Your search keyword '"Fredriksson SA"' showing total 12 results

1. EMISSION OF HYDROGEN-SULFIDE FROM SULFUR-DIOXIDE FUMIGATED PINE TREES

Author

HALLGREN, JE, FREDRIKSSON, SA, HALLGREN, JE, and FREDRIKSSON, SA

Published

1982

2. ABH blood group antigens in N-glycan of human glycophorin A.

Author

Fredriksson SA, Podbielska M, Nilsson B, Krotkiewska B, Lisowska E, and Krotkiewski H

Subjects

Humans, Mass Spectrometry methods, ABO Blood-Group System chemistry, Epitopes chemistry, Glycophorins chemistry, Oligosaccharides chemistry

Abstract

We previously showed that a small proportion of the O-linked oligosaccharide chains of human glycophorin A (GPA) contains blood group A, B or H antigens, relevant to the ABO phenotype of the donor. The structures of these minor O-glycans have been established (Podbielska et al. (2004) [20]). By the use of immunochemical methods we obtained results indicating that ABH blood group epitopes are also present in N-glycan of human GPA (Podbielska and Krotkiewski (2000) [22]). In the present paper we report a detailed analysis of GPA N-glycans using nanoflow electrospray ionization tandem mass spectrometry. N-glycans containing A-, B- and H-related sequences were identified in GPA preparations obtained from erythrocytes of blood group A, B and O donors, respectively. The ABH blood group epitopes are present on one antenna of the N-glycan, whereas a known sialylated sequence NeuAcalpha2-6Galbeta1-4GlcNAc- occurs on the other antenna and other details are in agreement with the known major structure of the GPA N-glycan. In the bulk of the biantennary sialylated N-glycans released from GPA preparations, the blood group ABH epitopes-containing N-glycans, similarly O-glycans, constituted only a minor part. The amount relative to other N-glycans was estimated to 2-6% of blood group H epitope-containing glycans released from GPA-O preparations and 1-2% of blood group A and B epitope-containing glycans, released from GPA-A and GPA-B, respectively., (Copyright (c) 2010 Elsevier Inc. All rights reserved.)

Published

2010

3. De novo sequencing of RCB-1 to -3: peptide biomarkers from the castor bean plant Ricinus communis.

Author

Ovenden SP, Fredriksson SA, Bagas CK, Bergström T, Thomson SA, Nilsson C, and Bourne DJ

Subjects

Amino Acid Sequence, Biomarkers analysis, Biomarkers chemistry, Ricinus communis classification, Forensic Medicine, Molecular Sequence Data, Peptides chemistry, Plants, Toxic, Ricin chemistry, Seeds chemistry, Sequence Analysis, Ricinus communis chemistry, Chromatography, High Pressure Liquid methods, Peptides analysis, Spectrometry, Mass, Electrospray Ionization methods

Abstract

Ricinus communis (also know as the castor bean plant) whose forbears escaped from suburban gardens or commercial cultivation grow wild in many countries. In temperate and tropical climates seeds will develop to maturity, and plants may be perennial. In Australia these plants have become widespread and are regarded as noxious weeds in many localities. The seeds of R. communis contain ricin, a protein toxin which can easily be extracted into an aqueous solution. Ricin is toxic by ingestion, inhalation, and injection. The history of terrorist and anarchist interest in the use of seeds from R. communis has driven the development of strategies for determination of cultivar and geographic location of the source of an extract of wild-grown castor bean seed. This forensic information is of considerable interest to law enforcement and intelligence organizations. During forensic studies of both the metabolome and proteome of extracts from eight specimens of six different cultivars of R. communis ("zanzibariensis" collected from Kenya and Tanzania, "gibsonii", "impala", "dehradun", "carmencita", and "sanguineus" collected from Spain and Tanzania), three peptide biomarkers (designated Ricinus communis biomarkers, or RCB) were identified in both the MALDI and electrospray LC-MS spectra. Two of these peptides (RCB-1 and RCB-2) were present in varying amounts in all cultivars, while RCB-3 was present only in the "carmencita" cultivar. The amino acid sequences of RCB-1 to -3 were determined using LC-MS(n) fragmentation and de novo sequencing on both the intact and the carbamidomethyl modified peptides. The connectivity of the two disulfide bonds that were present in all three RCB were determined using a strategy of partial reduction and differential alkylation using tris-(2-carboxyethyl)phosphine with N-ethylmaleimide to reduce and alkylate the most accessible disulfide bond, followed by reduction and alkylation of the remaining disulfide bond with dithiolthreitol and iodoacetamide. The possible functional role of RCB-1 to -3 in R. communis seeds is also discussed.

Published

2009

4. Solvent-assisted trypsin digestion of ricin for forensic identification by LC-ESI MS/MS.

Author

Ostin A, Bergström T, Fredriksson SA, and Nilsson C

Subjects

Chromatography, Liquid, Disulfides, Peptide Fragments analysis, Plant Extracts, Solvents, Spectrometry, Mass, Electrospray Ionization, Time Factors, Forensic Medicine, Ricin analysis, Tandem Mass Spectrometry methods

Abstract

The castor bean plant (Ricinus communis) is used in large quantities for oil production and is also a common ornamental garden plant. However, the beans contain 1-3% of the highly toxic protein ricin, a type II ribosome-inactivating protein that is covered by the Chemical Weapons Convention, and there have been a number of reports concerning the use, or alleged use, of the toxin in terrorist and criminal activities. In the study reported here, we investigated the potential utility of organic solvent-assisted trypsin digestion of crude extracts containing the closely related toxins ricin or abrin to prepare samples for peptide analysis by liquid chromatography combined with electrospray ionization quadrupole time-of-flight tandem mass spectrometry. Diagnostic tryptic fragments of the toxins were detected and unambiguously identified by this procedure. The sample preparation protocol substantially reduces the sample preparation time, from overnight to an hour, and thus greatly reduces the total time required for analyses, to less than 2 h. Furthermore, the reported procedure leaves the disulfide bonds in the protein intact. This is highly relevant in the context of the Chemical Weapons Convention, since the disulfide bond connecting the two chains of ricin indicates the presence of an intact toxin and provides additional forensic evidence for the analytical results.

Published

2007

5. Forensic identification of neat ricin and of ricin from crude castor bean extracts by mass spectrometry.

Author

Fredriksson SA, Hulst AG, Artursson E, de Jong AL, Nilsson C, and van Baar BL

Subjects

Amino Acid Sequence, Forensic Medicine, Molecular Sequence Data, Ricin chemistry, Ricinus communis chemistry, Plant Extracts analysis, Ricin analysis, Spectrometry, Mass, Matrix-Assisted Laser Desorption-Ionization methods

Abstract

The protein toxin ricin, which originates from the seeds of Ricinus communis plants, has been the subject of increased interest, due to its potential terrorist use. Exceptionally, this toxin is also subject to the Chemical Weapons Convention. In this paper, it is shown that mass spectrometry can be used to unambiguously verify the presence of ricin in crude toxin preparations. It is demonstrated that MALDI MS can be used for screening, either by direct analysis or by trypsin digestion and peptide mapping. Purified ricin from several varieties of R. communis was characterized by LC-ES MS(/MS). A crude ricin preparation from a single bean was similarly characterized. An LC method was set up with product ion MS/MS detection of selected marker peptides specific for ricin: T5, T7, T11, T12, and T13 from the A-chain and T3, T5, T14, T19, and T20 from the B-chain. This method was then used to unambiguously identify ricin in a crude preparation of ricin. The MALDI MS molecular weight analysis and the marker peptides LC-ES MS/MS analysis give a forensic level of identification of ricin when combined with activity testing.

Published

2005

6. ABH blood group antigens in O-glycans of human glycophorin A.

Author

Podbielska M, Fredriksson SA, Nilsson B, Lisowska E, and Krotkiewski H

Subjects

Blotting, Western, Carbohydrate Sequence, Electrophoresis, Polyacrylamide Gel, Methylation, Molecular Sequence Data, Polysaccharides immunology, Spectrometry, Mass, Electrospray Ionization, ABO Blood-Group System immunology, Glycophorins immunology, Polysaccharides chemistry

Abstract

The major O-linked oligosaccharide structures attached to human glycophorin A (GPA) have been extensively characterized previously. Our own recent findings, obtained by immunochemical methods, suggested the presence of blood group A and B determinants in O-glycans of human glycophorin originating from blood group A or B erythrocytes, respectively. Here, we elucidate the structure of O-glycans, isolated from GPA of blood group A, B, and O individuals by reductive beta-elimination, carrying A, B or H blood group epitopes, respectively. Structural studies based on nanoflow electrospray-ionization tandem mass spectrometry and earlier reported data on the carbohydrate moiety of GPA and ABH antigens allowed us to conclude that these blood group epitopes are elongations of the beta-GlcNAc branch attached to C-6 of the reducing GalNAc. The galactose linked to C-3 of the reducing GalNAc carries NeuAcalpha2-3 linked residue. Identified here O-glycans were found in low amounts, their content estimated at about one percent of all GPA O-glycans. These O-glycans with type-2 core, carrying the blood group A, B or H determinants, have not been identified in GPA so far. Our results demonstrate the efficacy of nanoESI MS/MS in detecting minor oligosaccharide components present in a mixture with much more abundant structures.

Published

2004

7. The chemotactic response of Vibrio anguillarum to fish intestinal mucus is mediated by a combination of multiple mucus components.

Author

O'Toole R, Lundberg S, Fredriksson SA, Jansson A, Nilsson B, and Wolf-Watz H

Subjects

Animals, Chromatography, Thin Layer, Gas Chromatography-Mass Spectrometry, Humans, Intestinal Mucosa microbiology, Methyltransferases genetics, Molecular Sequence Data, Mucus microbiology, Sequence Analysis, DNA, Skin chemistry, Skin microbiology, Vibrio physiology, Vibrio cholerae enzymology, Vibrio cholerae genetics, Virulence, Chemotaxis physiology, Intestinal Mucosa chemistry, Mucus chemistry, Oncorhynchus mykiss microbiology, Vibrio pathogenicity

Abstract

Chemotactic motility has previously been shown to be essential for the virulence of Vibrio anguillarum in waterborne infections of fish. To investigate the mechanisms by which chemotaxis may function during infection, mucus was isolated from the intestinal and skin epithelial surfaces of rainbow trout. Chemotaxis assays revealed that V. anguillarum swims towards both types of mucus, with a higher chemotactic response being observed for intestinal mucus. Work was performed to examine the basis, in terms of mucus composition, of this chemotactic response. Intestinal mucus was analyzed by using chromatographic and mass spectrometric techniques, and the compounds identified were tested in a chemotaxis assay to determine the attractants present. A number of mucus-associated components, in particular, amino acids and carbohydrates, acted as chemoattractants for V. anguillarum. Importantly, only upon combination of these attractants into a single mixture were levels of chemotactic activity similar to those of intestinal mucus generated. A comparative analysis of skin mucus revealed its free amino acid and carbohydrate content to be considerably lower than that of the more chemotactically active intestinal mucus. To study whether host specificity exists in relation to vibrio chemotaxis towards mucus, comparisons with a human Vibrio pathogen were made. A cheR mutant of a Vibrio cholerae El Tor strain was constructed, and it was found that V. cholerae and V. anguillarum exhibit a chemotactic response to mucus from several animal sources in addition to that from the human jejunum and fish epithelium, respectively.

Published

1999

8. Toxicokinetics of soman in cerebrospinal fluid and blood of anaesthetized pigs.

Author

Göransson-Nyberg A, Fredriksson SA, Karlsson B, Lundström M, and Cassel G

Subjects

Anesthesia, Animals, Biotransformation, Cholinesterase Inhibitors blood, Cholinesterase Inhibitors cerebrospinal fluid, Cholinesterases blood, Cholinesterases cerebrospinal fluid, Cisterna Magna metabolism, Gas Chromatography-Mass Spectrometry, Hemodynamics drug effects, Isomerism, Kinetics, Lethal Dose 50, Male, Respiratory Mechanics drug effects, Soman blood, Soman cerebrospinal fluid, Swine, Cholinesterase Inhibitors toxicity, Soman toxicity

Abstract

The toxicokinetics of the four stereoisomers of the nerve agent C(+/-)P(+/-)-soman was analysed in cerebrospinal fluid (CSF) and blood in anaesthetized, spontaneously breathing pigs during a 90-min period after injection of soman. The pigs were challenged with different intravenous (i.v.) doses of C(+/-)P(+/-)-soman corresponding to 0.75-3.0 LD50 (4.5, 9.0 and 18 microg/kg in a bolus injection and 0.45 microg/kg per min as a slow infusion). Artificial ventilatory assistance was given if, after soman intoxication, the respiratory rate decreased below 19 breaths/min. Blood samples were taken from a femoral artery and CSF samples from an intrathecal catheter. The concentrations of the soman isomers were determined by gas chromatography coupled with high resolution mass spectrometry. All four isomers of soman were detected in both blood and CSF samples. The relatively non-toxic C(+/-)P(+) isomers disappeared from the blood stream and CSF within the first minute, whereas the levels of the highly toxic C(+/-)P(-) isomers could be followed for longer, depending on the dose. Concurrently with the soman analyses in blood and CSF, cholinesterase (ChE) activity and cardiopulmonary parameters were measured. C(+/-)P(-) isomers showed approx. 100% bioavailability in CSF when C(+/-)P(+/-)-soman was given i.v. as a bolus injection. In contrast, C(+/-)P(-) isomers displayed only 30% bioavailability in CSF after slow i.v. infusion of soman. The ChE activity in blood decreased below 20% of baseline in all groups of pigs irrespective of the soman dose. The effect of soman intoxication on the respiratory rate, however, seems to be dose-dependent and the reason for ventilatory failure and death. Artificial ventilation resulted in survival of the pigs for the time-period studied.

Published

1998

9. The effect of the calcium antagonist nimodipine on the detoxification of soman in anaesthetized rabbits.

Author

Karlsson BM, Waara LM, Fredriksson SA, and Koskinen LO

Subjects

Acetylcholinesterase metabolism, Animals, Blood Gas Analysis, Cholinesterase Inhibitors pharmacokinetics, Cholinesterase Inhibitors poisoning, Inactivation, Metabolic, Organ Specificity, Rabbits, Soman pharmacokinetics, Soman poisoning, Antidotes pharmacology, Calcium Channel Blockers pharmacology, Cholinesterase Inhibitors blood, Nimodipine pharmacology, Soman blood

Abstract

The effect of nimodipine, a vasoactive calcium antagonist, on the disappearance of soman from blood was studied in anaesthetized rabbits intoxicated with soman (10.8 micrograms kg-1 i.v.). Blood samples from the left heart ventricle and femoral artery were used to investigate soman detoxification. The concentrations of the soman isomers C+P- and C-P- in blood samples were determined by gas chromatography coupled with high-resolution mass spectrometry. During the sampling, 15-300 s after soman injection, the soman concentration in control animals decreased from 50 to 0.029 ng mL-1; in animals pre-treated with nimodipine (10 mg kg-1) it decreased from 15 to 0.033 ng mL-1. In animals pre-treated with nimodipine the soman concentration was significantly reduced during the first minute of sampling. No differences were detected between soman concentrations in samples from the heart and femoral artery. Acetylcholinesterase inhibition was also used as an indicator of soman activity; there was no difference between the activity of this enzyme in different peripheral organs of control and nimodipine-treated animals. Nimodipine reduces the initial concentration of soman in the blood, which might be of significance in the treatment of soman intoxication.

Published

1997

10. The protective effect of nimodipine, a calcium antagonist, and its influence on soman clearance in the anaesthetized rabbit.

Author

Karlsson B, Fredriksson SA, Sellström A, and Algers G

Subjects

Acetylcholinesterase analysis, Anesthesia, Animals, Cholinesterases analysis, Gas Chromatography-Mass Spectrometry, Injections, Intraperitoneal, Nimodipine administration & dosage, Nimodipine pharmacokinetics, Rabbits, Tissue Distribution, Calcium antagonists & inhibitors, Nimodipine pharmacology, Poisoning drug therapy, Soman blood, Soman toxicity

Abstract

The effect of pretreatment with a vasoactive compound, nimodipine, on soman intoxication in peripheral organs of rabbits was studied by measuring changes in the cholinesterase and acetylcholinesterase activity and by measuring clearance of soman in blood using gas chromatography/high resolution mass spectrometry. In animals receiving soman only, initial blood concentrations were approximately 100 ng mL-1 and were still detectable after 5 min. The clearance rate of soman in blood markedly increased following nimodipine pretreatment such that soman was below the detection limit (0.002-0.003 ng mL-1) in all samples. Soman injection caused a significant inhibition of the acetylcholinesterase activity in serum, and in brain. In rabbits pretreated with nimodipine, no significant inhibition of acetylcholinesterase activity occurred after soman injection. In view of the effects of nimodipine on soman clearance and on the acetylcholinesterase and cholinesterase inhibition during soman intoxication, we suggest that nimodipine has profound circulatory effects, which during soman intoxication, increase the vascular perfusion through the body and thereby increase the detoxifying capacity.

Published

1994

11. Trace analysis for chlorinated hydrocarbons in air by quantitative combustion and coulometric chloride determination: application to standardization of vinyl chloride permeation tubes.

Author

Cedergren A and Fredriksson SA

Abstract

Methods for high-temperature combustion of vinyl chloride in air were studied theoretically and two types of gas mixtures were found to give 100% conversion into HCl. The chloride was determined by coulometric titration with silver, in 70% acetic acid. Good agreement between theoretical and experimental results was obtained. Permeation rates of vinyl chloride from fluorinated ethylene propylene permeation tubes were determined gravimetrically and with the coulometric method developed. The standard deviations of the methods were 0.002 and 0.001 microg min respectively for permeation rates of 0.5 microg min when the temperature was controlled to +/- 0.02 degrees . The coulometric mean value was 99.9% of the gravimetric mean; 1 ppm of vinyl chloride in air could be determined coulometrically with a standard deviation of about 0.002 ppm.

Published

1976

12. Emission of hydrogen sulfide from sulfur dioxide-fumigated pine trees.

Author

Hällgren JE and Fredriksson SA

Abstract

Pine (Pinus silvestris L.) trees subjected to relatively low concentration of SO(2) in the field emit H(2)S from the needles, as demonstrated by gas chromatographic analysis after preconcentration on a molecular sieve. H(2)S is the only reduced sulfurous compound emitted from SO(2) fumigated leaves. The emission is light and SO(2) concentration dependent. Pine trees in the field and in laboratory experiments continue to emit H(2)S several hours after the termination of prolonged SO(2) fumigation. The maximum emission rates observed from pine trees in the field and in laboratory experiments, 14 and 20 nanomoles per milligram chlorophyll per hour respectively, are about the activity expected for the sulfur assimilation pathway in the chloroplasts.

Published

1982