Your search keyword '"Johnston GI"' showing total 39 results

1. THU0220 Seletalisib, a novel selective pi3kΔ inhibitor with therapeutic potential in inflammation and autoimmunity

Author

Payne, A, primary, Juarez, M, additional, Johnston, GI, additional, Helmer, E, additional, and Thomson, M, additional

Published

2017

2. Time Course Toxicogenomic Profiles in CD-1 Mice after Nontoxic and Nonlethal Hepatotoxic Paracetamol Administration

Author

Brain P, Dominic P. Williams, Provost Jp, Roddy Walsh, Hanton G, Garcia-Allan C, Smith Da, Johnston Gi, LeNet Jl, and B.K. Park

Subjects

Male, Time Factors, Down-Regulation, Gene Expression, Biology, Pharmacology, Toxicology, Mice, chemistry.chemical_compound, Animals, Statistical analysis, Gene, Heat-Shock Proteins, Acetaminophen, Gene Expression Profiling, Hepatotoxin, RNA, Dipeptides, General Medicine, Metabolism, Glutathione, Up-Regulation, Liver, chemistry, Time course, Gene chip analysis

Abstract

Adverse drug reactions are a major clinical problem. Drug-induced hepatotoxicity constitutes a large percentage of these reactions. A thorough understanding of the genetic events, specifically, the early "decision-making" processes underlying biological changes caused by drugs and metabolites, is required. To assist in the understanding of these events, we have employed the model hepatotoxin, paracetamol (APAP), and GeneChip technology to investigate global genetic events seen after nontoxic and toxic doses in the mouse. Mice were dosed [vehicle, nontoxic APAP (1 mmol/kg), and toxic APAP (3.5 mmol/kg)], and individual hepatic RNA samples were hybridized to separate chips to determine interanimal variation. Statistical analysis detected 175 CD-1 mouse genes that were significantly regulated (P4.1 x 10(-6)), and nonsignificant genes were discarded. For clarity, the significantly regulated genes were then binned into categories according to their major function-antioxidant, glutathione, metabolism, transcription, immune, and apoptosis. There was no hepatic stress observed after dosing 1 mmol/kg APAP, when measured by serum alanine aminotransferase levels. Hepatic toxicity was observed at both 4 and 24 h after a 3.5 mmol/kg dose of APAP. Time course expression profiles for selected genes have been created. These results demonstrate that most active gene expression occurs around 4 h after a toxic dose of APAP. Down-regulation of these genes is observed over 24 h, coinciding with the development of overt toxicity. These data provide a deeper understanding of the in vivo time course of physiological responses of the liver to chemical stress and provide a logical step forward for the investigation of new chemical entities demonstrated positive in chemically reactive metabolite screens. The complete data set can be viewed at http://www.ebi.ac.uk/arrayexpress/. The accession number is E-MEXP-82.

Published

2004

3. Proposed Information System For Management Of Electromedical Equipment

Author

Johnston Gi

Subjects

Equipment Safety, business.industry, Computer science, Hospital Bed Capacity, 300 to 499, Biomedical Engineering, Medicine (miscellaneous), Hospital Records, Investment (macroeconomics), Hospital records, Oregon, Engineering management, Health care, Safety Equipment, Information system, Maintenance and Engineering, Hospital, business, Information Systems

Abstract

The equipment investment in modern health care facilities warrants management attention to selection, maintenance, operation, and retirement requirements. An equipment information system is described that has been working for seven years, and a total system using modern hardware and data base technology is proposed to supplement the present system.

Published

1982

4. Cloning of glycoprotein IIIa cDNA from human erythroleukemia cells and localization of the gene to chromosome 17

Author

Rosa, JP, Bray, PF, Gayet, O, Johnston, GI, Cook, RG, Jackson, KW, Shuman, MA, and McEver, RP

Abstract

Platelet aggregation requires the binding of adhesive proteins such as fibrinogen to the heterodimer of membrane glycoproteins IIb (GPIIb) and IIIa (GPIIIa). Human erythroleukemia (HEL) cells synthesize both GPIIb and GPIIIa. Using poly(A+) RNA purified from HEL cells, we constructed a cDNA library in the lambda gt10 phage vector. This library was screened with a 38mer oligonucleotide derived from a platelet GPIIIa peptide, and three overlapping cDNAs were isolated. The three inserts encompassed 3.5 kilobases (kb), including the entire coding region of mature GPIIIa (2,286 basepairs, bp) and 1.3 kb of 3' untranslated sequence. All 222 residues determined directly from platelet GPIIIa tryptic peptides exactly matched the HEL cell-deduced amino acid sequence. The HEL cell sequence matched a previously reported endothelial cell cDNA sequence except for eight nucleotides. Five of these nucleotide differences were silent changes consistent with genetic polymorphisms. The other three differences resulted in changes in the deduced amino acid sequence of GPIIIa; reexamination of the endothelial cell cDNA sequence in these three areas revealed that it is actually identical to the HEL cell sequence. The virtual identity of the endothelial and HEL cell cDNA sequences provides direct evidence that GPIIIa is a subunit common to cell-adhesion receptors present in more than one cell type. We localized the gene for GPIIIa to chromosome 17, the same chromosome to which we had previously mapped the gene for GPIIb.

Published

1988

5. Platelet aggregation in whole blood from patients with Glanzmann's thrombasthenia

Author

Burgess-Wilson, ME, Cockbill, SR, Johnston, GI, and Heptinstall, S

Abstract

We examined platelet aggregation in platelet-rich plasma (PRP) and in whole blood from two patients with Glanzmann's thrombasthenia. In PRP, aggregation was measured by monitoring the changes in light absorbance that occurred in response to aggregating agents; to measure platelet aggregation in whole blood, we used a platelet counting technique. In PRP, the patients' platelets showed defective aggregation in response to ADP, adrenaline, arachidonic acid (AA), and collagen, but normal agglutination occurred in response to ristocetin. In whole blood, however, platelet aggregation in response to the aggregating agents appeared to be either very similar to that which occurred in blood from normal subjects or only slightly reduced. There was a reduced response to all concentrations of ADP and to low concentrations of collagen but a normal response to all concentrations of adrenaline, AA, and higher concentrations of collagen. Conversely, there seemed to be an increased agglutination response to ristocetin. The abnormality in our two patients with Glanzmann's thrombasthenia probably lies in the inability of their platelets to form large, macroscopic aggregates rather than in platelet aggregation per se.

Published

1987

6. Heterogeneity of platelet secretion in response to thrombin demonstrated by fluorescence flow cytometry

Author

Johnston, GI, primary, Pickett, EB, additional, McEver, RP, additional, and George, JN, additional

Published

1987

7. Target occupancy biomarker assay development using a conformation-selective antibody against small-molecule-bound TNF.

Author

Hickford ES, O'Connell J, Maloney A, Florian P, Johnston GI, Rospo CC, Herrmann M, Wright S, and Bourne T

Subjects

Enzyme-Linked Immunosorbent Assay, Antibodies

Abstract

Background: An antibody specific to small-molecule inhibitor-bound TNF has enabled the development of target occupancy biomarker assays to support the development of novel treatments for autoimmune disorders. Materials & methods: ELISAs were developed for inhibitor-bound and total TNF to determine the percentage of TNF occupancy in samples from stimulated blood. Inhibitor-saturated samples allowed measurement of total and inhibitor-bound TNF in a single electrochemiluminescence immunoassay. Results: TNF occupancy was proportional to inhibitor concentration in plasma samples. An electrochemiluminescence method for inhibitor-bound TNF was validated for use as a potential clinical occupancy biomarker assay. Conclusion: Development of these assays has allowed measurement of a target occupancy biomarker, which has supported progression of the first small-molecule inhibitors of TNF.

Published

2023

8. A phase 2 randomized, double-blind, placebo-controlled, proof-of-concept study of oral seletalisib in primary Sjögren's syndrome.

Author

Juarez M, Diaz N, Johnston GI, Nayar S, Payne A, Helmer E, Cain D, Williams P, Devauchelle-Pensec V, Fisher BA, Giacomelli R, Gottenberg JE, Guggino G, Kvarnström M, Mariette X, Ng WF, Rosas J, Sánchez Bursón J, Triolo G, Barone F, and Bowman SJ

Subjects

Administration, Oral, Antirheumatic Agents administration & dosage, Antirheumatic Agents adverse effects, Double-Blind Method, Female, Humans, Male, Middle Aged, Proof of Concept Study, Pyridines administration & dosage, Pyridines adverse effects, Quinolines administration & dosage, Quinolines adverse effects, Salivary Glands pathology, Sjogren's Syndrome pathology, Antirheumatic Agents therapeutic use, Pyridines therapeutic use, Quinolines therapeutic use, Sjogren's Syndrome drug therapy

Abstract

Objectives: This phase 2 proof-of-concept study (NCT02610543) assessed efficacy, safety and effects on salivary gland inflammation of seletalisib, a potent and selective PI3Kδ inhibitor, in patients with moderate-to-severe primary Sjögren's syndrome (PSS)., Methods: Adults with PSS were randomized 1:1 to seletalisib 45 mg/day or placebo, in addition to current PSS therapy. Primary end points were safety and tolerability and change from baseline in EULAR Sjögren's Syndrome Disease Activity Index (ESSDAI) score at week 12. Secondary end points included change from baseline at week 12 in EULAR Sjögren's Syndrome Patient Reported Index (ESSPRI) score and histological features in salivary gland biopsies., Results: Twenty-seven patients were randomized (seletalisib n = 13, placebo n = 14); 20 completed the study. Enrolment challenges led to early study termination with loss of statistical power (36% vs 80% planned). Nonetheless, a trend for improvement in ESSDAI and ESSPRI [difference vs placebo: -2.59 (95% CI: -7.30, 2.11; P=0.266) and -1.55 (95% CI: -3.39, 0.28), respectively] was observed at week 12. No significant changes were seen in saliva and tear flow. Serious adverse events (AEs) were reported in 3/13 of patients receiving seletalisib vs 1/14 for placebo and 5/13 vs 1/14 discontinued due to AEs, respectively. Serum IgM and IgG concentrations decreased in the seletalisib group vs placebo. Seletalisib demonstrated efficacy in reducing size and organisation of salivary gland inflammatory foci and in target engagement, thus reducing PI3K-mTOR signalling compared with placebo., Conclusion: Despite enrolment challenges, seletalisib demonstrated a trend towards clinical improvement in patients with PSS. Histological analyses demonstrated encouraging effects of seletalisib on salivary gland inflammation and organisation., Trial Registration: https://clinicaltrials.gov, NCT02610543., (© The Author(s) 2020. Published by Oxford University Press on behalf of the British Society for Rheumatology. All rights reserved. For permissions, please email: journals.permissions@oup.com.)

Published

2021

9. Seletalisib for Activated PI3Kδ Syndromes: Open-Label Phase 1b and Extension Studies.

Author

Diaz N, Juarez M, Cancrini C, Heeg M, Soler-Palacín P, Payne A, Johnston GI, Helmer E, Cain D, Mann J, Yuill D, Conti F, Di Cesare S, Ehl S, Garcia-Prat M, Maccari ME, Martín-Nalda A, Martínez-Gallo M, Moshous D, Santilli V, Semeraro M, Simonetti A, Suarez F, Cavazzana M, and Kracker S

Subjects

Adolescent, Adult, CD8-Positive T-Lymphocytes drug effects, CD8-Positive T-Lymphocytes metabolism, Child, Female, Humans, Immunologic Deficiency Syndromes metabolism, Male, Mutation drug effects, Precursor Cells, B-Lymphoid immunology, Precursor Cells, B-Lymphoid metabolism, Young Adult, Class I Phosphatidylinositol 3-Kinases antagonists & inhibitors, Immunologic Deficiency Syndromes drug therapy, Pyridines therapeutic use, Quinolines therapeutic use

Abstract

Mutations in two genes can result in activated PI3Kδ syndrome (APDS), a rare immunodeficiency disease with limited therapeutic options. Seletalisib, a potent, selective PI3Kδ inhibitor, was evaluated in patients with APDS1 and APDS2. In the phase 1b study (European Clinical Trials Database 2015-002900-10) patients with genetic and clinical confirmation of APDS1 or APDS2 received 15-25 mg/d seletalisib for 12 wk. Patients could enter an extension study (European Clinical Trials Database 2015-005541). Primary endpoints were safety and tolerability, with exploratory efficacy and immunology endpoints. Seven patients (median age 15 years; APDS1 n = 3; APDS2 n = 4) received seletalisib; five completed the phase 1b study. For the extension study, four patients entered, one withdrew consent (week 24), three completed ≥84 wk of treatment. In the phase 1b study, patients had improved peripheral lymphadenopathy ( n = 2), lung function ( n = 1), thrombocyte counts ( n = 1), and chronic enteropathy ( n = 1). Overall, effects were maintained in the extension. In the phase 1b study, percentages of transitional B cells decreased, naive B cells increased, and senescent CD8 T cells decreased (human cells); effects were generally maintained in the extension. Seletalisib-related adverse events occurred in four of seven patients (phase 1b study: hepatic enzyme increased, dizziness, aphthous ulcer, arthralgia, arthritis, increased appetite, increased weight, restlessness, tendon disorder, and potential drug-induced liver injury) and one of four patients had adverse events in the extension (aphthous ulcer). Serious adverse events occurred in three of seven patients (phase 1b study: hospitalization, colitis, and potential drug-induced liver injury) and one of four patients had adverse events in the extension (stomatitis). Patients with APDS receiving seletalisib had improvements in variable clinical and immunological features, and a favorable risk-benefit profile was maintained for ≤96 wk., (Copyright © 2020 by The American Association of Immunologists, Inc.)

Published

2020

10. Mitochondrial dysfunction and increased glycolysis in prodromal and early Parkinson's blood cells.

Author

Smith AM, Depp C, Ryan BJ, Johnston GI, Alegre-Abarrategui J, Evetts S, Rolinski M, Baig F, Ruffmann C, Simon AK, Hu MTM, and Wade-Martins R

Subjects

Case-Control Studies, Cytokines metabolism, Electron Transport Complex IV metabolism, Enzyme Inhibitors pharmacology, Female, Flow Cytometry, Gene Expression Regulation drug effects, Gene Expression Regulation genetics, Glucose metabolism, Glucose Transporter Type 1 metabolism, Humans, Male, Mitochondria metabolism, Mitochondria pathology, Oxygen Consumption physiology, Parkinson Disease pathology, Prodromal Symptoms, REM Sleep Behavior Disorder blood, REM Sleep Behavior Disorder complications, REM Sleep Behavior Disorder pathology, RNA, Messenger metabolism, Reactive Oxygen Species metabolism, Receptors, CCR2 metabolism, Superoxide Dismutase genetics, Superoxide Dismutase metabolism, Glycolysis physiology, Leukocytes, Mononuclear ultrastructure, Mitochondrial Diseases etiology, Parkinson Disease blood, Parkinson Disease complications

Abstract

Background: Although primarily a neurodegenerative process, there is increasing awareness of peripheral disease mechanisms in Parkinson's disease. To investigate disease processes in accessible patient cells, we studied peripheral blood mononuclear cells in recently diagnosed PD patients and rapid eye movement-sleep behavior disorder patients who have a greatly increased risk of developing PD. We hypothesized that peripheral blood mononuclear cells may recapitulate cellular pathology found in the PD brain and investigated these cells for mitochondrial dysfunction and oxidative stress., Methods: Peripheral blood mononuclear cells were isolated and studied from PD patients, rapid eye movement-sleep behavior disorder patients and age- and sex-matched control individuals from the well-characterized Oxford Discovery cohort. All participants underwent thorough clinical assessment., Results: Initial characterization showed that PD patients had elevated levels of CD14 + monocytes and monocytes expressing C-C motif chemokine receptor 2. Mitochondrial dysfunction and oxidative stress were increased in PD patient peripheral blood mononuclear cells, with elevated levels of mitochondrial reactive oxygen species specifically in patient monocytes. This was combined with reduced levels of the antioxidant superoxide dismutase in blood cells from PD patients and, importantly, also in rapid eye movement-sleep behavior disorder patients. This mitochondrial dysfunction was associated with a concomitant increase in glycolysis in both PD and rapid eye movement-sleep behavior disorder patient blood cells independent of glucose uptake or monocyte activation., Conclusions: This work demonstrates functional bioenergetic deficits in PD and rapid eye movement-sleep behavior disorder patient blood cells during the early stages of human disease. © 2018 The Authors. Movement Disorders published by Wiley Periodicals, Inc. on behalf of International Parkinson and Movement Disorder Society., (© 2018 The Authors. Movement Disorders published by Wiley Periodicals, Inc. on behalf of International Parkinson and Movement Disorder Society.)

Published

2018

11. Repeated administration of dapirolizumab pegol in a randomised phase I study is well tolerated and accompanied by improvements in several composite measures of systemic lupus erythematosus disease activity and changes in whole blood transcriptomic profiles.

Author

Chamberlain C, Colman PJ, Ranger AM, Burkly LC, Johnston GI, Otoul C, Stach C, Zamacona M, Dörner T, Urowitz M, and Hiepe F

Subjects

Administration, Intravenous, Adolescent, Adult, Aged, CD40 Ligand drug effects, Dose-Response Relationship, Drug, Double-Blind Method, Drug Administration Schedule, Female, Humans, Lupus Erythematosus, Systemic blood, Male, Middle Aged, RNA blood, Severity of Illness Index, Treatment Outcome, Young Adult, Immunoglobulin Fab Fragments administration & dosage, Immunologic Factors administration & dosage, Lupus Erythematosus, Systemic drug therapy, Polyethylene Glycols administration & dosage, Transcriptome drug effects

Abstract

Objectives: Systemic lupus erythematosus (SLE) is a heterogeneous autoimmune disease associated with diffuse immune cell dysfunction. CD40-CD40 ligand (CD40L) interaction activates B cells, antigen-presenting cells and platelets. CD40L blockade might provide an innovative treatment for systemic autoimmune disorders. We investigated the safety and clinical activity of dapirolizumab pegol, a polyethylene glycol conjugated anti-CD40L Fab' fragment, in patients with SLE., Methods: This 32-week randomised, double-blind, multicentre study (NCT01764594) evaluated repeated intravenous administration of dapirolizumab pegol in patients with SLE who were positive for/had history of antidouble stranded DNA/antinuclear antibodies and were on stable doses of immunomodulatory therapies (if applicable). Sixteen patients were randomised to 30 mg/kg dapirolizumab pegol followed by 15 mg/kg every 2 weeks for 10 weeks; eight patients received a matched placebo regimen. Randomisation was stratified by evidence of antiphospholipid antibodies. Patients were followed for 18 weeks after the final dose., Results: No serious treatment-emergent adverse events, thromboembolic events or deaths occurred. Adverse events were mild or moderate, transient and resolved without intervention. One patient withdrew due to infection.Efficacy assessments were conducted only in patients with high disease activity at baseline. Five of 11 (46%) dapirolizumab pegol-treated patients achieved British Isles Lupus Assessment Group-based Composite Lupus Assessment response (vs 1/7; 14% placebo) and 5/12 (42%) evaluable for SLE Responder Index-4 responded by week 12 (vs 1/7; 14% placebo). Mechanism-related gene expression changes were observed in blood RNA samples., Conclusions: Dapirolizumab pegol could be an effective biological treatment for SLE. Further studies are required to address efficacy and safety., Trial Registration Number: NCT01764594., Competing Interests: Competing interests: CC, PJC, GIJ, CO and MZ are full-time employees of UCB Pharma and hold stock awards and/or options. CS is a full-time employee of UCB Biosciences GmbH and holds stock awards and/or options. AMR was a full-time employee and stock holder of Biogen at the time the study was conducted. LCB is a full time employee and stockholder of Biogen. FH has received consultancy fees from UCB, Sanofi, Eli Lilly, Baxter, BMS and research grants from Deutsche Forschungsgemeinschaft, IMI (PRECISESADS) and attended speakers’ bureau for GSK, Roche Pharma and Pfizer. TD has received consultancy fees and research grants from UCB, Biogen, Roche, Sanofi, Eli Lilly, Jansen and research grants from Deutsche Forschungsgemeinschaft and EU Horizon 2020 (Harmonics). MU has served as Chair of the Data and Safety Monitoring Committee for the study., (© Article author(s) (or their employer(s) unless otherwise stated in the text of the article) 2017. All rights reserved. No commercial use is permitted unless otherwise expressly granted.)

Published

2017

12. Prevalence and markers of advanced liver disease in type 2 diabetes.

Author

Williamson RM, Price JF, Hayes PC, Glancy S, Frier BM, Johnston GI, Reynolds RM, and Strachan MW

Subjects

Aged, Alanine Transaminase blood, Biomarkers analysis, Female, Humans, Hyaluronic Acid analysis, Liver Diseases etiology, Male, Middle Aged, Platelet Count, Predictive Value of Tests, Prevalence, Radiography, Spleen diagnostic imaging, gamma-Glutamyltransferase blood, Diabetes Mellitus, Type 2 complications, Liver Diseases diagnosis

Abstract

Background: Type 2 diabetes is a risk factor for progression of non-alcoholic fatty liver disease (NAFLD) to fibrosis and cirrhosis. We examined the prevalence of advanced liver disease in people with type 2 diabetes and analysed the effectiveness of liver function tests (LFTs) as a screening tool., Methods: Participants (n = 939, aged 61-76 years) from the Edinburgh Type 2 Diabetes Study, a randomly selected population of people with type 2 diabetes, underwent abdominal ultrasonography. Hyaluronic acid (HA) and platelet count/spleen diameter ratio (PSR) were used as non-invasive markers of hepatic fibrosis and portal hypertension. Subjects were screened for secondary causes of liver disease that excluded them from a diagnosis of NAFLD. The efficacy of LFTs [alanine aminotransferase (ALT) and gamma-glutamyltransferase (GGT)] in screening for liver disease was determined., Results: Cirrhosis was identified by ultrasound in four participants (0.4%). Ten (1.1%) had evidence of portal hypertension (PSR < 909), and two (0.2%) had hepatocellular carcinoma. Fifty-three participants (5.7%) had evidence of hepatic fibrosis (HA > 100 ng/ml in the absence of joint disease); a further 169 had HA > 50 ng/ml. In participants with NAFLD-related fibrosis (HA > 100 ng/ml), 12.5% had an elevated ALT level and 17.5% had an elevated GGT level., Conclusion: The prevalence of hepatic fibrosis and cirrhosis were lower than expected. The use of LFTs to screen for liver disease missed most cases of fibrosis predicted by raised HA levels.

Published

2012

13. Sequence analysis of the IL28A/IL28B inverted gene duplication that contains polymorphisms associated with treatment response in hepatitis C patients.

Author

Reynolds JM, Paciga SA, Sanders FA, Hyde CL, Loomis AK, and Johnston GI

Subjects

Alleles, Base Sequence, Computational Biology, Databases, Genetic, Gene Frequency genetics, Genetic Predisposition to Disease, Genotyping Techniques, Humans, Interferons, Molecular Sequence Data, Polymerase Chain Reaction, Sequence Alignment, Sequence Homology, Nucleic Acid, Treatment Outcome, Gene Duplication genetics, Hepatitis C drug therapy, Hepatitis C genetics, Interleukins genetics, Polymorphism, Single Nucleotide genetics, Sequence Analysis, DNA

Abstract

Several SNPs located in or around the IL28B gene are associated with response of patients infected with Hepatitis C virus to treatment with pegylated interferon-α ⁺/⁻ ribavirin or with spontaneous clearance of the virus. The results of such studies are so compelling that future treatment approaches are likely to involve clinical decisions being made on the basis of a patient's genotype. Since IL28B is a paralogue of IL28A with greater than 95% sequence identity, it is possible that without genotyping assay specificity, sequences in IL28A may contribute to genotype identification, and potentially confound treatment decisions. This study aimed to 1) examine DNA sequences in IL28B surrounding each of the reported associated SNPs and the corresponding regions in IL28A; and 2) develop a robust assay for rs12979860, the most 'cosmopolitan' SNP most strongly associated with treatment response across all global populations studied to date. Bioinformatic analysis of genomic regions surrounding IL28A and IL28B demonstrated that 3 SNPs were unique to IL28B, whereas the remaining 6 SNP regions shared >93% identity between IL28A and IL28B. Using a panel of DNA samples, PCR amplification followed by Sanger sequencing was used to examine IL28B SNPs and the corresponding regions in IL28A. For the overlapping SNPs, all 6 in IL28B were confirmed to be polymorphic whereas the corresponding positions in IL28A were monomorphic. Based upon IL28A and IL28B sequence data, a specific TaqMan® assay was developed for SNP rs12979860 that was 100% concordant to the sequence-derived genotypes. Analysis using a commercial assay identified one discordant result which led to a change in their genotype-calling algorithm. Where future treatment decisions are made upon the results of genotyping assays, it is very important that results are concordant with data from a sequence-based format. This is especially so in situations where designing specific PCR primers is a challenge.

Published

2012

14. Prevalence of and risk factors for hepatic steatosis and nonalcoholic Fatty liver disease in people with type 2 diabetes: the Edinburgh Type 2 Diabetes Study.

Author

Williamson RM, Price JF, Glancy S, Perry E, Nee LD, Hayes PC, Frier BM, Van Look LA, Johnston GI, Reynolds RM, and Strachan MW

Subjects

Aged, Fatty Liver diagnosis, Female, Humans, Male, Middle Aged, Non-alcoholic Fatty Liver Disease, Risk Factors, Diabetes Mellitus, Type 2 epidemiology, Diabetes Mellitus, Type 2 physiopathology, Fatty Liver epidemiology

Abstract

Objective: Type 2 diabetes is an established risk factor for development of hepatic steatosis and nonalcoholic fatty liver disease (NAFLD). We aimed to determine the prevalence and clinical correlates of these conditions in a large cohort of people with type 2 diabetes., Research Design and Methods: A total of 939 participants, aged 61-76 years, from the Edinburgh Type 2 Diabetes Study (ET2DS)-a large, randomly selected population of people with type 2 diabetes-underwent liver ultrasonography. Ultrasound gradings of steatosis were compared with magnetic resonance spectroscopy in a subgroup. NAFLD was defined as hepatic steatosis in the absence of a secondary cause (screened by questionnaire assessing alcohol and hepatotoxic medication use, plasma hepatitis serology, autoantibodies and ferritin, and record linkage to determine prior diagnoses of liver disease). Binary logistic regression was used to analyze independent associations of characteristics with NAFLD., Results: Hepatic steatosis was present in 56.9% of participants. After excluding those with a secondary cause for steatosis, the prevalence of NAFLD in the study population was 42.6%. Independent predictors of NAFLD were BMI, lesser duration of diabetes, HbA(1c), triglycerides, and metformin use. These remained unchanged after exclusion of participants with evidence of hepatic fibrosis from the group with no hepatic steatosis., Conclusions: Prevalences of hepatic steatosis and NAFLD were high in this unselected population of older people with type 2 diabetes, but lower than in studies in which ultrasound gradings were not compared with a gold standard. Associations with features of the metabolic syndrome could be used to target screening for this condition.

Published

2011

15. The use of ultrasound to diagnose hepatic steatosis in type 2 diabetes: intra- and interobserver variability and comparison with magnetic resonance spectroscopy.

Author

Williamson RM, Perry E, Glancy S, Marshall I, Gray C, Nee LD, Hayes PC, Forbes S, Frier BM, Johnston GI, Lee AJ, Reynolds RM, Price JF, and Strachan MW

Subjects

Aged, Diabetes Mellitus, Type 2 diagnostic imaging, Disease Progression, Fatty Liver diagnostic imaging, Fatty Liver pathology, Female, Humans, Male, Middle Aged, Observer Variation, Sensitivity and Specificity, Ultrasonography, United Kingdom, Diabetes Mellitus, Type 2 diagnosis, Fatty Liver diagnosis, Magnetic Resonance Spectroscopy methods

Abstract

Aim: To compare ultrasound gradings of steatosis with fat fraction (FF) on magnetic resonance spectroscopy (MRS; the non-invasive reference standard for quantification of hepatic steatosis), and evaluate inter- and intraobserver variability in the ultrasound gradings., Materials and Methods: Triple grading of hepatic ultrasound examination was performed by three independent graders on 131 people with type 2 diabetes. The stored images of 60 of these individuals were assessed twice by each grader on separate occasions. Fifty-eight patients were pre-selected on the basis of ultrasound grading (normal, indeterminate/mild steatosis, or severe steatosis) to undergo (1)H-MRS. The sensitivity and specificity of the ultrasound gradings were determined with reference to MRS data, using two cut-offs of FF to define steatosis, ≥9% and ≥6.1%., Results: Median (intraquartile range) MRS FF (%) in the participants graded on ultrasound as normal, indeterminate/mild steatosis, and severe steatosis were 4.2 (1.2-5.7), 4.1 (3.1-8.5) and 19.4 (12.9-27.5), respectively. Using a liver FF of ≥6.1% on MRS to denote hepatic steatosis, the unadjusted sensitivity and specificity of ultrasound gradings (severe versus other grades of steatosis) were 71 and 100%, respectively. Interobserver agreement within one grade was observed in 79% of cases. Exact intraobserver agreement ranged from 62 to 87%., Conclusion: Hepatic ultrasound provided a good measure of the presence of significant hepatic steatosis with good intra- and interobserver agreement. The grading of a mildly steatotic liver was less secure and, in particular, there was considerable overlap in hepatic FF with those who had a normal liver on ultrasound., (Copyright © 2011 The Royal College of Radiologists. Published by Elsevier Ltd. All rights reserved.)

Published

2011

16. Toward a dynamic model of deposition and utilization of yolk steroids.

Author

Moore MC and Johnston GI

Abstract

The discovery by Schwabl that maternal steroid hormones are transferred to the egg yolk and have effects on the phenotype of offspring revealed a new pathway for non-genetic maternal effects. The initial model relied on passive transfer. The thinking was that steroids passively entered the lipophillic yolk during yolk deposition and then were deposited in the yolk until they were passively delivered to the embryo as the yolk was used. Subsequent studies revealed that the system is much more dynamic than that. Here, we explore questions about how dynamic the system really is and look at questions like: Is transfer of maternal steroids to the yolk passive or is it actively regulated? At what stages of the maternal reproductive cycle are steroids transferred? During reproduction, how dynamic are the levels of yolk steroids? Especially in the case of potentially deleterious steroids (e.g., androgens in female offspring; glucocorticoids), once deposited can they come out of the yolk over time? Can they be metabolized by the yolk or by the embryo? During incubation, how much do steroid levels in the yolk change? Can steroids diffuse from the yolk to the embryo prior to yolk utilization? Does the embryo contribute to yolk steroid levels as it develops? We believe that comprehensive answers to questions like these will eventually allow us to generate a much more accurate and complete model of the transfer and utilization of yolk steroids and that this model will be much more dynamic and active than the one initially proposed.

Published

2008

17. Corticosterone modulation of reproductive and immune systems trade-offs in female tree lizards: long-term corticosterone manipulations via injectable gelling material.

Author

French SS, McLemore R, Vernon B, Johnston GI, and Moore MC

Subjects

Animals, Drug Implants, Female, Gels, Reproduction drug effects, Time Factors, Wound Healing drug effects, Corticosterone administration & dosage, Corticosterone pharmacology, Lizards physiology

Abstract

Physiological trade-offs arise because multiple processes compete for the same limiting resources. While competition for resources has been demonstrated between reproduction and immune function, the regulation of this competition remains unclear. Corticosterone (CORT) is a likely mediator due to its dual role in mobilizing energy stores throughout the body and regulating physiological responses to stressors. We manipulated CORT concentrations and resources in pre-reproductive and reproductive female tree lizards (Urosaurus ornatus) to test the hypothesis that CORT regulates the distribution of limiting resources between the reproductive and immune systems. To manipulate circulating concentrations of CORT we utilized a novel method of hormone implantation, in which a polymeric compound is mixed with hormone and injected in liquid form into the animal. After injection, the liquid quickly gels in situ forming a slow release hormone implant. This method of hormone delivery eliminated the need for substantial wounds to the animal or repeated handling required by other methods. In this study, the hormone-treated animals had plasma CORT concentrations comparable to high physiological concentrations. We found that CORT treatment suppressed immune function, but only when animals were energetically compromised. We assessed immune function by measuring the healing rate of a cutaneous biopsy. Healing was suppressed in all CORT-treated reproductive animals and in all CORT-treated animals (pre-reproductive and reproductive) undergoing food restriction, but CORT had no effect in ad libitum non-reproductive females. The context-dependent action of CORT renders its response adjustable to changing environmental conditions and may allow for the suppression of specific functions depending on resource availability.

Published

2007

18. Hex acts with beta-catenin to regulate anteroposterior patterning via a Groucho-related co-repressor and Nodal.

Author

Zamparini AL, Watts T, Gardner CE, Tomlinson SR, Johnston GI, and Brickman JM

Subjects

Animals, Body Patterning genetics, Body Patterning physiology, Cell Line, Cells, Cultured, Embryonic Stem Cells cytology, Embryonic Stem Cells metabolism, Endoderm cytology, Endoderm metabolism, Gene Expression Regulation, Developmental, Homeodomain Proteins genetics, Homeodomain Proteins metabolism, Humans, In Situ Hybridization, Mesoderm cytology, Mesoderm metabolism, Models, Genetic, Nodal Protein, Oligonucleotide Array Sequence Analysis methods, Protein Binding, Repressor Proteins metabolism, Reverse Transcriptase Polymerase Chain Reaction, Signal Transduction genetics, Signal Transduction physiology, Transcription Factors genetics, Transcription Factors metabolism, Transforming Growth Factor beta metabolism, Wnt Proteins genetics, Wnt Proteins metabolism, Xenopus Proteins metabolism, Xenopus laevis embryology, Xenopus laevis metabolism, beta Catenin metabolism, Repressor Proteins genetics, Transforming Growth Factor beta genetics, Xenopus Proteins genetics, Xenopus laevis genetics, beta Catenin genetics

Abstract

In Xenopus, the establishment of the anteroposterior axis involves two key signalling pathways, canonical Wnt and Nodal-related TGFbeta. There are also a number of transcription factors that feedback upon these pathways. The homeodomain protein Hex, an early marker of anterior positional information, acts as a transcriptional repressor, suppressing induction and propagation of the Spemman organiser while specifying anterior identity. We show that Hex promotes anterior identity by amplifying the activity of canonical Wnt signalling. Hex exerts this activity by inhibiting the expression of Tle4, a member of the Groucho family of transcriptional co-repressors that we identified as a Hex target in embryonic stem (ES) cells and Xenopus embryos. This Hex-mediated enhancement of Wnt signalling results in the upregulation of the Nieuwkoop centre genes Siamois and Xnr3, and the subsequent increased expression of the anterior endodermal marker Cerberus and other mesendodermal genes downstream of Wnt signalling. We also identified Nodal as a Hex target in ES cells. We demonstrate that in Xenopus, the Nodal-related genes Xnr1 and Xnr2, but not Xnr5 and Xnr6, are regulated directly by Hex. The identification of Nodal-related genes as Hex targets explains the ability of Hex to suppress induction and propagation of the organiser. Together, these results support a model in which Hex acts early in development to reinforce a Wnt-mediated, Nieuwkoop-like signal to induce anterior endoderm, and later in this tissue to block further propagation of Nodal-related signals. The ability of Hex to regulate the same targets in both Xenopus and mouse implies this model is conserved.

Published

2006

19. Time course toxicogenomic profiles in CD-1 mice after nontoxic and nonlethal hepatotoxic paracetamol administration.

Author

Williams DP, Garcia-Allan C, Hanton G, LeNet JL, Provost JP, Brain P, Walsh R, Johnston GI, Smith DA, and Park BK

Subjects

Acetaminophen pharmacology, Animals, Dipeptides genetics, Down-Regulation, Gene Expression Profiling, Heat-Shock Proteins genetics, Liver enzymology, Male, Mice, Time Factors, Up-Regulation, Acetaminophen toxicity, Gene Expression drug effects, Liver drug effects

Abstract

Adverse drug reactions are a major clinical problem. Drug-induced hepatotoxicity constitutes a large percentage of these reactions. A thorough understanding of the genetic events, specifically, the early "decision-making" processes underlying biological changes caused by drugs and metabolites, is required. To assist in the understanding of these events, we have employed the model hepatotoxin, paracetamol (APAP), and GeneChip technology to investigate global genetic events seen after nontoxic and toxic doses in the mouse. Mice were dosed [vehicle, nontoxic APAP (1 mmol/kg), and toxic APAP (3.5 mmol/kg)], and individual hepatic RNA samples were hybridized to separate chips to determine interanimal variation. Statistical analysis detected 175 CD-1 mouse genes that were significantly regulated (P < 4.1 x 10(-6)), and nonsignificant genes were discarded. For clarity, the significantly regulated genes were then binned into categories according to their major function-antioxidant, glutathione, metabolism, transcription, immune, and apoptosis. There was no hepatic stress observed after dosing 1 mmol/kg APAP, when measured by serum alanine aminotransferase levels. Hepatic toxicity was observed at both 4 and 24 h after a 3.5 mmol/kg dose of APAP. Time course expression profiles for selected genes have been created. These results demonstrate that most active gene expression occurs around 4 h after a toxic dose of APAP. Down-regulation of these genes is observed over 24 h, coinciding with the development of overt toxicity. These data provide a deeper understanding of the in vivo time course of physiological responses of the liver to chemical stress and provide a logical step forward for the investigation of new chemical entities demonstrated positive in chemically reactive metabolite screens. The complete data set can be viewed at http://www.ebi.ac.uk/arrayexpress/. The accession number is E-MEXP-82.

Published

2004

20. Problems, perils, precautions and rewards in overseas clinical engineering training.

Author

Johnston GI

Subjects

Attitude of Health Personnel, Biomedical Engineering organization & administration, China, Cultural Characteristics, Egypt, Guyana, Humans, Interprofessional Relations, Jamaica, Saudi Arabia, Workforce, Biomedical Engineering education, Developing Countries, Maintenance and Engineering, Hospital

Published

1996

21. Cloning and pharmacological characterization of human alpha-1 adrenergic receptors: sequence corrections and direct comparison with other species homologues.

Author

Schwinn DA, Johnston GI, Page SO, Mosley MJ, Wilson KH, Worman NP, Campbell S, Fidock MD, Furness LM, and Parry-Smith DJ

Subjects

Amino Acid Sequence, Animals, Cattle, Cloning, Molecular, Cricetinae, Genes, Humans, Molecular Sequence Data, Phosphatidylinositols metabolism, Rats, Receptors, Adrenergic, alpha drug effects, Second Messenger Systems, Sequence Alignment, Sequence Homology, Amino Acid, Signal Transduction, Structure-Activity Relationship, Receptors, Adrenergic, alpha genetics

Abstract

We have cloned cDNAs encoding three human alpha-1 adrenergic receptor (AR) subtypes and characterized pharmacological properties of the expressed receptor protein. A number of significant sequence corrections have been identified and compared with previously published data, at both nucleotide and amino acid levels; the most major differences occur for the human alpha-1a/dAR. Pharmacological characterization was performed simultaneously using six cloned alpha-1AR subtypes (human and rat alpha-1a/d, human and hamster alpha-1b, human and bovine alpha-1c) stably expressed in rat-1 fibroblasts at approximately equal receptor concentrations (1-2 pmol/mg of total protein). In general, human alpha-1AR subtypes have similar pharmacology compared to their rat, hamster and bovine homologs, although a few minor species differences important for alpha-1AR classification are noted. In addition, much lower inactivation (approximately 20%) by the alkylating agent chloroethylclonidine is noted in this study compared to previous reports for both human and bovine alpha-1cAR membrane preparations. All six alpha-1AR subtypes couple to phosphoinositide hydrolysis in a pertussis toxin-insensitive manner, including the cloned human alpha-1a/dAR which had not been expressed previously. In spite of significant sequence differences between human alpha-1ARs and their other species counterparts, previously established ligand selectivity remains fairly comparable. In summary, these data represent the first side-by-side comparison of pharmacological properties between species homologs of alpha-1AR subtypes and should facilitate the development of alpha-1AR subtype selective drugs for clinical use.

Published

1995

22. Structure and chromosomal location of the gene for endothelial-leukocyte adhesion molecule 1.

Author

Collins T, Williams A, Johnston GI, Kim J, Eddy R, Shows T, Gimbrone MA Jr, and Bevilacqua MP

Subjects

Amino Acid Sequence, Base Sequence, Cell Adhesion Molecules, Chromosome Mapping, Consensus Sequence, E-Selectin, Exons, Genes, Humans, Introns, Molecular Sequence Data, Promoter Regions, Genetic, Regulatory Sequences, Nucleic Acid, Restriction Mapping, Transcription, Genetic, Cell Adhesion, Chromosomes, Human, Pair 1, Membrane Glycoproteins genetics

Abstract

Endothelial-leukocyte adhesion molecule 1 is a cell surface glycoprotein expressed by cytokine-activated endothelium that mediates the adhesion of blood neutrophils. Endothelial-leukocyte adhesion molecule 1 is a member of the selectin family of cell adhesion molecules each of which contain an amino-terminal lectin-like domain, followed by an epidermal growth factor-like domain and a variable number of short consensus repeats similar to those found in complement binding proteins. Genomic clones encoding the ELAM gene were isolated and the organization of the ELAM gene was determined. The gene, which is present in a single copy in the human genome, contains 14 exons spanning about 13 kilobases of DNA. The positions of exon-intron boundaries correlate with the putative functional subdivisions of the protein. Introns are found at similar positions in all of the six complement regulatory repeats, suggesting that these elements arose by internal gene duplication. A consensus TATAA element is located upstream of the transcriptional start site. The ELAM promoter contains an inverted CCAAT box and consensus NF-kappa B- and AP-1-binding sites. The ELAM gene was assigned to the q12 greater than qter region of human chromosome 1 by analysis of human-mouse hybrid cell lines. Two other members of the selectin gene family, the leukocyte adhesion molecule 1 (LAM-1, TQ1, LEC-CAM 1, or Leu-8) and the granule membrane protein 140 (GMP-140, PADGEM, or CD62) have been localized to the long arm of chromosome 1, as have the structurally related complement binding proteins, suggesting that these genes may share a common evolutionary history.

Published

1991

23. Structure of the human gene encoding granule membrane protein-140, a member of the selectin family of adhesion receptors for leukocytes.

Author

Johnston GI, Bliss GA, Newman PJ, and McEver RP

Subjects

Amino Acid Sequence, Base Sequence, Cloning, Molecular, Exons, Gene Library, Humans, Introns, Molecular Sequence Data, P-Selectin, Polymerase Chain Reaction, Protein Conformation, RNA Splicing, Restriction Mapping, Transcription, Genetic, Cell Adhesion Molecules genetics, Genes, Leukocytes metabolism, Multigene Family, Platelet Membrane Glycoproteins genetics

Abstract

GMP-140, an inducible granule membrane protein of platelets and endothelial cells, is a member of the selectin family of cell surface receptors that mediate interactions of leukocytes with the blood vessel wall. These molecules all contain an N-terminal lectin-like domain, followed by an epidermal growth factor-like domain, a variable number of consensus repeats related to those in complement-binding proteins, a transmembrane domain, and a cytoplasmic tail. Two variant cDNAs for GMP-140 have been identified, one predicting a soluble form of the molecule lacking the transmembrane domain and the other predicting a molecule containing eight instead of nine consensus repeats. Here we describe the organization of the human gene encoding GMP-140, which spans over 50 kilobase pairs and contains 17 exons. Almost all exons encode distinct structural domains, including the lectin-like domain, the epidermal growth factor-like domain, each of the nine consensus repeats, and the transmembrane region. Each of the two deletions found in the variant cDNAs is precisely encoded by an exon, suggesting that these forms of GMP-140 are derived from alternative splicing of mRNA. By using the polymerase chain reaction, transcripts encoding the putative soluble form of GMP-140 can be amplified from both platelet and endothelial cell RNA. The structure of the GMP-140 gene supports the concept that the selectins evolved as a result of exon duplication and rearrangement.

Published

1990

24. Genomic organization of the selectin family of leukocyte adhesion molecules on human and mouse chromosome 1.

Author

Watson ML, Kingsmore SF, Johnston GI, Siegelman MH, Le Beau MM, Lemons RS, Bora NS, Howard TA, Weissman IL, and McEver RP

Subjects

Animals, Blotting, Southern, Chromosome Banding, Crosses, Genetic, DNA Probes, E-Selectin, Gene Expression, Genetic Linkage genetics, Humans, Hybrid Cells, Mice, Mice, Inbred C3H, Multigene Family, Nucleic Acid Hybridization, P-Selectin, Receptors, Lymphocyte Homing, Restriction Mapping, Cell Adhesion Molecules genetics, Chromosomes, Human, Pair 1, Platelet Membrane Glycoproteins genetics, Receptors, Immunologic genetics

Abstract

A structurally and functionally related group of genes, lymph node homing receptor (LHR), granule membrane protein 140 (GMP-140), and endothelial leukocyte adhesion molecule 1 (ELAM-1) are shown to constitute a gene cluster on mouse and human chromosome 1. In situ hybridization mapped GMP-140 to human chromosome 1 bands 21-24 consistent with chromosomal localization of LHR. Gene linkage analysis in the mouse indicated that these genes and serum coagulation factor V (FV) all map to a region of distal mouse chromosome 1 that is syntenic with human chromosome 1, with no crossovers identified between these four genes in 428 meiotic events. Moreover, long range restriction site mapping demonstrated that these genes map to within 300 kb in both the human and mouse genomes. These data suggest that LHR, ELAM-1, and GMP-140 comprise an adhesion protein family, the selectins, that arose by multiple gene duplication events before divergence of mouse and human. Furthermore, the location of these genes on mouse and human chromosome 1 is consistent with a close evolutionary relationship to the complement receptor-related genes, which also are positioned on the same chromosomes in both species and with which these genes share a region of sequence homology. These data characterize the organization of a genomic region that may be critical for intercellular communication within the immune system.

Published

1990

25. Structural and biosynthetic studies of the granule membrane protein, GMP-140, from human platelets and endothelial cells.

Author

Johnston GI, Kurosky A, and McEver RP

Subjects

Amino Acids analysis, Disulfides analysis, Hexosaminidases metabolism, Humans, Molecular Weight, Oligosaccharides analysis, P-Selectin, Platelet Membrane Glycoproteins biosynthesis, Tunicamycin pharmacology, Blood Platelets analysis, Endothelium, Vascular analysis, Platelet Membrane Glycoproteins analysis

Abstract

GMP-140 is an integral membrane glycoprotein of apparent Mr = 140,000 located in secretory storage granules of platelets and vascular endothelial cells. When these cells are activated, GMP-140 redistributes from the membrane of the granules to the plasma membrane. To gain insight into the potential function of GMP-140, we examined aspects of its structure and biosynthesis. The amino acid composition of platelet GMP-140 revealed elevated numbers of cystinyl (6.1%), prolinyl (7.2%), and tryptophanyl (2.1%) residues. GMP-140 contained 28.8% carbohydrate by weight, distributed among N-acetylneuraminic acid, neutral sugar, and N-acetylglucosamine residues. Enzymatic removal of N-linked oligosaccarides reduced the protein's apparent Mr by more than 50,000. The biosynthesis of GMP-140 in HEL cells, which share biochemical features with megakaryocytes, was studied by pulse-chase labeling with [35S]cysteine followed by immunoprecipitation. HEL cells synthesized a heterogeneous GMP-140 precursor of 98-125 kDa which converted to a mature 140-kDa form within 40-60 min. Removal of high mannose oligosaccarides by endo-beta-N-acetylglucosaminidase H treatment reduced the apparent Mr of the precursor but not the mature protein. Tunicamycin-treated HEL cells synthesized three to four precursors of 80-92 kDa, suggesting the possibility of heterogeneity of GMP-140 at the protein level. Exposure of activated platelets to proteases followed by Western blotting indicated that most of the mass of GMP-140 was located on the extracytoplasmic side of the membrane. Our studies indicate that GMP-140 is a cysteine-rich, heavily glycosylated protein with a large extracytoplasmic domain. These features are compatible with a receptor function for the molecule when it is exposed on the surface of activated platelets and endothelial cells.

Published

1989

26. Are productivity and cost-effectiveness comparisons between in-house clinical engineering departments possible or useful?

Author

Johnston GI

Subjects

Reference Standards, United States, Biomedical Engineering standards, Cost-Benefit Analysis methods, Efficiency, Maintenance and Engineering, Hospital standards

Abstract

Inter-institutional comparisons of productivity and cost-effectiveness can be a valuable source of feedback to the in-house biomedical or clinical engineering services manager. But for such comparisons to be valid, all institutions must use the same criteria. As yet, there are no standard definitions for such criteria and, in most cases, the necessary data are not kept. Therefore, reliable comparisons are not possible. It is possible, however, to keep data on the variety of tasks common to all clinical engineering departments that can then be compared inter-institutionally. As task comparisons become more common, "norms" will evolve that can become standards for the profession. From there, it is a realizable step to standards that permit comparison of productivity and cost-effectiveness. A national organization, like the American Hospital Association could help by including clinical engineering data as part of their annual hospitals survey.

Published

1987

27. The expression of glycoproteins on single blood platelets from healthy individuals and from patients with congenital bleeding disorders.

Author

Johnston GI, Heptinstall S, Robins RA, and Price MR

Subjects

Fluorescent Antibody Technique, Glycoproteins isolation & purification, Humans, Membrane Proteins isolation & purification, Molecular Weight, Reference Values, Blood Platelets metabolism, Glycoproteins blood, Membrane Proteins blood, Thrombocytopenia blood

Abstract

Glycoproteins present on the surface of blood platelets are fundamental to normal blood platelet behaviour. We have used monoclonal antibodies and flow cytofluorimetry to study the expression of glycoproteins on single platelets from normal subjects, and from patients with Glanzmann's thrombasthenia and the Bernard-Soulier syndrome. We show that normal platelets are heterogeneous in that individual cells display markedly different numbers of glycoprotein IIb/IIIa complex and glycoprotein Ib molecules. We also show that the two congenital bleeding disorders are associated with markedly reduced numbers of glycoprotein IIb/IIIa complex or glycoprotein Ib molecules on all the platelets rather than the difference residing in a sub-population.

Published

1984

28. Identity of saturable calcium-binding sites on blood platelets and their involvement in platelet aggregation.

Author

Johnston GI and Heptinstall S

Subjects

Binding Sites, Glycoproteins metabolism, Humans, Magnesium pharmacology, Thrombasthenia metabolism, Blood Platelets metabolism, Calcium metabolism, Platelet Aggregation

Abstract

Extracellular Ca2+ ions are required for platelet aggregation and we show that they enter two platelet pools. One pool is rapidly filled and easily displaced by EGTA. The second is filled more slowly and is not displaced by EGTA. The EGTA-displaceable pool is believed to be surface-located and was found to contain at least one class of saturable binding sites as well as a class of non-saturable binding sites. The saturable sites were found to be highly selective for Ca2+ (dissociation constant, 3.5 X 10(-7) M) even in the presence of 1 mM Mg2+ ions, and they took up between 261,000 and 307,000 Ca2+ ions/platelet. Full occupancy of the saturable binding sites appeared to be necessary for platelet aggregation to proceed. We also studied platelets that were unable to aggregate normally, either due to the congenital bleeding disorder Glanzmann's thrombastenia or due to experimental manipulation. In both cases we found decreased Ca2+ uptake specifically by the saturable Ca2+ binding sites, and that this was associated with decreased number of GP IIb/IIIa molecules expressed on these platelets. We suggest that the Ca2+ binding sites involved in platelet aggregation are located on the GP IIb/IIIa complexes and may be involved in holding the glycoproteins in the complex together, and that the binding sites need to be fully occupied before aggregation can proceed.

Published

1988

29. A maintenance model for clinical engineering.

Author

Johnston GI

Abstract

The numbers presented here for an equipment maintenance model are derived from a mix of soft data and intuition based on experience. They relate best to university hospitals in the 250-400-bed range. They relate better to numbers of devices than number of beds. In summary, they are: 1. Ideal technician workload = 400 to 550 devices. 2. Average technician productivity or ;;hands-on'' maintenance time = 75%. 3. Average dollar value per device = $2,000. 4. Annual in-house maintenance ratio = 5% to 7% of value plus parts in excess of $200/item. 5. Effective rate per hour = $35 to $45/hr (depending upon region and labor costs in that region). 6. In-house maintenance costs should be less than outside costs. However, the in-house department should be aware of cost-effective outside options and employ them as appropriate. 7. Appropriate resources. 250 sq ft/technician, $20,000 capital equipment/technician, and $15 to $25/device in supplies. 8. Clinical engineers. One engineer to start the service and one engineer for each three additional technicians added. 9. Clerical support. One clerical FTE for a minimum 3 technician department, and one additional clerical FTE for each additional 1.5 FTE clinical engineers or each additional 5 FTE technicians. 10. Annual maintenance = 2.5 hr/device. (When clinical devices are distinguished from nonclinical devices, averages are 3 hr/clinical device and 2 hr/nonclinical device.) As clinical engineers, BMETs, and their departments gather experience to support or modify these numbers, I encourage them to share their findings in an experience pool available to all.

Published

1985

30. Cloning of GMP-140, a granule membrane protein of platelets and endothelium: sequence similarity to proteins involved in cell adhesion and inflammation.

Author

Johnston GI, Cook RG, and McEver RP

Subjects

Amino Acid Sequence, Base Sequence, Blotting, Northern, Blotting, Southern, Cytoplasmic Granules ultrastructure, DNA analysis, DNA isolation & purification, Endothelium, Vascular cytology, Endothelium, Vascular ultrastructure, Homeostasis, Humans, Inflammation metabolism, Intracellular Membranes analysis, Megakaryocytes cytology, Megakaryocytes ultrastructure, Membrane Proteins genetics, Membrane Proteins physiology, Molecular Sequence Data, P-Selectin, Platelet Membrane Glycoproteins analysis, Platelet Membrane Glycoproteins physiology, Protein Biosynthesis, Cell Adhesion, Cloning, Molecular, Cytoplasmic Granules analysis, Endothelium, Vascular analysis, Inflammation physiopathology, Megakaryocytes analysis, Membrane Proteins analysis, Platelet Membrane Glycoproteins genetics

Abstract

GMP-140 is an integral membrane glycoprotein found in secretory granules of platelets and endothelial cells. After cellular activation, it is rapidly redistributed to the plasma membrane. The cDNA-derived primary structure of GMP-140 predicts a cysteine-rich protein with multiple domains, including a "lectin" region, an "EGF" domain, nine tandem consensus repeats related to those in complement-binding proteins, a transmembrane domain, and a short cytoplasmic tail. Some cDNAs also predict a soluble protein with a deleted transmembrane segment. The domain organization of GMP-140 is similar to that of ELAM-1, a cytokine-inducible endothelial cell receptor that binds neutrophils. This similarity suggests that GMP-140 belongs to a new family of inducible receptors with related structure and function on vascular cells.

Published

1989

31. Effects of diamide and iodoacetamide on the expression of the glycoprotein IIb/IIIa complex on blood platelets.

Author

Johnston GI, Heptinstall S, and Lösche W

Subjects

Antibodies, Monoclonal, Arachidonic Acid, Arachidonic Acids pharmacology, Blood Platelets drug effects, Epitopes immunology, Glycoproteins immunology, Humans, Immunologic Techniques, Membrane Proteins immunology, Platelet Aggregation drug effects, Platelet Membrane Glycoproteins, Azo Compounds pharmacology, Blood Platelets metabolism, Diamide pharmacology, Glycoproteins blood, Iodoacetamide pharmacology, Iodoacetates pharmacology, Membrane Proteins blood

Abstract

We have examined the effects of two agents that alter platelet thiol-disulphide status on platelet aggregation and on the ability of platelets to bind a monoclonal antibody (M148) that is directed toward an epitope on the glycoprotein IIb/IIIa complex. The immediate effect of both diamide and iodoacetamide is to enhance aggregation but after further incubation diamide, but not iodoacetamide, inhibits platelet aggregation. Incubation of platelets with diamide, but not iodoacetamide, is accompanied by a marked increase in the amount of M148 that binds to platelets. This is presumably a reflection of an altered distribution of glycoproteins on the platelet surface. It is known that diamide, but not iodoacetamide, leads to polymerisation of cytoskeletal proteins in platelets. Thus evidence is provided that agents that interact with the cytoskeleton inhibit platelet behaviour via an effect on surface glycoproteins.

Published

1985

32. Platelet glycoprotein IIb. Chromosomal localization and tissue expression.

Author

Bray PF, Rosa JP, Johnston GI, Shiu DT, Cook RG, Lau C, Kan YW, McEver RP, and Shuman MA

Subjects

Amino Acid Sequence, Base Sequence, Cell Line, Humans, Leukemia, Erythroblastic, Acute genetics, Molecular Sequence Data, Chromosomes, Human, Pair 17, Platelet Membrane Glycoproteins genetics

Abstract

The GPIIb-IIIa complex functions as a receptor for cytoadhesive proteins on the platelet surface. Both GPIIb and GPIIIa are synthesized by a human erythroleukemia (HEL) cell line. We isolated several cDNA clones by screening a HEL cell cDNA library with an oligonucleotide derived from amino acid sequence of GPIIb. Nucleotide and amino acid sequences were determined from 703 bp of one of these clones. Amino acid sequence of purified platelet GPIIb peptides confirmed the identity of the clone. The cDNA encodes the carboxyl terminus of the large (alpha) subunit of GPIIb and all of the smaller (beta) subunit of GPIIb. By hybridizing the cDNA directly to chromosomes separated by dual laser chromosome sorting, the gene for GPIIb was mapped to chromosome 17. Northern blot analysis showed a approximately 3.4-kb GPIIb mRNA in HEL cells. We also compared the amino acid sequences determined from eight additional platelet GPIIb peptides with the derived amino acids from a published HEL cell GPIIb cDNA, and the platelet and HEL cell proteins appear to be the same. Despite previous reports that vascular endothelial cells and monocytes contain GPIIb, no GPIIb mRNA was observed in either type of cell. Thus, GPIIb appears to be specific for the platelet-megakaryocyte membrane and is distinct from the alpha subunits of the adhesion receptors in other normal tissues.

Published

1987

33. A lineoperated power supply for movable anode transducer tube.

Author

JOHNSTON GI and VUREK GG

Subjects

Electric Power Supplies, Electrodes, Physics instrumentation, Transducers

Published

1959

34. THE ROLE OF THE ENGINEER IN BIOLOGICAL RESEARCH.

Author

JOHNSTON GI

Subjects

Biology, Engineering, Research

Published

1963

35. Effect of changes in blood volume on body impedance.

Author

Underwood RJ, Gowing D, and Johnston GI

Subjects

Anesthesia, General, Animals, Cats, Dogs, Electrophysiology, Infusions, Parenteral, Blood Volume, Blood Volume Determination, Monitoring, Physiologic, Plethysmography, Impedance instrumentation

Published

1967

36. A simple integrating attachment for Servo recorders.

Author

Johnston GI, Morris RL, Conn RB Jr, and Kemnitz GW

Subjects

Chemistry, Clinical, Humans, Autoanalysis, Blood Protein Electrophoresis, Densitometry, Electronics, Medical

Published

1968

37. A sine wave constant-current biological stimulator.

Author

Roth JG, Johnston GI, and Macpherson CH

Subjects

Electric Stimulation, Electrophysiology instrumentation

Published

1967

38. A Vacuum tube oxygen polarograph.

Author

DAHNKE J, JOHNSTON GI, O'REILLY ME, and STARR A

Subjects

Vacuum, Equipment and Supplies, Heart, Heart, Artificial, Oximetry supply & distribution, Oxygen, Polarography

Published

1961

39. A twenty-four-channel temporal-event digital recording system.

Author

Morris RL, Johnston GI, Bailey DD, and Wiens AN

Subjects

Behavior, Electronics, Medical, Computers

Published

1968