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11 results on '"Roberts, D. M."'

1. Enhanced elimination of phenobarbital using charcoal haemoperfusion in a patient with severe poisoning.

Author

Roberts DM, Chau AM, Nair P, and Day RO

Subjects
Aged, Humans, Hypnotics and Sedatives blood, Hypnotics and Sedatives pharmacokinetics, Male, Phenobarbital blood, Phenobarbital pharmacokinetics, Severity of Illness Index, Treatment Outcome, Antidotes therapeutic use, Charcoal therapeutic use, Hemoperfusion methods, Hypnotics and Sedatives poisoning, Phenobarbital poisoning, Suicide, Attempted prevention & control
Published
2011
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2. Analysis of intracellular ice nucleation in Xenopus oocytes by differential scanning calorimetry.

Author

Kleinhans FW, Guenther JF, Roberts DM, and Mazur P

Subjects
Animals, Cryoelectron Microscopy methods, Female, Temperature, Calorimetry, Differential Scanning methods, Ice analysis, Oocytes metabolism, Xenopus metabolism
Abstract

Intracellular ice formation (IIF) plays a central role in cell damage during cryopreservation. We are investigating the factors which trigger IIF in Xenopus oocytes, with and without aquaporin water channels. Here, we report differential scanning calorimeter studies of Xenopus control oocytes which do not express aquaporins. Stage I to VI oocytes (which increase progressively in size) were investigated with emphasis on stage I and II because they are translucent and can also be studied under the cryomicroscope. Measurements were made in 1, 1.5, and 2M ethylene glycol (EG) in frog Ringers plus SnoMax. A multistep freezing protocol was used in which the samples were cooled until extracellular ice formation (EIF) occurred, partially remelted, slowly recooled through the EIF temperature, and then rapidly (10 degrees C/min) cooled. EIF in the 1, 1.5, and 2M EG occurred at -6.4, -7.8, and -8.9 degrees C, respectively. Freezing exotherms of individual stage I-VI oocytes were readily visible. A general trend was observed in which the IIF temperature of the early stage oocytes (I-III) was well below T(EIF) while the later stages (IV-VI) froze at temperatures much closer to T(EIF). Thus, in 1.5M EG, T(IIF) was -21.1, -25, and -26.6 degrees C in stages I-III, but was -17 and -8.5 degrees C for stage IV and V-VI. Concurrently, the percentage of oocytes in which IIF was observed fell dramatically from a high of 40 to 72% in early stages (I-III) to a low of only 7% in stage V-VI because, particularly in the later stages, IIF was hidden in the EIF exotherm. We conclude that early stage oocytes are a good model system in which to investigate modulators of IIF, but that late stage oocytes are damaged during EIF and infrequently supercool.

Published
2006
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3. Soybean nodule sucrose synthase (nodulin-100): further analysis of its phosphorylation using recombinant and authentic root-nodule enzymes.

Author

Zhang XQ, Lund AA, Sarath G, Cerny RL, Roberts DM, and Chollet R

Subjects
Amino Acid Sequence, Amino Acid Substitution, Cloning, Molecular, Escherichia coli, Gene Library, Glucosyltransferases chemistry, Glucosyltransferases isolation & purification, Kinetics, Molecular Sequence Data, Mutagenesis, Site-Directed, Peptide Fragments chemistry, Phosphopeptides chemistry, Phosphorylation, Plant Roots enzymology, Recombinant Proteins chemistry, Recombinant Proteins isolation & purification, Recombinant Proteins metabolism, Sequence Alignment, Sequence Homology, Amino Acid, Spectrometry, Mass, Secondary Ion, Spectrophotometry, Glucosyltransferases metabolism, Glycine max enzymology
Abstract

Sucrose synthase (SS) is a known phosphoserine-containing enzyme in legume root nodules and various other plant "sink" tissues. In order to begin to investigate the possible physiological significance of this posttranslational modification, we have cloned a full-length soybean nodule SS (nodulin-100) cDNA and overexpressed it in Escherichia coli. Authentic nodule SS and recombinant wild-type and mutant forms of the enzyme were purified and characterized. We document that a conserved serine near the N-terminus (Ser(11)) is the primary phosphorylation site for a nodule Ca(2+)-dependent protein kinase (CDPK) in vitro. Related tryptic digestion and mass spectral analyses indicated that this target residue was also phosphorylated in planta in authentic nodulin-100. In addition, a secondary phosphorylation site(s) in recombinant nodule SS was implicated given that all active mutant enzyme forms (S11A, S11D, S11C, and N-terminal truncation between Ala(2) and Arg(13)) were phosphorylated, albeit weakly, by the CDPK. This secondary site(s) likely resides between Glu(14) and Met(193) as evidenced by CNBr cleavage and phosphopeptide mapping. Phosphorylation of the recombinant and authentic nodule Ser(11) enzymes in vitro by the nodule CDPK had no major effect on the sucrose-cleavage activity and/or kinetic properties. However, phosphorylation decreased the apparent surface hydrophobicity of the recombinant wild-type enzyme, suggesting that this covalent modification could potentially play some role in the documented partitioning of nodulin-100 between the nodule symbiosome/plasma membranes and cytosol in planta., (Copyright 1999 Academic Press.)

Published
1999
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4. Expansion of the human microphthalmic orbit.

Author

Gossman MD, Mohay J, and Roberts DM

Subjects
Child, Child, Preschool, Eye growth & development, Humans, Infant, Microphthalmos diagnostic imaging, Orbit diagnostic imaging, Orbit growth & development, Prospective Studies, Tomography, X-Ray Computed, Microphthalmos surgery, Orbit surgery, Tissue Expansion methods, Tissue Expansion Devices
Abstract

Objective: To determine the effects of long-term, incremental enlargement of an orbital tissue expander on bone and eyelid growth in microphthalmia., Design: A prospective, noncomparative case series., Participants: Five consecutive patients with microphthalmos treated with orbital expansion were evaluated., Intervention: A tissue expander was placed into the orbits of five children (age, 10 months-6 years) with unilateral microphthalmos and gradually enlarged by saline injections., Main Outcome Measure: The midorbital width of each patient was determined from axial computed tomographic scans before insertion of the device. The length of the normal and abnormal eyelid fissures was measured at surgery. The postexpansion dimensions of both the normal and microphthalmic orbits and the eyelids were remeasured when the expanders were removed. The residual deficits between the normal and the microphthalmic sides were expressed in percentages., Results: Gradual inflation of the expander to a diameter of 22 mm reduced the average preoperative orbital dimension deficit of the group from 14.6% (range, 8%-25%) to 3.8% after surgery (range, 0.5%-6.3%). The average pre-expansion eyelid length deficit for the group was 17.5% (range, 12%-26%) compared to 2.3% (range, 0.0%-5.3%) after expansion. The average expansion period was 56.8 weeks (range, 20-100 weeks). Two outpatient surgical procedures were required in each patient., Conclusion: Incremental inflation of a tissue expander placed within the microphthalmic orbit induced sufficient osseous and eyelid growth to ameliorate the major stigmata of this syndrome in all patients treated.

Published
1999
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5. Determination of codeine in human plasma by high-performance liquid chromatography with fluorescence detection.

Author

Weingarten B, Wang HY, and Roberts DM

Subjects
Humans, Nalorphine blood, Reproducibility of Results, Spectrometry, Fluorescence, Chromatography, High Pressure Liquid methods, Codeine blood
Abstract

A rapid, reliable and rugged assay for determining codeine in human plasma using reversed-phase high-performance liquid chromatography with fluorescence detection was developed. This analytical method utilized an ion-exchange/mixed-mode solid-phase extraction procedure. The chromatographic separation was achieved using a 150 x 4.6 mm I.D., 3-microns reversed-phase C8 (deactivated for basic analytes) column at ambient temperature. Fluorescence detection (excitation at 214 nm and emission above 345 nm) for codeine and nalorphine allowed for a detectable limit of 5 ng/ml. The results showed that the method was linear from 10 to 300 ng/ml. The method had good reproducibility, precision, accuracy and recoveries of 91 and 90% for codeine and nalorphine, respectively. This method has been applied to study the pharmacokinetics of codeine in normal human subjects.

Published
1995
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6. Protein kinases with calmodulin-like domains: novel targets of calcium signals in plants.

Author

Roberts DM

Subjects
Amino Acid Sequence, Binding Sites, Calcium pharmacology, Enzyme Activation drug effects, Molecular Sequence Data, Sequence Homology, Amino Acid, Calmodulin chemistry, Plants enzymology, Protein Kinases chemistry
Abstract

Recently, a novel calcium-dependent protein kinase has been identified that is structurally distinguished by the localization of a calcium-binding regulatory domain fused to a serine/threonine catalytic domain. The regulatory domain is homologous to calmodulin and contains four helix-loop-helix calcium-binding sites. As a result, the kinase is directly activated by calcium without a requirement for other effector molecules.

Published
1993
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7. Modulation of calmodulin levels, calmodulin methylation, and calmodulin binding proteins during carrot cell growth and embryogenesis.

Author

Oh SH, Steiner HY, Dougall DK, and Roberts DM

Subjects
Calmodulin isolation & purification, Calmodulin-Binding Proteins isolation & purification, Cells, Cultured, Electrophoresis, Polyacrylamide Gel, Kinetics, Methylation, Molecular Weight, Plant Cells, Plant Development, Seeds metabolism, Time Factors, Calmodulin metabolism, Calmodulin-Binding Proteins metabolism, Plants metabolism
Abstract

Carrot cell cultures were used to study the dynamics of calmodulin protein levels, calmodulin methylation, and calmodulin-binding proteins during plant growth and development. Comparisons of proliferating and nonproliferating wild carrot cells show that, while calmodulin protein levels does not vary significantly, substantial variation in post-translational methylation of calmodulin on lysine-115 is observed. Calmodulin methylation is low during the lag and early exponential stages, but increases substantially as exponential growth proceeds and becomes maximal in the postexponential phase. Unmethylated calmodulin quickly reappears within 12 h of reinoculation of cells into fresh media, suggesting that the process is regulated according to the cell growth state. Calmodulin and calmodulin-binding proteins were also analyzed during the formation and germination of domestic carrot embryos in culture. Neither calmodulin methylation nor calmodulin protein levels varied significantly during somatic embryogenesis. However, upon germination of embryos, the level of calmodulin protein doubled. By calmodulin overlay analysis, we have detected a major 54,000 M(r) calmodulin-binding protein that also increased during embryo germination. This protein was purified from carrot embryo extracts by calmodulin-Sepharose chromatography. Overall, the data suggest that calmodulin methylation is regulated depending upon the state of cell growth and that calmodulin and its target proteins are modulated during early plant development.

Published
1992
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9. Calmodulin-binding proteins are developmentally regulated in gametes and embryos of fucoid algae.

Author

Brawley SH and Roberts DM

Subjects
Autoradiography, Calcium Radioisotopes, Calcium-Binding Proteins analysis, Calmodulin analysis, Chromatography, DEAE-Cellulose, Electrophoresis, Polyacrylamide Gel, Immunoblotting, Male, Molecular Weight, Ovum analysis, Phaeophyceae analysis, Spermatozoa analysis, Zygote analysis, Calmodulin-Binding Proteins analysis, Eukaryota growth & development, Phaeophyceae growth & development
Abstract

Calcium-binding proteins and calmodulin-binding proteins were identified in gametes and zygotes of the marine brown algae Fucus vesiculosus, Fucus distichus, and Pelvetia fastigiata using gel (SDS-PAGE) overlay techniques. A calcium current appears to be important during cell polarization in fucoid zygotes (K.R. Robinson and L.F. Jaffe, 1975, Science 187, 70-72; K.R. Robinson and R. Cone, 1980, Science 207, 77-78), but there are no biochemical data on calcium-binding proteins in these algae. By using a sensitive 45Ca2+ overlay method designed to detect high-affinity calcium-binding proteins, at least 9-11 polypeptides were detected in extracts of fucoid gametes and zygotes. All samples had calcium-binding proteins with apparent molecular weights of about 17 and 30 kDa. A 17-kDa calcium-binding protein was purified by calcium-dependent hydrophobic chromatography and was identified as calmodulin by immunological and enzyme activator criteria. A 125I-calmodulin overlay assay was used to identify potential targets of calmodulin action. Sperm contained one major calmodulin-binding protein of about 45 kDa. Eggs lacked major calmodulin-binding activity. A 72-kDa calmodulin-binding protein was prominent in zygotes from 1-65 hr postfertilization. Both calmodulin-binding proteins showed calcium-dependent binding activity. Overall, the data suggest that the appearance and distribution of certain calcium-binding and calmodulin-binding proteins are under developmental regulation, and may reflect the different roles of calcium during fertilization and early embryogenesis.

Published
1989
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11. The -macrofetoprotein response to an inflammatory stimulus in fasted rats.

Author

Weimer HE, Roberts DM, and Comb JC

Subjects
Animal Nutritional Physiological Phenomena, Animals, Body Weight, Fasting, Hematocrit, Hemoglobins metabolism, Inflammation chemically induced, Male, Rats, Stress, Physiological, Turpentine, Fetal Proteins metabolism, Inflammation blood, Mucoproteins blood, Serum Albumin metabolism
Published
1972
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