few minutes, the present results suggest that flow cytometry may have potential as a rapid and quantitative technique that can be automated for clinical and experimental susceptibility testing of antibacterial drugs.

Published

1996

32. Distribution of 5-aminolevulinic acid-induced porphyrins in noduloulcerative basal cell carcinoma.

Author

Peng Q, Warloe T, Moan J, Heyerdahl H, Steen HB, Nesland JM, and Giercksky KE

Subjects

Adult, Aged, Aged, 80 and over, Carcinoma, Basal Cell metabolism, Dimethyl Sulfoxide pharmacology, Humans, Microscopy, Fluorescence, Middle Aged, Photochemotherapy methods, Skin Neoplasms metabolism, Aminolevulinic Acid pharmacology, Carcinoma, Basal Cell drug therapy, Porphyrins metabolism, Skin Neoplasms drug therapy

Abstract

Microscopic fluorescence photometry incorporating a light-sensitive thermo-electrically cooled charge-coupled device (CCD) camera was employed to investigate the fluorescence distribution of 5-aminolevulinic acid (ALA)-induced porphyrins in 22 patients with a total number of 52 noduloulcerative basal cell carcinomas (BCC) after topical ALA application with or without dimethylsulfoxide (DMSO)/ethylenediaminetetraacetic acid (EDTA) or after intravenous administration of ALA. Both localization patterns and amounts of ALA-induced porphyrins in the BCC were studied. The ALA-induced porphyrins were localized only in the superficial layers of the noduloulcerative BCC lesions after topical application of 20% ALA alone for 3 h. However, both the penetration of ALA into deep lesions and the production of the ALA-induced porphyrin fluorescence were increased after topical administration of 20% ALA and 20% DMSO/4% EDTA for 3 h. Prior treatment with 99% DMSO for 15 min further enhanced the ALA penetration into the BCC lesions after topical application of the ALA/DMSO/EDTA mixture and produced more ALA-induced porphyrins by a factor of about three compared with those treated with ALA alone. The penetration of ALA into the deep BCC lesions could also be increased by prolonging the time of topical application of 20% ALA/4% EDTA to 29-48 h (without DMSO). Intravenous injection of ALA led to a more homogeneous distribution of the ALA-derived porphyrins in the whole noduloulcerative BCC lesions.

Published

1995

33. SYBR green I DNA staining increases the detection sensitivity of viruses by polymerase chain reaction.

Author

Karlsen F, Steen HB, and Nesland JM

Subjects

Benzothiazoles, Diamines, Ethidium, Humans, Papillomaviridae genetics, Quinolines, Sensitivity and Specificity, Tumor Cells, Cultured, DNA, Viral analysis, Fluorescent Dyes, Organic Chemicals, Papillomaviridae isolation & purification, Polymerase Chain Reaction methods

Published

1995

34. Staining of Escherichia coli for flow cytometry: influx and efflux of ethidium bromide.

Author

Jernaes MW and Steen HB

Subjects

Cell Separation methods, Cell Wall drug effects, Cell Wall metabolism, Cold Temperature adverse effects, Edetic Acid pharmacology, Escherichia coli cytology, Flow Cytometry methods, Hot Temperature adverse effects, Organophosphates pharmacology, Escherichia coli metabolism, Ethidium pharmacokinetics

Abstract

In an attempt to develop procedures for nucleic acid staining of bacteria for clinical routine assays, the uptake of ethidium bromide (EB) in wild-type Escherichia coli was studied using flow cytometry. Phosphate-buffered saline (PBS) containing EDTA or Tris significantly increased the net uptake of EB compared to PBS only. However, in the majority of the cells, the net uptake reached a constant level that was only a few percent of that of fully permeabilized cells, apparently due to the activity of a metabolically driven efflux pump. When cells were exposed to cold shock (0 degrees C for 30 min) in the presence of Tris or EDTA, the net uptake of dye was similar to that of fully permeabilized cells, whereas it was about half that value in PBS. When cold shock was given in growth medium, the cells split up into four subpopulations, with a net dye uptake ranging from that of fully permeabilized cells to less than 1% of that value. As expected, metabolic inhibitors (Na-azide, 2-deoxy-D-glucose, and CCCP) reduced efflux activity. However, fluorescence of metabolically inhibited cells never exceeded more than about half the value of that of dead cells, possibly reflecting conformational changes in DNA structure as a result of cell death.

Published

1994

35. Intracellular calcium and pH alterations induced by tri-n-butyltin chloride in isolated rainbow trout hepatocytes: a flow cytometric analysis.

Author

Reader S, Steen HB, and Denizeau F

Subjects

Animals, Calcium metabolism, Cell Separation, Cell Survival, Cytosol metabolism, Environmental Pollution, Flow Cytometry, Hydrogen-Ion Concentration, Liver cytology, Liver drug effects, Liver metabolism, Oncorhynchus mykiss metabolism, Trialkyltin Compounds pharmacology

Abstract

The effects of tri-n-butyltin chloride (TBT) on ionic homeostasis on isolated trout hepatocytes were investigated by flow cytometry (FCM), using the Ca(2+)-sensitive and pH-sensitive fluorescent probes Indo-1 and SNARF-1, respectively. Cell viability was monitored concurrently. Treatment of hepatocytes with 1 and 5 microM TBT caused a rapid and sustained elevation of cytosolic free Ca2+ concentration [Ca2+]i and an important cytoplasmic acidification. These changes were dependent upon TBT concentration and were maintained over 60 min, the maximum exposure period investigated. At 0.5 microM TBT, there was a slight but not significant increase in [Ca2+]i and a significant reduction in intracellular pH (pHi) only after 60 min of exposure. A rise in [Ca2+]i and cytoplasmic acidification were observed before loss of viability was detectable. Experiments carried out in Ca(2+)-free medium suggest that TBT mainly mobilizes Ca2+ from intracellular stores in trout hepatocytes. The cytoplasmic acidification following TBT exposure seems to be caused by the combination of intracellular Ca2+ mobilization and by direct action of TBT. The present results suggest that ionic homeostasis perturbations could be early events in the mechanism of cell injury by TBT.

Published

1994

36. The initiation mass for DNA replication in Escherichia coli K-12 is dependent on growth rate.

Author

Wold S, Skarstad K, Steen HB, Stokke T, and Boye E

Subjects

Cell Division drug effects, Cell Division physiology, DNA, Bacterial biosynthesis, Escherichia coli drug effects, Escherichia coli growth & development, Flow Cytometry, Rifampin pharmacology, Time Factors, DNA Replication, Escherichia coli genetics

Abstract

It is widely accepted that the initiation mass of Escherichia coli is constant and independent of growth rate, and therefore is an important parameter in the regulation of initiation of DNA replication. We have used flow cytometry to measure the initiation mass of E. coli K-12 cells as a function of growth rate. The average initiation mass was determined by two methods: (i) from a mathematical relationship between average cell mass, cell age at initiation and number of origins present in the cells, and (ii) directly from the cell mass distribution. The light scattering signal from individual cells and the protein content per cell were employed as measures of cell mass. The initiation mass was found to increase monotonically with decreasing growth rate, being 1.6 times higher (light scattering) or 2.1 times higher (protein content) at 0.3 than at 2.5 doublings per hour. We conclude that the initiation mass is dependent on growth rate. This finding indicates that the control for timing of initiation is not governed by a direct connection between mass accumulation and the molecule(s) determining initiation of replication.

Published

1994

37. Characterization of singlet oxygen-induced guanine residue damage after photochemical treatment of free nucleosides and DNA.

Author

Kvam E, Berg K, and Steen HB

Subjects

Deoxyguanosine chemistry, Free Radicals, Methylene Blue, Nucleosides isolation & purification, Photochemistry, Porphyrins, Singlet Oxygen, DNA chemistry, Guanine chemistry, Nucleosides chemistry, Oxygen chemistry

Abstract

DNA and free nucleosides were photosensitized with the DNA-binding dyes methylene blue (MB) and meso-tetra(4-N-methyl-pyridyl) porphyrin (p-TMPyP) and the non-binding meso-tetra (4-sulphonatophenyl) porphyrin (TSPP). After light exposure DNA was enzymatically digested to nucleosides. Only the guanine residues were photodegraded. By measuring optical absorption, at least 20 photoproducts were detected. Singlet oxygen (1O2) was involved in induction of all these products since D2O enhanced their yields from 4 to 10 times. The photoproducts were the same for all sensitizers. However, several photoproducts were found only with DNA or only with free 2'-deoxyguanosine. Four of 20 photoproducts were induced both in DNA and free 2'-deoxy-guanosine. The yield of the photoproduct 8-oxo-7,8-dihydro-2'-deoxyguanosine (8-oxo-dG) relative to the degree of 2'-deoxy-guanosine degradation depended on which sensitizer was used and on whether nucleosides or DNA was exposed. Apparently, DNA structure affected the types of as well as the yields of photo-products induced by 1O2.

Published

1994

38. No correlation between DNA strand breaks and HPRT mutation induced by photochemical treatment in V79 cells.

Author

Noodt BB, Moan J, Kvam E, and Steen HB

Subjects

Animals, Cells, Cultured, Cricetinae, DNA drug effects, DNA Damage, DNA Repair, Mutation, Photosensitizing Agents pharmacology, Porphyrins pharmacology, X-Rays, DNA radiation effects, Hypoxanthine Phosphoribosyltransferase genetics, Light

Abstract

DNA strand breaks, measured by alkaline elution, and hypoxanthine guanine phosphoribosyltransferase (HPRT) mutation were studied in V79 cells after photochemical treatment (PCT) or exposure to X-rays. Cells were incubated with the photosensitizers Photofrin II (PII) and three closely related porphyrins tetra-(3-hydroxyphenyl) porphyrin (3THPP), meso-tetra-(4-sulfonatophenyl) porphine (TPPS4) and meso-tetra-(N-methyl-4-pyridyl) porphine (TMPyPH2). These dyes are assumed to act on cellular targets mainly via singlet oxygen when excited by light. While the hydrophilic TPPS4 and TMPyPH2 did not photoinduce mutants to any significant extent, both lipophilic dyes, 3THPP and PII, were significantly mutagenic when excited by light. On the other hand, TPPS4 was the most efficient sensitizer of alkali-labile DNA strand breaks, while TMPyPH2 did not induce any significant amount of either type of DNA damage. Surprisingly, no correlation between the two parameters was found for PCT, either after exposures inactivating 50% of the cells or after exposures inactivating 90% of them. The lack of correlation between the yields of DNA strand breaks and of mutants could not be explained by differences in the intracellular localization pattern of the dyes.

Published

1994

39. Staining and measurement of DNA in bacteria.

Author

Steen HB, Jernaes MW, Skarstad K, and Boye E

Subjects

Cell Cycle, Escherichia coli cytology, Fixatives, Flow Cytometry standards, Quality Control, Reference Standards, DNA, Bacterial analysis, Escherichia coli chemistry, Flow Cytometry methods, Staining and Labeling methods

Published

1994

40. Primary DNA damage, HPRT mutation and cell inactivation photoinduced with various sensitizers in V79 cells.

Author

Noodt BB, Kvam E, Steen HB, and Moan J

Subjects

Animals, Cell Line, Cell Survival drug effects, Cell Survival radiation effects, Cricetinae, Cricetulus, Dihematoporphyrin Ether toxicity, Light, Mutagenesis, Porphyrins toxicity, X-Rays, DNA Damage drug effects, Hypoxanthine Phosphoribosyltransferase genetics, Radiation-Sensitizing Agents toxicity

Abstract

DNA strand breaks and hypoxanthine guanine phosphoribosyl transferase (HPRT) mutants were measured in parallel in photochemically treated (PCT) cells and compared at the same level of cell survival. Chinese hamster fibroblasts (V79 cells) were either incubated with the lipophilic dyes tetra(3-hydroxyphenyl)porphyrin (3THPP) and Photofrin II (PII), the anionic dye meso-tetra(4-sulfonatophenyl)porphine (TPPS4) or the cationic dye meso-tetra(N-methyl-4-pyridyl)porphine (p-TMPyPH2) before light exposure. In the cells, the lipophilic dyes were localized in membranes, including the nuclear membrane, while the hydrophilic dyes were taken up primarily into spots in the cytoplasm. In addition, the hydrophilic TPPS4 was distributed homogeneously throughout the whole cytoplasm and nucleoplasm. According to the HPRT mutation test, the mutagenicity of light doses survived by 10% of the cells was a factor of six higher in the presence of 3THPP than of PII, whereas for X-rays it was a factor of three higher than for PCT with 3THPP. Light exposure in the presence of the hydrophilic dyes TPPS4 and p-TMPyPH2 was not significantly mutagenic. There was no correlation between the induced rates of HPRT mutants and of DNA strand breaks. Thus, TPPS4 was the most efficient sensitizer with regard to DNA strand breaks when compared at the same level of cell survival, followed by 3THPP, PII and p-TMPyPH2. Hence, the rate of DNA strand breaks cannot be used to predict the mutagenicity of PCT.

Published

1993

41. Potentiation of photodynamic therapy by mitomycin C in cultured human colon adenocarcinoma cells.

Author

Ma LW, Moan J, Berg K, Peng Q, and Steen HB

Subjects

Cell Survival drug effects, Dose-Response Relationship, Drug, Drug Synergism, Drug Therapy, Combination, Humans, Tumor Cells, Cultured, Adenocarcinoma drug therapy, Colonic Neoplasms drug therapy, Dihematoporphyrin Ether therapeutic use, Mitomycin therapeutic use, Photochemotherapy

Abstract

The effects of photodynamic therapy (PDT) alone and in combination with Mitomycin C (MMC) on WiDr cells, a human colon adenocarcinoma cell line, were investigated. The addition of MMC increased the cytotoxicity of PDT. The presence of MMC resulted in a reduction or a removal of the shoulder of the PDT survival curves as well as an increase in their slopes. Increasing with the concentrations of MMC from 0.01 to 0.025 micrograms/ml, the cytotoxic effects of the two treatments changed from additivity to supra-additivity as judged by comparing dose-response curves for each treatment alone with survival curves after combination therapy and by isobologram analysis. The cytotoxicity of MMC could also be enhanced by a practically nontoxic treatment of PDT (8% cell inactivation). The cytotoxicities of MMC and PDT in combination were found to be dependent on the sequence of the two treatments. When MMC (> or = 0.02 micrograms/ml) and Photofrin II were given simultaneously for 16 h and then followed by irradiation, the combination was found to be more effective than when MMC was given to the cells immediately after PDT and kept in the medium for 16 h. Possible mechanisms of the combination effects of PDT and MMC are discussed briefly.

Published

1993

42. Expression of CD18 (integrin beta 2 chain) correlates with prognosis in malignant B cell lymphomas.

Author

Erikstein BK, Holte H, Kvaløy S, Andersson KB, Steen HB, Hannisdal E, and Smeland EB

Subjects

Antigens, CD analysis, CD18 Antigens, Female, Humans, Lymphoma, B-Cell mortality, Lymphoma, B-Cell pathology, Male, Middle Aged, Norway epidemiology, Prognosis, Retrospective Studies, Sialyltransferases, Survival Rate, Thymidine metabolism, Lymphoma, B-Cell immunology, Receptors, Leukocyte-Adhesion analysis

Abstract

Several studies have shown that cell cycle related parameters including DNA synthesis and activation antigen expression can predict patient survival in lymphoma patients. In this study of 69 malignant B cell lymphomas we have examined the cell surface expression of several cell interaction and activation molecules by flow cytometry. Expression of CD18 (integrin beta 2 chain) was found to correlate strongly with patient survival (median follow up 50 months) even when adjusting for other important prognostic factors (P = 0.0001). The percentage of cells positive for CDw75 proved important both as a single parameter and in the multivariate analysis. Histology, classified as low versus high grade malignancy, bulky versus not bulky disease and high versus low thymidine incorporation, was also found to correlate with prognosis in this study.

Published

1993

43. Pulse modulation of the excitation light source boosts the sensitivity of an arc lamp-based flow cytometer.

Author

Steen HB and Sørensen OI

Subjects

Light, Sensitivity and Specificity, Flow Cytometry instrumentation

Abstract

It has been found that the type of short arc high-pressure lamps used in some flow cytometers can be pulsed to reach intensities many times higher than that measured when they are operated on constant power. A 75 W mercury-xenon lamp was fed 20 microseconds current pulses super-imposed on its rated current of 5.4 A. Pulses of 50 A produced a 75-fold increase of the emission intensity at the excitation wavelength of FITC, which means that the excitation intensity in the flow chamber at this wavelength exceeded 100 mW. At the major emission lines of mercury, i.e., 366, 436, and 546 nm, the increase was about 25-fold, corresponding to intensities of the order of 300 mW. The light pulses were found to be reproducible to within 2% and the intensity was independent of the pulse frequency up to at least 250 pulses/s. Operated in this mode the lamp produced more than 1 x 10(8) 30 A pulses, which is sufficient to measure some 10,000 typical size samples. The rise time of the light pulses was about 5 microseconds. This was sufficiently short that the leading edge of the light scattering signal from a cell entering the excitation focus of the flow cytometer could be used to trigger the current pulse so that the cells were exposed to the full light pulse intensity while they were still within the focus.(ABSTRACT TRUNCATED AT 250 WORDS)

Published

1993

44. The retinoblastoma gene product is bound in the nucleus in early G1 phase.

Author

Stokke T, Erikstein BK, Smedshammer L, Boye E, and Steen HB

Subjects

Cell Cycle, Cell Division, Cell Line, Cell Nucleus metabolism, Humans, Phosphorylation, Retinoblastoma Protein metabolism

Abstract

The product of the retinoblastoma susceptibility gene (pRB) exerts its growth-regulatory effects during the G1 phase of the cell cycle, where all pRB present has been assumed to be in the underphosphorylated form. We demonstrate here that pRB is underphosphorylated and firmly bound in the nucleus only in early G1 phase. All G0 cells contain bound, underphosphorylated pRB. The duration of the cell cycle and of the G1 phase seems to be determined by the time during which pRB is underphosphorylated and bound in the nucleus. The observed time lag between the phosphorylation and release of pRB in the G1 phase and entry into S phase was 6.5 h and independent of the G1 transit time. The data suggest that pRB is not directly involved in initiation of DNA replication.

Published

1993

45. Plateau distributions of DNA fragment lengths produced by extended light exposure of extranuclear photosensitizers in human cells.

Author

Kvam E, Stokke T, Moan J, and Steen HB

Subjects

Cell Line, DNA isolation & purification, DNA Probes, Electrophoresis, Agar Gel, Genes, fos, Genes, myc, Genes, p53, Humans, Microscopy, Fluorescence, Molecular Weight, DNA drug effects, Light, Oligodeoxyribonucleotides isolation & purification, Porphyrins pharmacology, Radiation-Sensitizing Agents pharmacology

Abstract

We have exploited properties of photosensitizers to study an aspect of the packing of chromatin in the cell nucleus. The fluorescent photosensitizers mesotetra(3-hydroxyphenyl) porphyrin and Photofrin II were both localized in the nuclear membrane and other membrane structures, but could not be found inside the nuclei. Light exposure of cells at 1 degrees C in the presence of the sensitizers induced DNA double-strand breaks. The length distributions of DNA fragments were determined by pulsed field gel electrophoresis. Because DNA damage is produced mainly via singlet oxygen diffusing less than 0.1 microns from the sensitizer, DNA double-strand breaks were supposedly produced within this distance of the nuclear membrane. Consistent with this, with prolonged illumination and with increasing concentrations of sensitizer the distribution of DNA fragment lengths reached a plateau level. In contrast, with the hydrophilic, intranuclear sensitizer meso-tetra(4-sulphonatophenyl)porphyrin, no such plateau level was found. The plateau distributions of DNA fragment lengths of different cell types had the same general shape with average fragment lengths ranging from 174 to 194 kilobasepairs. Particular genes, c-myc, fos and p53, were found on broad distributions of photocleaved fragment lengths. The results indicate that on each side of the genes the locus of the chromatin fibre situated close to the nuclear membrane, varied randomly.

Published

1992

46. Cytotoxicity and cytokinetic effects of mitomycin C and/or photochemotherapy in a human colon adenocarcinoma cell line.

Author

Ma LW, Steen HB, Moan J, Berg K, Peng Q, Saether H, and Rimington C

Subjects

Adenocarcinoma pathology, Cell Cycle drug effects, Cell Survival, Colonic Neoplasms pathology, Flow Cytometry, Humans, Tumor Cells, Cultured, Adenocarcinoma drug therapy, Colonic Neoplasms drug therapy, Mitomycin therapeutic use, Photochemotherapy

Abstract

1. The cytotoxicity and cytokinetic effects of Mitomycin C (MC) and/or photochemotherapy (PCT) in cultured human colon adenocarcinoma (WiDr) cells were investigated using colony formation to determine cell survival and DNA flow cytometry to analyze cell kinetics. 2. A low concentration of MC (0.01 micrograms/ml) caused accumulation of cells in late S and early G2 phase; higher concentrations (0.05-0.5 micrograms/ml) induced accumulation of the cells in mid and early S phase. 3. The effects of the lowest concentration of MC (0.01 micrograms/ml) were reversible upon removal of the drug, whereas a higher concentration of MC (0.1 micrograms/ml) resulted in a permanent inhibition of cell cycle progression. 4. The sensitivity of Photofrin II-loaded cells to PCT can be enhanced significantly by the addition of MC. 5. The MC-induced accumulation of the cells in S phase may be one reason for the increased cytotoxicity of PCT combined with MC. 6. The data suggest that MC may also inhibit repair of PCT-induced DNA damage.

Published

1992

47. Differential chromatin structure-dependent binding of 7-aminoactinomycin D in normal and malignant bone marrow hematopoietic cells.

Author

Stokke T, Holte H, Smeland EB, Lie SO, and Steen HB

Subjects

Antigens, CD analysis, Cell Cycle, Child, Chromatin metabolism, Dactinomycin metabolism, Flow Cytometry, Hematopoietic Stem Cells immunology, Humans, Leukemia, Myeloid, Acute diagnosis, Leukemia, Myeloid, Acute immunology, Precursor Cell Lymphoblastic Leukemia-Lymphoma diagnosis, Precursor Cell Lymphoblastic Leukemia-Lymphoma immunology, Survival Analysis, Transcription, Genetic, Chromatin ultrastructure, DNA metabolism, Dactinomycin analogs & derivatives, Hematopoietic Stem Cells metabolism, Leukemia, Myeloid, Acute metabolism, Precursor Cell Lymphoblastic Leukemia-Lymphoma metabolism

Abstract

Chromatin structure-dependent binding of the DNA-specific dye 7-aminoactinomycin D (7-AMD) in leukemic and normal cells in bone marrow aspirates from childhood acute leukemia patients and patients without bone marrow neoplasia was assessed by multiparameter flow cytometry. Simultaneous staining with fluorescein isothiocyanate-labeled antibodies was needed in many cases for determination of the immunophenotype of the cells that exhibited differential binding of 7-AMD. 7-AMD binding was enhanced in normal (4 patients) and malignant (8 patients) myeloid cells, and was generally low in normal and leukemic lymphocytes and normoblasts. Four of 18 aspirates from 16 patients with acute lymphoblastic leukemia contained neoplastic cells with increased 7-AMD binding capability. The 7-AMD binding of the leukemic cells was not correlated to S-phase fraction (P = 0.07), but was significantly correlated to cell size as measured by forward angle light scattering (r = 0.49, P = 0.007). Patients with tumor cells exhibiting low 7-AMD binding at last aspirate survived significantly longer than the patients with leukemic cells binding high amounts of 7-AMD (P = 0.03). Neither cell size, S-phase fraction, nor ploidy status predicted patient survival in this small scale study.

Published

1992

48. Effect of mitomycin C on the uptake of photofrin II in a human colon adenocarcinoma cell line.

Author

Ma LW, Moan J, Steen HB, Berg K, and Peng Q

Subjects

Cell Cycle drug effects, Cell Division drug effects, Cell Membrane Permeability drug effects, Cell Survival, Dihematoporphyrin Ether, Flow Cytometry, Humans, Time Factors, Tumor Cells, Cultured drug effects, Adenocarcinoma metabolism, Colonic Neoplasms metabolism, Hematoporphyrins metabolism, Mitomycin pharmacology

Abstract

Flow cytometry (FCM) was used to investigate the effect of mitomycin C (MC) on the cellular uptake of Photofrin II (PII) in a cultured human colon adenocarcinoma cell line (WiDr). The surface area of the cells increased as they passed through the cell cycle from G0/G1 to G2/M phase. MC retarded the cells in G2/M phase and enhanced the surface area of the cells. A 1.3-2.3-fold increase in the cell surface area and a 1.3-2.7-fold increase in the cellular uptake of PII in the tumor cells was observed after 2 h-8 h incubation with MC. Within each sample, an almost linear relationship between the intensity of PII fluorescence in the cells and the surface area of the cells was found. However, for the cells incubated with MC the surface area was not the only determinant of PII uptake. Effects of MC on the cell cycle, the cell surface area and the permeability of the cell membrane are suggested as possible reasons for the increase of cellular uptake of PII in the tumor cells.

Published

1992

49. Synergistic effects of photoactivated tetra(4-sulfonatophenyl)porphine and nocodazole on microtubule assembly, accumulation of cells in mitosis and cell survival.

Author

Berg K, Steen HB, Winkelman JW, and Moan J

Subjects

Carcinoma in Situ, Cell Line, Cell Survival radiation effects, DNA, Neoplasm drug effects, DNA, Neoplasm radiation effects, Dose-Response Relationship, Radiation, Drug Synergism, Female, Fluorescent Antibody Technique, Humans, Light, Microtubules drug effects, Microtubules physiology, Mitosis, Mitotic Index drug effects, Mitotic Index radiation effects, Porphyrins radiation effects, Tubulin drug effects, Uterine Cervical Neoplasms, Cell Survival drug effects, Microtubules ultrastructure, Nocodazole pharmacology, Porphyrins pharmacology, Radiation-Sensitizing Agents pharmacology, Tubulin metabolism

Abstract

Human carcinoma cells of the line NHIK 3025 were incubated with meso-tetra(4-sulfonatophenyl)porphine (TPPS4) for 18 h and exposed to light in the absence or presence of nocodazole. Nocodazole (1 microgram ml-1) was applied to the cells 15 min prior to light exposure and washed off the cells immediately afterwards. The presence of nocodazole during photoactivation of TPPS4-loaded cells leads to a significantly reduced ability of tubulin to repolymerize after withdrawal of nocodazole, an increased accumulation of the cells in mitosis with a larger fraction in c-metaphase and a higher yield of photoactivated cells. A higher proportion of the cells accumulating in mitosis 6-12 h after exposure to light is unable to form colonies when exposed to light in the presence of nocodazole than in its absence. The present results are consistent with a specific TPPS4-induced photodamage to the unpolymerized form of the microtubule components.

Published

1992

50. Noise, sensitivity, and resolution of flow cytometers.

Author

Steen HB

Subjects

Calibration, Fluorescence, Mathematics, Poisson Distribution, Sensitivity and Specificity, Stochastic Processes, Flow Cytometry instrumentation

Abstract

The sensitivity and resolution of flow cytometers are functions of the signal produced by a given particle as well as by the noise in the presence of which the signal is detected. The noise is primarily due to the fact that emission of light as well as its detection by photoelectric devises are stochastic processes. This fact leads to equations describing how resolution and sensitivity are limited by the magnitude of the signal, the background, and the photoelectron quantum yield of the detector. The equations are pointing to a method by which the signal and noise of a flow cytometer can be measured in absolute terms, as well as a way to determine fluorescence sensitivity without having to extrapolate to the noise level. The equations appear to be validated when applied to measuring data obtained with two different flow cytometers.

Published

1992