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306. Thermodynamic model of quasiliquid formation on H2O ice: Comparison with experiment.

Author

Henson, B. F., Voss, L. F., Wilson, Kevin R., and Robinson, J. M.

Subjects
*THERMODYNAMICS, *ATMOSPHERIC chemistry, *SURFACE chemistry, *SEPARATION (Technology), *CRYOSCOPY, *ENTROPY
Abstract

We have developed a new thermodynamic theory of the quasiliquid layer, which has been shown to be effective in modeling the phenomenon in a number of molecular systems. Here we extend our analysis to H2O ice, which has obvious implications for environmental and atmospheric chemistry. In the model, the liquid layer exists in contact with an ice defined as a two-dimensional lattice of sites. The system free energy is defined by the bulk free energies of ice Ih and liquid water and is minimized in the grand canonical ensemble. An additional configurational entropy term arises from the occupation of the lattice sites. Furthermore, the theory predicts that the layer thickness as a function of temperature depends only on the liquid activity. Two additional models are derived, where slightly different approximations are used to define the free energy. With these two models, we illustrate the connection between the quasiliquid phenomenon and multilayer adsorption and the possibility of a two-dimensional phase transition connecting a dilute low coverage phase of adsorbed H2O and the quasiliquid phase. The model predictions are in agreement with a subset of the total suite of experimental measurements of the liquid thickness on H2O ice as a function of temperature. The theory indicates that the quasiliquid layer is actually equivalent to normal liquid water, and we discuss the impact of such an identification. In particular, observations of the liquid layer to temperatures as low as 200 K indicate the possibility that the quasiliquid is, in fact, an example of deeply supercooled normal water. Finally, we briefly discuss the obvious extension of the pure liquid theory to a thermodynamic theory of interfacial solutions on ice in the environment. [ABSTRACT FROM AUTHOR]

Published
2005
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307. Architectural studies.

Author

Robinson, J. M.

Abstract

The article reviews several books related to architecture, including "Athenian Stuart: Pioneer of the Greek Revival," by David Watkin, "William Talman: Maverick Architect," by John Harris, and "Architects of the Arts and Crafts Movement," by Margaret Richardson.

Published
1984

312. A Fermi-degenerate three-dimensional optical lattice clock.

Author

Campbell, S. L., Hutson, R. B., Marti, G. E., Goban, A., Darkwah Oppong, N., McNally, R. L., Sonderhouse, L., Robinson, J. M., Zhang, W., Bloom, B. J., and Ye, J.

Subjects
*OPTICAL lattices, *ELECTRON gas, *FERMI level, *CLOCKS & watches, *TIME measurements, *LATTICE dynamics
Abstract

Strontium optical lattice clocks have the potential to simultaneously interrogate millions of atoms with a high spectroscopic quality factor of 4 × 1017. Previously, atomic interactions have forced a compromise between clock stability, which benefits from a large number of atoms, and accuracy, which suffers from density-dependent frequency shifts. Here we demonstrate a scalable solution that takes advantage of the high, correlated density of a degenerate Fermi gas in a three-dimensional (3D) optical lattice to guard against on-site interaction shifts. We show that contact interactions are resolved so that their contribution to clock shifts is orders of magnitude lower than in previous experiments. A synchronous clock comparison between two regions of the 3D lattice yields a measurement precision of 5 × 10–19 in 1 hour of averaging time. [ABSTRACT FROM AUTHOR]

Published
2017
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313. Kinetics of the β–δ Phase Transition in PBX 9501.

Author

Smilowitz, L. B., Henson, B. F., Asay, B. W., Dickson, P. M., and Robinson, J. M.

Subjects
*PHASE transitions, *EXPLOSIVES, *DYNAMICS
Abstract

The initial step in the thermal decomposition of HMX is the solid state phase transition from the centrosymmetric beta form to the noncentrosymmetric delta form. The symmetry change makes the phase transition amenable to the application of second harmonic generation (SHG) as a probe of transition kinetics. We have used SHG to study the temperature dependence of the kinetics for unconfined PBX9501 and HMX. Spatially resolved SHG measurements have shown a nucleation and growth mechanism for the solid state phase transition. We have measured the transition rate as a function of temperature in order to obtain the activation energy and entropy of transition, which determine the phase transition kinetics. Additionally, we have observed temperature dependent reversion of the delta phase to beta phase and have found that we can control the reversion rate by controlling the cooling. [ABSTRACT FROM AUTHOR]

Published
2002

314. Mechanically evoked 5-hydroxytryptamine release is mediated by caveolin-associated cholesterol rich membrane domains.

Author

Kim, M., Christofi, F. L., Xue, J., Robinson, J. M., and Cooke, H. J.

Subjects
*SEROTONIN, *CELLS, *SECRETION, *IMMUNOFLUORESCENCE, *CHOLESTEROL, *CYCLODEXTRINS
Abstract

5-Hydroxytryptamine (5-HT) from enterochromaffin cells activates neural reflexes that govern intestinal motility and secretion. Mechanical stimulation of human enterochromaffin cell-derived BON cells activates a G αq-signalling pathway coupled to 5-HT release. Molecular mechanisms identifying elements of mechanosensory transduction are unknown. The aim of this study was to determine the role of caveolin and caveolin-associated cholesterol rich microdomains in mechanically stimulated 5-HT release from BON cells. Caveolin-1 transcripts and immunofluorescence were found in BON cells. In the static state, caveolins-1 and -2 co-precipitated with G αq in cholesterol rich cell fractions, but not with G αs, G αi/o and G β. Mechanical stimulation transiently uncoupled G αq from caveolin-1 and increased 5-HT release. Disassembly of caveolin-associated membrane microdomains by filipin or by cholesterol depletion with methyl- β-cyclodextrin decreased mechanically evoked 5-HT release. These results suggest that caveolin and caveolin-associated cholesterol rich membrane microdomains are key regulators in mechanically evoked 5-HT release from enterochromaffin cells. [ABSTRACT FROM AUTHOR]

Published
2007
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315. Immunomodulation in Type 1 Diabetes by NBI-6024, an Altered Peptide Ligand of the Insulin B(9−23) Epitope.

Author

Alleva, D. G., Maki, R. A., Putnam, A. L., Robinson, J. M., Kipnes, M. S., Dandona, P., Marks, J. B., Simmons, D. L., Greenbaum, C. J., Jimenez, R. G., Conlon, P. J., and Gottlieb, P. A.

Subjects
*IMMUNOREGULATION, *DIABETES, *LIGANDS (Biochemistry), *AMINO acids, *INSULIN, *PEOPLE with diabetes, *LYMPHOCYTES, *CLINICAL trials
Abstract

NBI-6024 is an altered peptide ligand (APL) corresponding to the 9–23 amino acid region of the insulin B chain (B(9−23)), an epitope recognized by inflammatory interferon-γ-producing T helper (Th)1 lymphocytes in type 1 diabetic patients. Immunomodulatory effects of NBI-6024 administration in recent-onset diabetic patients in a phase I clinical trial (NBI-6024-0003) were measured in peripheral blood mononuclear cells using the enzyme-linked immunosorbent spot assay. Analysis of the mean magnitude of cytokine responses to B(9−23) and NBI-6024 for each cohort showed significant increases in interleukin-5 responses (a Th2 regulatory phenotype) in cohorts that received APL relative to those receiving placebo. A responder analysis showed that Th1 responses to B(9−23) and NBI-6024 were observed almost exclusively in the placebo-treated diabetic population but not in nondiabetic control subjects and that APL administration (five biweekly subcutaneous injections) significantly and dose-dependently reduced the percentage of patients with these Th1 responses. The results of this phase I clinical study strongly suggest that NBI-6024 treatment shifted the Th1 pathogenic responses in recent-onset type 1 diabetic patients to a protective Th2 regulatory phenotype. The significance of these findings on the clinical outcome of disease is currently under investigation in a phase II multidose study. [ABSTRACT FROM AUTHOR]

Published
2006
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316. Cathepsin D, but not cathepsin E, degrades desmosomes during epidermal desquamation.

Author

Igarashi, S., Takizawa, T., Yasuda, Y., Uchiwa, H., Hayashi, S., Brysk, H., Robinson, J. M., Yamamoto, K., Brysk, M. M., and Horikoshi, T.

Subjects
*ASPARTIC proteinases, *ASPARTIC acid, *IMMUNOCYTOCHEMISTRY, *IMMUNOFLUORESCENCE, *CHEMICAL inhibitors, *DESMOSOMES, *EPITHELIAL cells
Abstract

We previously reported that an ambient aspartic proteinase is crucial to desquamation of the stratum corneum at pH 5. Identification of this aspartic proteinase by using enzyme inhibitors suggested it to be cathepsin D, although we could not exclude cathepsin E. To determine the identity of this aspartic proteinase and its distribution within the stratum corneum. We measured enzyme activities of cathepsin D and cathepsin E in the salt and detergent extracts from callus stratum corneum, using a fluorogenic peptide as a substrate and comparing the effect of addition of Ascaris pepsin inhibitor (specific for cathepsin E) with that of pepstatin A (which inhibits both cathepsin D and cathepsin E). Both enzymes were then extracted and purified from plantar stratum corneum samples and identified by Western blotting. Immunofluorescence microscopy was used to investigate the localization of proteinases within human plantar stratum corneum sample sections. We found that 20% of total aspartic proteinase activity could be attributed to cathepsin E, the remainder to cathepsin D. Two subunits of cathepsin D were identified, a mature active form at 33 kDa and an intermediate active form at 48 kDa; cathepsin E was also identified at 48 kDa, although in a stained band 10-fold weaker in the immunoblot. Immunofluorescence microscopy showed the antibody to cathepsin D to be localized in the lipid envelopes of the stratum corneum, whereas that to cathepsin E stained the tissue diffusely. The labelling for cathepsin D was similar to that observed for desmosomes, and immunoelectron microscopy confirmed that cathepsin D was present on desmosomes. On the other hand, cathepsin E occurred intracellularly within the squames. We conclude that cathepsin D, and not cathepsin E, causes desquamation by degrading desmosomes. [ABSTRACT FROM AUTHOR]

Published
2004
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317. 1.5 μm Lasers with Sub-10 mHz Linewidth.

Author

Matei, D. G., Legero, T., Häfner, S., Grebing, C., Weyrich, R., Zhang, W., Sonderhouse, L., Robinson, J. M., Ye, J., Riehle, F., and Sterr, U.

Subjects
*LASERS, *SILICON
Abstract

We report on two ultrastable lasers each stabilized to independent silicon Fabry-Pérot cavities operated at 124 K. The fractional frequency instability of each laser is completely determined by the fundamental thermal Brownian noise of the mirror coatings with a flicker noise floor of 4×10-17 for integration times between 0.8 s and a few tens of seconds. We rigorously treat the notorious divergences encountered with the associated flicker frequency noise and derive methods to relate this noise to observable and practically relevant linewidths and coherence times. The individual laser linewidth obtained from the phase noise spectrum or the direct beat note between the two lasers can be as small as 5 mHz at 194 THz. From the measured phase evolution between the two laser fields we derive usable phase coherence times for different applications of 11 to 55 s. [ABSTRACT FROM AUTHOR]

Published
2017
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318. Flavor-specific enhancement of electronic cigarette liquid consumption and preference in mice.

Author

Wong AL, McElroy SM, Robinson JM, Mulloy SM, El Banna FK, Harris AC, LeSage MG, and Lee AM

Subjects
Animals, Choice Behavior drug effects, Fruit, Male, Mice, Mice, Inbred C57BL, Taste drug effects, Nicotiana, Choice Behavior physiology, Electronic Nicotine Delivery Systems, Flavoring Agents administration & dosage, Nicotine administration & dosage, Taste physiology
Abstract

Background: The use of electronic cigarettes has increased over the past decade. To determine how the abuse liability of electronic cigarette liquids (e-liquids) differs from nicotine alone, and to determine the impact of flavor, we compared nicotine-containing fruit- and tobacco-flavored e-liquids, and their nicotine-free versions, to nicotine alone in mouse models of oral consumption, reward and aversion., Methods: Adult male C57BL/6 J mice voluntarily consumed oral nicotine, equivalent nicotine concentrations of fruit- and tobacco-flavored e-liquid, and equivalent dilutions of the nicotine-free versions in 2-bottle choice tests. Conditioned place preference and place aversion were assessed with peripherally administered e-liquids or nicotine. Serum nicotine and cotinine levels were measured after subcutaneous injections of e-liquid or nicotine., Results: Mice showed higher consumption and preference for the fruit-flavored e-liquid compared with nicotine alone. This increase was not due to the flavor itself as consumption of the nicotine-free fruit-flavored e-liquid was not elevated until the highest concentration tested. The increased consumption and preference were not observed with the tobacco-flavored e-liquid. The conditioned place preference, place aversion and nicotine pharmacokinetics of the fruit-flavored e-liquid were not significantly different from nicotine alone., Conclusions: Our data suggest that fruit, but not tobacco flavor, increased the oral consumption of e-liquid compared with nicotine alone. Moreover, this enhancement was not due to increased consumption of the flavor itself, altered rewarding or aversive properties after peripheral administration, or altered pharmacokinetics. This flavor-specific enhancement suggests that some flavors may lead to higher nicotine intake and increased use of e-liquids compared with nicotine alone., Competing Interests: Declaration of Competing Interest The authors declare no conflicts of interest., (Copyright © 2020 Elsevier B.V. All rights reserved.)

Published
2020
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319. Differential gene expression and gene-set enrichment analysis in Caco-2 monolayers during a 30-day timeline with Dexamethasone exposure.

Author

Robinson JM, Turkington S, Abey SA, Kenea N, and Henderson WA

Subjects
Caco-2 Cells, Dexamethasone pharmacology, Humans, Time Factors, Cytoskeleton drug effects, Dexamethasone therapeutic use, Gene Expression genetics
Abstract

Glucocorticoid hormones affect gene expression via activation of glucocorticoid receptor NR3C1, causing modulation of inflammation and autoimmune activation. The glucocorticoid Dexamethasone is an important pharmaceutical for the treatment of colitis and other inflammatory bowel diseases. While suppressive effects of glucocorticoids on activated immune cells is significant, their effects upon epithelial cells are less well studied. Previous research shows that the effects of Dexamethasone treatment on polarized Caco-2 cell layer permeability is delayed for >10 treatment days (as measured by transepithelial electrical resistance). In vivo intestinal epithelial cells turn over every 3-5 days; we therefore hypothesized that culture age may produce marked effects on gene expression, potentially acting as a confounding variable. To investigate this issue, we cultured polarized Caco-2 monolayers during a 30-day timecourse with ~15 days of continuous Dexamethasone exposure. We collected samples during the timecourse and tested differential expression using a 250-plex gene expression panel and Nanostring nCounter® system. Our custom panel was selectively enriched for KEGG annotations for tight-junction, actin cytoskeleton regulation, and colorectal cancer-associated genes, allowing for focused gene ontology-based pathway enrichment analyses. To test for confounding effects of time and Dexamethasone variables, we used the Nanostring nSolver differential expression data model which includes a mixturenegative binomial modelwith optimization. We identified a time-associated "EMT-like" signature with differential expression seen in important actomyosin cytoskeleton, tight junction, integrin, and cell cycle pathway genes. Dexamethasone treatment resulted in a subtle yet significant counter-signal showing suppression of actomyosin genes and differential expression of various growth factor receptors.

Published
2019
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320. Modelling the structure of a ceRNA-theoretical, bipartite microRNA-mRNA interaction network regulating intestinal epithelial cellular pathways using R programming.

Author

Robinson JM and Henderson WA

Subjects
Databases, Genetic, Humans, Adherens Junctions metabolism, Epithelial Cells metabolism, Intestinal Mucosa metabolism, MicroRNAs metabolism, Models, Genetic, RNA, Messenger metabolism, Signal Transduction, Tight Junctions metabolism
Abstract

Objective: We report a method using functional-molecular databases and network modelling to identify hypothetical mRNA-miRNA interaction networks regulating intestinal epithelial barrier function. The model forms a data-analysis component of our cell culture experiments, which produce RNA expression data from Nanostring Technologies nCounter ® system. The epithelial tight-junction (TJ) and actin cytoskeleton interact as molecular components of the intestinal epithelial barrier. Upstream regulation of TJ-cytoskeleton interaction is effected by the Rac/Rock/Rho signaling pathway and other associated pathways which may be activated or suppressed by extracellular signaling from growth factors, hormones, and immune receptors. Pathway activations affect epithelial homeostasis, contributing to degradation of the epithelial barrier associated with osmotic dysregulation, inflammation, and tumor development. The complexity underlying miRNA-mRNA interaction networks represents a roadblock for prediction and validation of competing-endogenous RNA network function., Results: We developed a network model to identify hypothetical co-regulatory motifs in a miRNA-mRNA interaction network related to epithelial function. A mRNA-miRNA interaction list was generated using KEGG and miRWalk2.0 databases. R-code was developed to quantify and visualize inherent network structures. We identified a sub-network with a high number of shared, targeting miRNAs, of genes associated with cellular proliferation and cancer, including c-MYC and Cyclin D.

Published
2018
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321. Exocyst complex protein expression in the human placenta.

Author

Gonzalez IM, Ackerman WE 4th, Vandre DD, and Robinson JM

Subjects
Cell Differentiation, Exocytosis, Female, Humans, Immunohistochemistry, Microscopy, Confocal, Models, Biological, Placenta cytology, Pregnancy, Trophoblasts cytology, Trophoblasts metabolism, rab GTP-Binding Proteins metabolism, Placenta metabolism, Vesicular Transport Proteins metabolism
Abstract

Introduction: Protein production and secretion are essential to syncytiotrophoblast function and are associated with cytotrophoblast cell fusion and differentiation. Syncytiotrophoblast hormone secretion is a crucial determinant of maternal-fetal health, and can be misregulated in pathological pregnancies. Although, polarized secretion is a key component of placental function, the mechanisms underlying this process are poorly understood., Objective: While the octameric exocyst complex is classically regarded as a master regulator of secretion in various mammalian systems, its expression in the placenta remained unexplored. We hypothesized that the syncytiotrophoblast would express all exocyst complex components and effector proteins requisite for vesicle-mediated secretion more abundantly than cytotrophoblasts in tissue specimens., Methods: A two-tiered immunobiological approach was utilized to characterize exocyst and ancillary proteins in normal, term human placentas. Exocyst protein expression and localization was documented in tissue homogenates via immunoblotting and immunofluorescence labeling of placental sections., Results: The eight exocyst proteins, EXOC1, 2, 3, 4, 5, 6, 7, and 8, were found in the human placenta. In addition, RAB11, an important exocyst complex modulator, was also expressed. Exocyst and Rab protein expression appeared to be regulated during trophoblast differentiation, as the syncytiotrophoblast expressed these proteins with little, if any, expression in cytotrophoblast cells. Additionally, exocyst proteins were localized at or near the syncytiotrophoblast apical membrane, the major site of placental secretion., Discussion/conclusion: Our findings highlight exocyst protein expression as novel indicators of trophoblast differentiation. The exocyst's regulated localization within the syncytiotrophoblast in conjunction with its well known functions suggests a possible role in placental polarized secretion., (Copyright © 2014 Elsevier Ltd. All rights reserved.)

Published
2014
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322. TEMS: results of a specialist centre.

Author

Flexer SM, Durham-Hall AC, Steward MA, and Robinson JM

Subjects
Adenocarcinoma pathology, Adenoma pathology, Adult, Aged, Aged, 80 and over, Female, Follow-Up Studies, Humans, Intraoperative Complications surgery, Male, Neoplasm Recurrence, Local pathology, Neoplasm Recurrence, Local surgery, Neoplasm Staging, Operative Time, Preoperative Care, Prospective Studies, Rectal Neoplasms pathology, Surgical Stomas, Adenocarcinoma surgery, Adenoma surgery, Colonic Polyps surgery, Endoscopy methods, Microsurgery methods, Rectal Neoplasms surgery
Abstract

Introduction: Transanal endoscopic microsurgery (TEMS) is becoming more widespread due to the increasing body of evidence to support its role. Previous published data has reported recurrence rates in excess of 10% for benign polyps after TEMS., Methods: Bradford Royal Infirmary is a tertiary referral centre for TEMS and early rectal cancer in the UK. Data for all TEMS operations were entered into a prospective database over a 7-year period. Demographic data, complications and recurrence rates were recorded. Both benign adenomas and malignant lesions were included., Results: A total of 164 patients (65% male), with a mean age of 68 years were included; 114 (70%) of the lesions resected were benign adenomas, and 50 (30%) were malignant lesions. Median polyp size was 4 (range 0.6-14.5) cm. Mean length of operation was 55 (range 10-120) min. There were no recurrences in any patients with a benign adenoma resected; two patients with malignant lesions developed recurrences. Three intra-operative complications were recorded, two rectal perforations (repaired primarily, one requiring defunctioning stoma), and a further patient suffered a blood loss of >300 ml requiring transfusion. Six patients developed strictures requiring dilation either endoscopically or under anaesthetic in the post-operative period., Conclusions: We have demonstrated that TEMS procedures performed in a specialist centre provide low rates of both recurrence and complication. Within a specialist centre, TEMS surgery should be offered to all patients for rectal lesions, both benign and malignant, that are amenable to TEMS.

Published
2014
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323. IFPA Meeting 2012 Workshop Report I: comparative placentation and animal models, advanced techniques in placental histopathology, human pluripotent stem cells as a model for trophoblast differentiation.

Author

Ackerman WE 4th, Carter AM, De Mestre AM, Golos TG, Jeschke U, Kusakabe K, Laurent LC, Parast MM, Roberts RM, Robinson JM, Rutherford J, Soma H, Takizawa T, Ui-Tei K, and Lash GE

Subjects
Animals, Female, Humans, Placenta cytology, Pregnancy, Cell Differentiation physiology, Models, Animal, Placenta pathology, Placentation physiology, Pluripotent Stem Cells physiology, Trophoblasts physiology
Abstract

Workshops are an important part of the IFPA annual meeting as they allow for discussion of specialized topics. At IFPA meeting 2012 there were twelve themed workshops, three of which are summarized in this report. These workshops related to various aspects of placental biology but collectively covered areas of models and technical issues involved in placenta research: 1) comparative placentation and animal models; 2) advanced techniques in placental histopathology; 3) human pluripotent stem cells as a model for trophoblast differentiation., (Copyright © 2012 Elsevier Ltd. All rights reserved.)

Published
2013
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324. A placental sub-proteome: the apical plasma membrane of the syncytiotrophoblast.

Author

Vandré DD, Ackerman WE 4th, Tewari A, Kniss DA, and Robinson JM

Subjects
Cell Fractionation, Cell Membrane chemistry, Cell Polarity physiology, Chorionic Villi chemistry, Chorionic Villi metabolism, Female, Humans, Placenta chemistry, Placenta metabolism, Placenta ultrastructure, Pregnancy, Proteome metabolism, Proteomics methods, Trophoblasts chemistry, Cell Membrane metabolism, Proteome analysis, Trophoblasts metabolism, Trophoblasts ultrastructure
Abstract

As a highly vascularized tissue, the placenta mediates gas and solute exchange between maternal and fetal circulations. In the human placenta, the interface with maternal blood is a unique epithelial structure known as the syncytiotrophoblast. Previously we developed a colloidal-silica based method to generate highly enriched preparations of the apical plasma membrane of the syncytiotrophoblast. Using similar preparations, a proteomics assessment of this important sub-proteome has identified 340 proteins as part of this apical membrane fraction. The expression of 38 of these proteins was previously unknown in the human placental syncytiotrophoblast. Together with previous studies, the current proteomic database expands our knowledge of the proteome of the syncytiotrophoblast apical plasma membrane from normal placentas to include more than 500 proteins. This database is a valuable resource for future comparisons to diseased placentas. Additionally, this data set provides a basis for further experimental studies of placenta and trophoblast function., (Copyright © 2011 Elsevier Ltd. All rights reserved.)

Published
2012
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325. Preoperative portal vein embolization tailored to prepare the liver for complex resections: initial experience.

Author

de Baere T, Robinson JM, Deschamps F, Rao P, Teriitheau C, Goere D, and Elias D

Subjects
Adult, Aged, Angiography methods, Child, Cohort Studies, Disease-Free Survival, Female, Follow-Up Studies, Hepatectomy methods, Humans, Liver Neoplasms mortality, Liver Neoplasms pathology, Male, Middle Aged, Neoplasm Staging, Portal Vein, Preoperative Care methods, Retrospective Studies, Risk Assessment, Survival Analysis, Tomography, X-Ray Computed methods, Treatment Outcome, Embolization, Therapeutic methods, Liver Neoplasms secondary, Liver Neoplasms therapy, Radiography, Interventional
Abstract

The purpose of this study was to evaluate the safety and efficacy of preoperative portal vein embolization (PVE) tailored to prepare the liver for complex and extended resections. During the past 5 years, 12 PVEs were performed in noncirrhotic patients with liver metastases from colon cancer (n = 10), choroidal melanoma (n = 1), and leiomyosarcoma (n = 1) to prepare complex anatomical liver resections in patients with small future remnant livers. These liver resections planned to preserve only segment IV in four patients, segments IV, V, and VIII in four patients, segments II, III, VI, and VII in three patients, and segments V and VI in one patient. PVE was performed under general anesthesia with a flow-guided injection of a mixture of cyanoacrylate and Lipiodol using a 5-Fr catheter. All portal branches feeding the liver segments to be resected were successfully embolized with cyanoacrylate except one, which was occluded with coils due to the risk of reflux with cyanoacrylate. After a mean of 32 days, CT volumetry revealed a mean hypertrophy of the unembolized liver of 47 +/- 25% (range, 21-88%). Liver resections could be performed in 10 patients but were canceled in 2, due to the occurrence of a new hepatic tumor in one and an insufficiently increased volume in the other. Among the 10 patients who underwent the liver resection, 1 died of postoperative sepsis, 3 died 3 to 32 months after surgery, including 1 death unrelated to cancer, and 6 were alive after 6 to 36 months after surgery. In conclusion, in this preliminary report, PVE appears to be feasible and able to induce hypertrophy of the future remnant liver before a complex and extended hepatectomy. Further evaluation is needed in a larger cohort.

Published
2010
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326. The expression of caveolin-1 and the distribution of caveolae in the murine placenta and yolk sac: parallels to the human placenta.

Author

Mohanty S, Anderson CL, and Robinson JM

Subjects
Animals, Cell Polarity, Endoderm metabolism, Endoderm ultrastructure, Endothelial Cells metabolism, Endothelial Cells ultrastructure, Female, Fluorescent Antibody Technique, Indirect, Humans, Mice, Mice, Inbred BALB C, Microscopy, Confocal, Microscopy, Fluorescence, Myocytes, Smooth Muscle metabolism, Myocytes, Smooth Muscle ultrastructure, Pregnancy, Protein Transport, Species Specificity, Trophoblasts metabolism, Trophoblasts ultrastructure, Caveolae ultrastructure, Caveolin 1 metabolism, Placenta metabolism, Placenta ultrastructure, Pregnancy Proteins metabolism, Yolk Sac metabolism, Yolk Sac ultrastructure
Abstract

The expression pattern of caveolin-1 and the distribution of caveolae in the murine placental labyrinth and visceral yolk sac have been determined. Immunoblot analysis demonstrates that both placenta and yolk sac express the protein caveolin-1. Immunofluorescence microscopy was used to determine which cell types in the placental labyrinth and yolk sac express caveolin-1. In yolk sac, detectable caveolin-1 was restricted to endothelial cells and smooth muscle cells of the vitelline vasculature and to mesothelial cells. Endoderm, the major cell type in the yolk sac, does not express caveolin-1 as assessed by this assay. In the labyrinth region of the placenta, endothelial cells express caveolin-1 but this protein was not detectable in any of the three trophoblast layers. These tissues were also examined by electron microscopy to determine which cell types contain the specialized plasma membrane microdomains known as caveolae. Morphologically detectable caveolae were present in endothelial and smooth muscle cells, as well as mesothelial cells of the yolk sac and in endothelial cells of the placental labyrinth. Neither endodermal cells of the yolk sac nor trophoblastic cells in the placental labyrinth contained caveolae-like structures. We conclude that caveolin-1 and caveolae have restricted distribution in the murine placenta and yolk sac and that this parallels the situation in human placenta., (Copyright 2009. Published by Elsevier Ltd.)

Published
2010
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327. Where's the glass? Biomarkers, molecular clocks, and microRNAs suggest a 200-Myr missing Precambrian fossil record of siliceous sponge spicules.

Author

Sperling EA, Robinson JM, Pisani D, and Peterson KJ

Subjects
Animals, Biomarkers, Phylogeny, Porifera classification, Fossils, MicroRNAs genetics, Porifera genetics, Porifera metabolism
Abstract

The earliest evidence for animal life comes from the fossil record of 24-isopropylcholestane, a sterane found in Cryogenian deposits, and whose precursors are found in modern demosponges, but not choanoflagellates, calcareans, hexactinellids, or eumetazoans. However, many modern demosponges are also characterized by the presence of siliceous spicules, and there are no convincing demosponge spicules in strata older than the Cambrian. This temporal disparity highlights a problem with our understanding of the Precambrian fossil record--either these supposed demosponge-specific biomarkers were derived from the sterols of some other organism and are simply retained in modern demosponges, or spicules do not primitively characterize crown-group demosponges. Resolving this issue requires resolving the phylogenetic placement of another group of sponges, the hexactinellids, which not only make a spicule thought to be homologous to the spicules of demosponges, but also make their first appearance near the Precambrian/Cambrian boundary. Using two independent analytical approaches and data sets--traditional molecular phylogenetic analyses and the presence or absence of specific microRNA genes--we show that demosponges are monophyletic, and that hexactinellids are their sister group (together forming the Silicea). Thus, spicules must have evolved before the last common ancestor of all living siliceans, suggesting the presence of a significant gap in the silicean spicule fossil record. Molecular divergence estimates date the origin of this last common ancestor well within the Cryogenian, consistent with the biomarker record, and strongly suggests that siliceous spicules were present during the Precambrian but were not preserved.

Published
2010
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328. Correlative fluorescence and electron microscopy in tissues: immunocytochemistry.

Author

Robinson JM and Takizawa T

Subjects
Chorionic Villi chemistry, Chorionic Villi ultrastructure, Fluorescence, Gold, Humans, Image Processing, Computer-Assisted methods, Nanoparticles, Neutrophils chemistry, Neutrophils ultrastructure, Microscopy, Fluorescence methods, Microscopy, Immunoelectron methods, Staining and Labeling methods
Abstract

Correlative microscopy is a collection of procedures that rely upon two or more imaging modalities to examine the same specimen. The imaging modalities employed should each provide unique information and the combined correlative data should be more information rich than that obtained by any of the imaging methods alone. Currently the most common form of correlative microscopy combines fluorescence and electron microscopy. While much of the correlative microscopy in the literature is derived from studies of model cell culture systems we have focused, primarily, on correlative microscopy in tissue samples. The use of tissue, particularly human tissue, may add constraints not encountered in cell culture systems. Ultrathin cryosections, typically used for immunoelectron microscopy, have served as the substrate for correlative fluorescence and electron microscopic immunolocalization in our studies. In this work, we have employed the bifunctional reporter FluoroNanogold. This labeling reagent contains both a fluorochrome and a gold-cluster compound and can be imaged by sequential fluorescence and electron microscopy. This approach permits the examination of exactly the same sub-cellular structures in both fluorescence and electron microscopy with a high level of spatial resolution.

Published
2009
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329. Placental dysferlin expression is reduced in severe preeclampsia.

Author

Lang CT, Markham KB, Behrendt NJ, Suarez AA, Samuels P, Vandre DD, Robinson JM, and Ackerman WE 4th

Subjects
Adolescent, Adult, Calcium-Binding Proteins, Case-Control Studies, Cell Membrane metabolism, Cell-Derived Microparticles metabolism, Cross-Sectional Studies, Down-Regulation, Dysferlin, Female, Humans, Microscopy, Fluorescence, Middle Aged, Pregnancy, RNA, Messenger genetics, RNA, Messenger metabolism, Tissue Distribution, Trophoblasts metabolism, Young Adult, Membrane Proteins genetics, Membrane Proteins metabolism, Muscle Proteins genetics, Muscle Proteins metabolism, Placenta metabolism, Pre-Eclampsia genetics, Pre-Eclampsia metabolism
Abstract

Dysferlin (DYSF) and myoferlin (MYOF), members of the ferlin family of membrane proteins, are co-expressed in human placental syncytiotrophoblast (STB). Although the role of these ferlin proteins in the placenta has yet to be established, it has been suggested that DYSF and MYOF may contribute to the stability of the apical STB plasma membrane. The release of STB-derived cellular debris increases in the setting of preeclampsia (PE), suggesting relative destabilization of the hemochorial interface. To test whether PE was associated with alterations in placental expression of DYSF and/or MYOF, a cross-sectional study was performed using specimens of villous placenta collected form women with severe PE (n=10) and normotensive controls (n=10). DYSF and MYOF expression were examined using quantitative real-time RT-PCR, immunoblotting, and immunofluorescence labeling of tissue specimens. Placental DYSF expression was 57% lower at the mRNA level (p=0.03) and 38% lower at the protein level (p=0.026) in severe PE as compared to normotensive subjects. There were no differences in placental MYOF protein or mRNA expression between these groups. No appreciable changes in the distribution of DYSF or MYOF within placental villi was observed in PE relative to control specimens. We conclude that DYSF expression is reduced in severe PE relative to gestational age-matched controls. As DYSF has a role in membrane repair, these data suggest a role for DYSF in the stability of the apical STB plasma membrane and may account, at least in part, for the increased shedding of microparticles from this membrane in PE.

Published
2009
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330. Placental proteomics: a shortcut to biological insight.

Author

Robinson JM, Vandré DD, and Ackerman WE 4th

Subjects
Calcium-Binding Proteins, Cell Membrane chemistry, Dysferlin, Female, Humans, Membrane Proteins metabolism, Muscle Proteins metabolism, Pregnancy, Proteomics methods, Trophoblasts ultrastructure, Placenta metabolism, Trophoblasts metabolism
Abstract

Proteomics analysis of biological samples has the potential to identify novel protein expression patterns and/or changes in protein expression patterns in different developmental or disease states. An important component of successful proteomics research, at least in its present form, is to reduce the complexity of the sample if it is derived from cells or tissues. One method to simplify complex tissues is to focus on a specific, highly purified sub-proteome. Using this approach we have developed methods to prepare highly enriched fractions of the apical plasma membrane of the syncytiotrophoblast. Through proteomics analysis of this fraction we have identified over five hundred proteins several of which were previously not known to reside in the syncytiotrophoblast. Herein, we focus on two of these, dysferlin and myoferlin. These proteins, largely known from studies of skeletal muscle, may not have been found in the human placenta were it not for discovery-based proteomics analysis. This new knowledge, acquired through a discovery-driven approach, can now be applied for the generation of hypothesis-based experimentation. Thus discovery-based and hypothesis-based research are complimentary approaches that when coupled together can hasten scientific discoveries.

Published
2009
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331. Proteomics of the human placenta: promises and realities.

Author

Robinson JM, Ackerman WE 4th, Kniss DA, Takizawa T, and Vandré DD

Subjects
Cells, Cultured, Humans, Physiology, Comparative, Placenta metabolism, Proteomics trends
Abstract

Proteomics is an area of study that sets as its ultimate goal the global analysis of all of the proteins expressed in a biological system of interest. However, technical limitations currently hamper proteome-wide analyses of complex systems. In a more practical sense, a desired outcome of proteomics research is the translation of large protein data sets into formats that provide meaningful information regarding clinical conditions (e.g., biomarkers to serve as diagnostic and/or prognostic indicators of disease). Herein, we discuss placental proteomics by describing existing studies, pointing out their strengths and weaknesses. In so doing, we strive to inform investigators interested in this area of research about the current gap between hyperbolic promises and realities. Additionally, we discuss the utility of proteomics in discovery-based research, particularly as regards the capacity to unearth novel insights into placental biology. Importantly, when considering under studied systems such as the human placenta and diseases associated with abnormalities in placental function, proteomics can serve as a robust 'shortcut' to obtaining information unlikely to be garnered using traditional approaches.

Published
2008
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332. Association of PAT proteins with lipid storage droplets in term fetal membranes.

Author

Ackerman WE 4th, Robinson JM, and Kniss DA

Subjects
3T3 Cells, Animals, DNA Primers, Female, Goats, Guinea Pigs, Mice, Pregnancy, Rabbits, Reverse Transcriptase Polymerase Chain Reaction, Amino Acid Transport Systems, Neutral genetics, Amnion metabolism, Extraembryonic Membranes metabolism, Lipids physiology, Symporters genetics
Abstract

As depots for neutral lipids, lipid storage droplets (LDs) accumulate with advancing gestation within the fetal membranes. Little is currently known about the proteins associated with the LDs of these cells. The PAT family [perilipin, adipose differentiation-related protein (ADRP), and tail-interacting protein of 47 kilodaltons (TIP47)] represents a unique group of proteins thought to contribute to LD formation and function. We examined the association of each of the PAT proteins with LDs of term fetal membranes. We found that large LDs of amnion epithelial cells were reactive for neutral lipid stains and simultaneously encoated with ADRP and TIP47, but not perilipin. Within the remaining cell types, LDs were frequently co-labeled with antibodies recognizing ADRP and TIP47; however, in cells harboring only small LDs, the majority of TIP47 labeling was cytoplasmic. Structures labeled with perilipin antibodies were present only in chorion laeve trophoblasts. Gene and protein expression analyses suggested this to be a small molecular weight perilipin isoform, such as that seen in steroidogenic cells. We conclude that LDs are heterogeneous among differing cell types of the fetal membranes. Subclassification of LDs based on associated proteins suggests that these organelles may serve specialized functions within individual cells.

Published
2007
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333. Endothelial expression of Fc gamma receptor IIb in the full-term human placenta.

Author

Mishima T, Kurasawa G, Ishikawa G, Mori M, Kawahigashi Y, Ishikawa T, Luo SS, Takizawa T, Goto T, Matsubara S, Takeshita T, Robinson JM, and Takizawa T

Subjects
Female, Gene Expression, Humans, Microscopy, Fluorescence, Placenta blood supply, Pregnancy Trimester, Third metabolism, Reverse Transcriptase Polymerase Chain Reaction, Sequence Analysis, RNA, Endothelial Cells metabolism, Endothelium, Vascular metabolism, Placenta metabolism, Pregnancy metabolism, Receptors, IgG metabolism
Abstract

In the third trimester, human placental endothelial cells express Fc gamma receptor IIb (FcgammaRIIb). This expression is unique because FcgammaRIIb is generally expressed on immune cells and is typically undetectable in adult endothelial cells. Recently, we found a novel FcgammaRIIb-defined, IgG-containing organelle in placental endothelial cells; this organelle may be a key structure for the transcytosis of IgG across the endothelial layer. In this study, we verify the expression of FcgammaRIIb in endothelial placenta cells and use reverse transcriptase-polymerase chain reaction (RT-PCR) and sequencing analyses to define the expressed FCGR2B mRNA transcript variant. We also investigated the distribution of FCGR2B mRNA and protein within the vascular tree of the full-term human placenta by RT-PCR and quantitative microscopy. The mRNA sequence of FCGR2B expressed specifically in placental endothelial cells is that of transcript variant 2. FcgammaRIIb expression and synthesis occur throughout the placental vascular tree but do not extend into the umbilical cord. This study provides additional information on FcgammaRIIb expression in the human placenta.

Published
2007
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334. In situ immunolabeling allows for detailed localization of prostaglandin synthesizing enzymes within amnion epithelium.

Author

Ackerman WE 4th, Hughes LH, Robinson JM, and Kniss DA

Subjects
Animals, Cells, Cultured, Cryoultramicrotomy, Epithelium enzymology, Female, Humans, Amnion enzymology, Fluorescent Antibody Technique, Indirect, Prostaglandin-Endoperoxide Synthases analysis, Prostaglandins E biosynthesis
Abstract

Detailed information regarding the subcellular distribution of proteins within amnion epithelial cells is a goal of numerous placental biologists. In this report, we describe a versatile technique for in situ immunolabeling in amnion that is as technically permissible as traditional immunolabeling of cultured cells and, when coupled with confocal laser scanning microscopy, is similarly capable of providing detailed information regarding subcellular protein distribution. Using antibodies directed against sequential enzymes of the prostaglandin E biosynthesis cascade, we compared this novel method with immunofluorescent labeling using amnion cells in primary culture and cryosections of reflected fetal membrane rolls. By several criteria, we observed morphological variation between the cells cultured in vitro and the tissue specimens. Despite general consistencies in immunostaining patterns between the cryosectioned specimens and those labeled in situ, morphological preservation was superior using the latter technique. Relative to the cryosectioned specimens, in situ immunostaining was advantageous in that it permitted improved sampling efficiency, and allowed regional variations in labeling to be observed in a more global context within the tissue. Our results demonstrate that in situ immunolabeling provides a useful adjunct or alternative to immunolabeling using membrane roll preparations.

Published
2006
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335. Advanced techniques in placental biology -- workshop report.

Author

Nelson DM, Sadovsky Y, Robinson JM, Croy BA, Rice G, and Kniss DA

Subjects
Animals, Cryoultramicrotomy methods, Female, Fluorescent Antibody Technique, Gene Expression Regulation, Humans, Lymphocytes metabolism, Micromanipulation instrumentation, Uterus metabolism, MicroRNAs physiology, Microdissection methods, Micromanipulation methods, Microscopy, Immunoelectron methods, Placenta physiology, Protein Array Analysis methods
Abstract

Major advances in placental biology have been realized as new technologies have been developed and existing methods have been refined in many areas of biological research. Classical anatomy and whole-organ physiology tools once used to analyze placental structure and function have been supplanted by more sophisticated techniques adapted from molecular biology, proteomics, and computational biology and bioinformatics. In addition, significant refinements in morphological study of the placenta and its constituent cell types have improved our ability to assess form and function in highly integrated manner. To offer an overview of modern technologies used by investigators to study the placenta, this workshop: Advanced techniques in placental biology, assembled experts who discussed fundamental principles and real time examples of four separate methodologies. Y. Sadovsky presented the principles of microRNA function as an endogenous mechanism of gene regulation. J. Robinson demonstrated the utility of correlative microscopy in which light-level and transmission electron microscopy are combined to provide cellular and subcellular views of placental cells. A. Croy provided a lecture on the use of microdissection techniques which are invaluable for isolating very small subsets of cell types for molecular analysis. Finally, G. Rice presented an overview methods on profiling of complex protein mixtures within tissue and/or fluid samples that, when refined, will offer databases that will underpin a systems approach to modern trophoblast biology.

Published
2006
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336. Characterization of tumour-infiltrating lymphocytes and apoptosis in colitis-associated neoplasia: comparison with sporadic colorectal cancer.

Author

Michael-Robinson JM, Pandeya N, Walsh MD, Biemer-Huttmann AE, Eri RD, Buttenshaw RL, Lincoln D, Clouston AD, Jass JR, and Radford-Smith GL

Subjects
Aged, Apoptosis, CD2 Antigens immunology, CD8 Antigens immunology, Case-Control Studies, Colitis, Ulcerative complications, Colitis, Ulcerative pathology, Colorectal Neoplasms complications, Colorectal Neoplasms pathology, Epithelial Cells pathology, Female, Granzymes, Humans, Immunohistochemistry methods, Lymphocytes, Tumor-Infiltrating enzymology, Male, Microsatellite Repeats, Middle Aged, Neoplasm Staging, Prognosis, Serine Endopeptidases analysis, Colitis, Ulcerative immunology, Colorectal Neoplasms immunology, Lymphocytes, Tumor-Infiltrating immunology
Abstract

The development of colorectal cancer is a major complication for patients with chronic idiopathic colitis. Colitis-associated tumours tend to occur at a younger age and be more aggressive than sporadic colorectal cancers. While we have previously associated the presence of tumour-infiltrating lymphocytes (TILs) and increased apoptosis in sporadic colorectal cancer with high-level microsatellite instability and improved prognosis, little is known of the relationship between these variables in colitis-associated colorectal cancer. The aim of this study was to correlate TILs and tumour cell apoptosis in colitis-associated neoplasms stratified according to microsatellite instability. Twenty tumour and 11 dysplastic samples resected from 21 patients with long-standing colitis were analysed for microsatellite instability at 10 microsatellite markers. TIL distribution (CD3, CD8) and function (granzyme B) were quantified by immunohistochemistry. Neoplastic cell apoptosis was assessed using the M30 CytoDEATH antibody. These findings were compared with 40 microsatellite stable (MSS) sporadic colorectal cancers previously evaluated for TILs and neoplastic apoptosis. Low-level microsatellite instability was found in 1/20 colitis-associated tumours. All other colitis-associated lesions were designated MSS. CD3(+) and CD8(+) TIL counts were significantly higher in colitis-associated lesions compared with MSS sporadic colorectal cancer (p < 0.0001, p = 0.001 respectively). Despite their higher TIL density, colitis-associated tumours were more likely to present late (Dukes' stage C or D) (p = 0.02). Functionally, colitis-associated TILs demonstrated significantly less granzyme B expression compared to sporadic cancers (p = 0.002). The level of tumour cell apoptosis was similar between the two groups (sporadic, 1.53%; colitis cancers, 1.45%). In conclusion, MSS colitis-associated tumours have a higher prevalence of CD3(+)/CD8(+) TILs but no associated increase in tumour cell killing by apoptosis. Unlike cytotoxic T cells in sporadic colorectal cancer, TILs do not appear to enhance the prognosis of colitis-associated colorectal cancer. This may be related to an impairment of granzyme B expression within these lesions.

Published
2006
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337. Immunomodulation in type 1 diabetes by NBI-6024, an altered peptide ligand of the insulin B epitope.

Author

Alleva DG, Maki RA, Putnam AL, Robinson JM, Kipnes MS, Dandona P, Marks JB, Simmons DL, Greenbaum CJ, Jimenez RG, Conlon PJ, and Gottlieb PA

Subjects
Adolescent, Adult, Child, Female, Humans, Immunodominant Epitopes administration & dosage, Male, Th1 Cells immunology, Th2 Cells immunology, Cytokines metabolism, Diabetes Mellitus, Type 1 immunology, Immunologic Factors administration & dosage, Insulin administration & dosage, Interferon-gamma metabolism, Peptide Fragments administration & dosage
Abstract

NBI-6024 is an altered peptide ligand (APL) corresponding to the 9-23 amino acid region of the insulin B chain (B(9-23)), an epitope recognized by inflammatory interferon-gamma-producing T helper (Th)1 lymphocytes in type 1 diabetic patients. Immunomodulatory effects of NBI-6024 administration in recent-onset diabetic patients in a phase I clinical trial (NBI-6024-0003) were measured in peripheral blood mononuclear cells using the enzyme-linked immunosorbent spot assay. Analysis of the mean magnitude of cytokine responses to B(9-23) and NBI-6024 for each cohort showed significant increases in interleukin-5 responses (a Th2 regulatory phenotype) in cohorts that received APL relative to those receiving placebo. A responder analysis showed that Th1 responses to B(9-23) and NBI-6024 were observed almost exclusively in the placebo-treated diabetic population but not in nondiabetic control subjects and that APL administration (five biweekly subcutaneous injections) significantly and dose-dependently reduced the percentage of patients with these Th1 responses. The results of this phase I clinical study strongly suggest that NBI-6024 treatment shifted the Th1 pathogenic responses in recent-onset type 1 diabetic patients to a protective Th2 regulatory phenotype. The significance of these findings on the clinical outcome of disease is currently under investigation in a phase II multidose study.

Published
2006
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338. Thermodynamic model of quasiliquid formation on H2O ice: comparison with experiment.

Author

Henson BF, Voss LF, Wilson KR, and Robinson JM

Abstract

We have developed a new thermodynamic theory of the quasiliquid layer, which has been shown to be effective in modeling the phenomenon in a number of molecular systems. Here we extend our analysis to H(2)O ice, which has obvious implications for environmental and atmospheric chemistry. In the model, the liquid layer exists in contact with an ice defined as a two-dimensional lattice of sites. The system free energy is defined by the bulk free energies of ice I(h) and liquid water and is minimized in the grand canonical ensemble. An additional configurational entropy term arises from the occupation of the lattice sites. Furthermore, the theory predicts that the layer thickness as a function of temperature depends only on the liquid activity. Two additional models are derived, where slightly different approximations are used to define the free energy. With these two models, we illustrate the connection between the quasiliquid phenomenon and multilayer adsorption and the possibility of a two-dimensional phase transition connecting a dilute low coverage phase of adsorbed H(2)O and the quasiliquid phase. The model predictions are in agreement with a subset of the total suite of experimental measurements of the liquid thickness on H(2)O ice as a function of temperature. The theory indicates that the quasiliquid layer is actually equivalent to normal liquid water, and we discuss the impact of such an identification. In particular, observations of the liquid layer to temperatures as low as 200 K indicate the possibility that the quasiliquid is, in fact, an example of deeply supercooled normal water. Finally, we briefly discuss the obvious extension of the pure liquid theory to a thermodynamic theory of interfacial solutions on ice in the environment.

Published
2005
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339. Experimental isotherms of HCl on H2O ice under stratospheric conditions: connections between bulk and interfacial thermodynamics.

Author

Henson BF, Wilson KR, Robinson JM, Noble CA, Casson JL, and Worsnop DR

Abstract

The adsorption of HCl on the surface of H(2)O ice has been measured at temperatures and pressures relevant to the upper troposphere and lower stratosphere. The measured HCl surface coverage is found to be at least 100 times lower than currently assumed in models of chlorine catalyzed ozone destruction in cold regions of the upper atmosphere. Measurements were conducted in a closed system by simultaneous application of surface spectroscopy and gas phase mass spectrometry to fully characterize vapor/solid equilibrium. Surface adsorption is clearly distinguished from bulk liquid or solid phases. From 180 to 200 K, submonolayer adsorption of HCl is well described by a Bragg-Williams modified Langmuir model which includes the dissociation of HCl into H(+) and Cl(-) ions. Furthermore, adsorption is consistent with two distinct states on the ice substrate, one in which the ions only weakly adsorb on separate sites, and another where the ions adsorb as an H(+)-Cl(-) pair on a single site with adsorption energy comparable to the bulk trihydrate. The number of substrate H(2)O molecules per adsorption site is also consistent with the stoichiometry of bulk hydrates under these conditions. The ionic states exist in equilibrium, and the total adsorption energy is a function of the relative population of both states. These observations and model provide a quantitative connection between the thermodynamics of the bulk and interfacial phases of HCl/H(2)O, and represent a consistent physicochemical model of the equilibrium system.

Published
2004
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340. Dependence of quasiliquid thickness on the liquid activity: a bulk thermodynamic theory of the interface.

Author

Henson BF and Robinson JM

Abstract

Studies of the phenomenon of quasiliquid formation span systems as diverse as noble gases, complex organic molecules, and metals, and span triple point temperatures from 25 to 933 K. We show that when viewed as a single phenomenon essentially all published measurements of the quasiliquid layer thickness on solids below the melting point can be plotted as a function of the thermodynamic activity. Two classes of behavior are then observed: one for molecular systems and one for atomic systems. We derive a dependence on activity through a grand canonical lattice gas calculation. This is the only such unifying theory of this phenomenon.

Published
2004
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341. Correlative microscopy of ultrathin cryosections is a powerful tool for placental research.

Author

Takizawa T and Robinson JM

Subjects
Adult, Biomarkers analysis, Caveolin 1, Caveolins metabolism, Female, Humans, Microscopy, Immunoelectron methods, Placenta chemistry, Placenta metabolism, Pregnancy, Cryoelectron Microscopy methods, Microscopy, Fluorescence methods, Placenta ultrastructure
Abstract

In this report, we describe procedures for correlative fluorescence and electron microscopy in immunocytochemical studies on the human placenta. Ultrathin cryosections of placenta were used for detection of the distribution of antigens by immunofluorescence and subsequently by immunoelectron microscopy of the same ultrathin cryosection. This methodology has certain advantages over conventional immunohistochemistry and immunoelectron microscopy. The advantages are, most notably, that the same exact structures are examined by both imaging modalities. In addition, since the tissue is physically sectioned (50-100 nm thickness), greater resolution for fluorescence can be obtained in the z-dimension than can be obtained by optical sectioning in confocal microscopy. This last point is of particular importance for discriminating between structures closely stacked in the z-dimension. In this report, we have determined the distribution of caveolin-1 in ultrathin cryosections of terminal villi of the human term placenta. We demonstrate that the use of ultrathin cryosections is a powerful approach for immunofluorescence and correlative microscopy for the in situ localization of antigens.

Published
2003
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342. Patients with chronic critical limb ischaemia have reduced total antioxidant capacity and impaired nutritional status.

Author

Spark JI, Robinson JM, Gallavin L, Gough MJ, Homer-Vanniasinkam S, Kester RC, and Scott DJ

Subjects
Aged, Body Composition, Chronic Disease, Critical Illness, Female, Humans, Male, Middle Aged, Prospective Studies, Severity of Illness Index, Antioxidants analysis, Extremities blood supply, Ischemia blood, Ischemia complications, Nutrition Disorders blood, Nutrition Disorders complications, Peripheral Vascular Diseases blood, Peripheral Vascular Diseases complications
Abstract

Introduction: it has previously been demonstrated that total antioxidant capacity (TAC) can help predict which patients undergoing femoro-distal reconstruction are susceptible to postoperative infections., Aims: the aims of this study were to examine if TAC is influenced by the nutritional state of the patient and the degree of ischaemia., Patients and Methods: thirty patients with rest pain (21 men and 9 women), with a median age of 69 years and fifteen controls (9 men and 6 women), median age of 66 years, were studied. Nutritional status was assessed using serum albumin, body mass index (BMI), maximum voluntary contraction using a hand grip dynamometer and bioelectrical impedance to determine lean body mass. Blood was also taken for total antioxidant capacity (TAC)., Results: patients with chronic critical limb ischaemia (CCLI) had a lower TAC than controls (752 vs 1,130 micromol/l, p<0.05 Mann-Whitney U -test). There was no difference in serum albumin concentration between the CCLI group compared with controls (31 mmol/L vs 35 mmol/L, p>0.05 Mann-Whitney U-test). There was also no difference in BMI (23 vs 27, p>0.05 U-test) between the two groups. The other markers of nutrition including, maximum voluntary contractions (28.6 kg/m(2)vs 37.4 kg/m(2), p<0.05 M-W U-test), and lean body mass (3.0 vs 3.8 M-W U-test), showed a significant reduction in the vascular patients., Conclusion: TAC is significantly reduced in patients with CCLI and this may, in part, be explained by their impaired nutritional status.

Published
2002
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343. Large-angle electro-optic laser scanner on LiTaO(3) fabricated by in situ monitoring of ferroelectric-domain micropatterning.

Author

Scrymgeour DA, Barad Y, Gopalan V, Gahagan KT, Jia Q, Mitchell TE, and Robinson JM

Abstract

We report on a horn-shaped electro-optic scanner based on a ferroelectric LiTaO(3) wafer that is capable of scanning 632.8-nm light by an unprecedented 14.88 degrees angle for extraordinary polarized light and by 4.05 degrees for ordinary polarized light. The device concept is based on micropatterning ferroelectric domains in the shape of a series of optimized prisms whose refractive index is electric field tunable through the electro-optic effect. We demonstrate what we believe is a novel technique of using electro-optic imaging microscopy for in situ monitoring of the process of domain micropatterning during device fabrication, thus eliminating imperfect process control based on ex situ monitoring of transient currents.

Published
2001
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344. Ca(2+) induces an extended conformation of the inhibitory region of troponin I in cardiac muscle troponin.

Author

Dong WJ, Xing J, Robinson JM, and Cheung HC

Subjects
Actins antagonists & inhibitors, Amino Acid Sequence, Animals, Calcium metabolism, Energy Transfer, Fluorescence, Fluorescence Polarization, Mice, Models, Molecular, Molecular Sequence Data, Mutation genetics, Myosins antagonists & inhibitors, Protein Conformation drug effects, Rabbits, Rats, Troponin C genetics, Troponin C metabolism, Troponin I genetics, Troponin I metabolism, Troponin T genetics, Troponin T metabolism, Calcium pharmacology, Myocardium chemistry, Troponin I chemistry
Abstract

The inhibitory region of troponin I (TnI) plays a central regulatory role in the contraction and relaxation cycle of skeletal and cardiac muscle through its Ca(2+)-dependent interaction with actin. Detailed structural information on the interface between TnC and this region of TnI has been long in dispute. We have used fluorescence resonance energy transfer (FRET) to investigate the global conformation of the inhibitory region of a full-length TnI mutant from cardiac muscle (cTnI) in the unbound state and in reconstituted complexes with the other cardiac troponin subunits. The mutant contained a single tryptophan residue at the position 129 which was used as an energy transfer donor, and a single cysteine residue at the position 152 labeled with IAEDANS as energy acceptor. The sequence between Trp129 and Cys152 in cTnI brackets the inhibitory region (residues 130-149), and the distance between the two sites was found to be 19.4 A in free cTnI. This distance was insensitive to reconstitution of cTnI with cardiac troponin T (cTnT), cTnC, or cTnC and cTnT in the absence of bound regulatory Ca(2+) in cTnC. An increase of 9 A in the Trp129-Cys152 separation was observed upon saturation of the Ca(2+) regulatory site of cTnC in the complexes. This large increase suggests an extended conformation of the inhibitory region in the interface between cTnC and cTnI in holo cardiac troponin. This extended conformation is different from a recent model of the Ca(2+)-saturated skeletal TnI-TnC complex in which the inhibitory region is modeled as a beta-turn. The observed Ca(2+)-induced conformational change may be a switch mechanism by which movement of the regulatory region of cTnI to the exposed hydrophobic patch of the open regulatory N-domain of cTnC pulls the inhibitory region away from actin upon Ca(2+) activation in cardiac muscle., (Copyright 2001 Academic Press.)

Published
2001
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345. Integrated high-power electro-optic lens and large-angle deflector.

Author

Gahagan KT, Scrymgeour DA, Casson JL, Gopalan V, and Robinson JM

Abstract

We present a theoretical discussion and experimental demonstration of what to our knowledge is a novel integrated electro-optic lens and beam deflector fabricated in lithium tantalate. The cylindrical lens collimates Gaussian beams as small as 4 mum in diameter, whereas the independently controlled deflector is capable of scanning the collimated beam through an angular range of nearly 20 degrees .

Published
2001
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346. The VISA-A questionnaire: a valid and reliable index of the clinical severity of Achilles tendinopathy.

Author

Robinson JM, Cook JL, Purdam C, Visentini PJ, Ross J, Maffulli N, Taunton JE, and Khan KM

Subjects
Adult, Female, Humans, Male, Middle Aged, Pain Measurement instrumentation, Reproducibility of Results, Tendon Injuries classification, Achilles Tendon injuries, Surveys and Questionnaires, Tendon Injuries diagnosis, Trauma Severity Indices
Abstract

Background: There is no disease specific, reliable, and valid clinical measure of Achilles tendinopathy., Objective: To develop and test a questionnaire based instrument that would serve as an index of severity of Achilles tendinopathy., Methods: Item generation, item reduction, item scaling, and pretesting were used to develop a questionnaire to assess the severity of Achilles tendinopathy. The final version consisted of eight questions that measured the domains of pain, function in daily living, and sporting activity. Results range from 0 to 100, where 100 represents the perfect score. Its validity and reliability were then tested in a population of non-surgical patients with Achilles tendinopathy (n = 45), presurgical patients with Achilles tendinopathy (n = 14), and two normal control populations (total n = 87)., Results: The VISA-A questionnaire had good test-retest (r = 0.93), intrarater (three tests, r = 0.90), and interrater (r = 0.90) reliability as well as good stability when compared one week apart (r = 0.81). The mean (95% confidence interval) VISA-A score in the non-surgical patients was 64 (59-69), in presurgical patients 44 (28-60), and in control subjects it exceeded 96 (94-99). Thus the VISA-A score was higher in non-surgical than presurgical patients (p = 0.02) and higher in control subjects than in both patient populations (p<0.001)., Conclusions: The VISA-A questionnaire is reliable and displayed construct validity when means were compared in patients with a range of severity of Achilles tendinopathy and control subjects. The continuous numerical result of the VISA-A questionnaire has the potential to provide utility in both the clinical setting and research. The test is not designed to be diagnostic. Further studies are needed to determine whether the VISA-A score predicts prognosis.

Published
2001
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347. T1-T1 interactions occur in ER membranes while nascent Kv peptides are still attached to ribosomes.

Author

Lu J, Robinson JM, Edwards D, and Deutsch C

Subjects
Animals, Binding Sites, Dogs, Female, Kv1.3 Potassium Channel, Microsomes metabolism, Models, Molecular, Peptide Fragments biosynthesis, Potassium Channels chemistry, Protein Binding, Protein Conformation, Protein Folding, Protein Structure, Tertiary, Protein Transport, Xenopus laevis, Endoplasmic Reticulum metabolism, Potassium Channels metabolism, Potassium Channels, Voltage-Gated, Protein Biosynthesis, Ribosomes metabolism
Abstract

For voltage-gated K+ channels (Kv), it is not clear at which stage during biosynthesis in the endoplasmic reticulum (ER) oligomerization occurs, specifically whether it can begin while nascent peptide chains of individual subunits are still attached to ribosomes. Kv channels possess a T1-recognition domain in the NH2-terminus, which confers subfamily specificity for intersubunit assembly and forms a tetramer. Using pairs of cysteines engineered into the T1-T1 interface and cross-linking methods, we show that specific residues in the T1-T1 interface of different Kv1.3 subunits come into close proximity in the ER, both in microsomal membranes and in Xenopus oocytes. Furthermore, using translocation intermediates containing pairs of engineered cysteines in the T1 interface, we demonstrate that specific residues in the folded T1 domain interface can approach within 2 A of each other and form tetramers while the nascent Kv1.3 peptides are still attached to ribosomes and have translocated across the membrane. ER membranes are required for this interaction, and T1-T1 interactions occur inter-polysomally. Thus, folding of the T1 domain and intersubunit interaction may represent the first assembly event in channel formation.

Published
2001
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348. Proliferation, apoptosis, and survival in high-level microsatellite instability sporadic colorectal cancer.

Author

Michael-Robinson JM, Reid LE, Purdie DM, Biemer-Hüttmann AE, Walsh MD, Pandeya N, Simms LA, Young JP, Leggett BA, Jass JR, and Radford-Smith GL

Subjects
Aged, Colorectal Neoplasms genetics, Colorectal Neoplasms metabolism, Female, Follow-Up Studies, Humans, Immunohistochemistry, Ki-67 Antigen analysis, Male, Middle Aged, Mitotic Index, Survival Analysis, Apoptosis, Cell Division, Colorectal Neoplasms pathology, Microsatellite Repeats genetics
Abstract

Sporadic colorectal cancer (CRC) characterized by high-level DNA microsatellite instability (MSI-H) has a favorable prognosis. The reason for this MSI-H survival advantage is not known. The aim of this study was to correlate proliferation, apoptosis, and prognosis in CRC stratified by MSI status. The proliferative index (PI) was measured by immunohistochemical staining with the Ki-67 antibody in a selected series of 100 sporadic colorectal cancers classified according to the level of MSI as 31 MSI-H, 29 MSI-Low (MSI-L), and 40 microsatellite stable (MSS). The Ki-67 index was significantly higher in MSI-H cancers (P < 0.0001) in which the PI was 90.1 +/- 1.2% (mean +/- SE) compared with 69.5 +/- 3.1% and 69.5 +/- 2.3% in MSI-L and MSS subgroups, respectively. There was a positive linear correlation between the apoptotic index (AI) and PI (r = 0.51; P < 0.001), with MSI-H cancers demonstrating an increased AI:PI ratio indicative of a lower index of cell production. A high PI showed a trend toward predicting improved survival within MSI-H cancers (P = 0.09) but did not predict survival in MSI-L or MSS cancers. The AI was not associated with survival in any MSI subgroup. In conclusion, this is the first study to show that sporadic MSI-H cancers are characterized by a higher AI:PI ratio and increased proliferative activity compared with MSI-L and MSS cancers, and that an elevated PI may confer a survival advantage within the MSI-H subset.

Published
2001

349. Antigen retrieval in cells and tissues: enhancement with sodium dodecyl sulfate.

Author

Robinson JM and Vandré DD

Subjects
Caveolin 1, Caveolins analysis, Humans, Tubulin analysis, Antigens analysis, Immunohistochemistry methods, Sodium Dodecyl Sulfate, Surface-Active Agents
Abstract

Immunocytochemistry provides important information on the localization of antigens in cells and tissues. However, the procedures used to prepare cells and tissues for immunocytochemical labeling may have deleterious effects on the results achieved. That is, the antigen of interest may be difficult or impossible to detect following labeling. These sorts of observations have led to the concept of antigen masking in which the antigen (or specific epitope) is hidden from antibodies specific for that antigen (or epitope). Various procedures to circumvent this problem have been developed. These different procedures generally fit under the term "antigen retrieval" (or epitope retrieval). The practice of antigen retrieval is widely employed with paraffin-embedded material. Antigen retrieval is less often applied to cells and tissues that are not embedded in paraffin. However, in the latter preparations there are situations in which the observed immunolabeling achieved falls short of expectations. This poor level of immunolabeling may, in some situations, be improved upon with antigen retrieval procedures. In this review, we describe experimental situations in which immunolabeling fell short of expectations. We also describe a procedure that has been useful in enhancing immunolabeling efficiency in these cases. The major feature of this procedure is the incorporation of a permeabilization/denaturation step using sodium dodecyl sulfate. This postfixation and prelabeling step dramatically improves immunolabeling for a number of antigens in both cells and cryosections of tissue.

Published
2001
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350. Biological labeling and correlative microscopy.

Author

Robinson JM

Subjects
Animals, Cells, Cultured, Fluorescent Dyes metabolism, Green Fluorescent Proteins, Humans, Indicators and Reagents chemistry, Luminescent Proteins metabolism, Sodium Dodecyl Sulfate chemistry, Histocytological Preparation Techniques, Immunohistochemistry methods, Microscopy methods
Published
2001
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