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151. Effect of alkali cations on freeze-thaw-dependent reconstitution of amino acid transport from Ehrlich ascites cell plasma membrane.

Author

McCormick, J I, Silvius, J R, and Johnstone, R M

Abstract

Na+-dependent amino acid transport can be reconstituted by gel filtration of disaggregated plasma membrane and asolectin vesicles coupled to a freeze-thaw cycle. The resultant transport activity is markedly affected by the nature of the reconstitution medium. Reconstitution in K+ permits the formation of active liposomes, whereas reconstitution in Na+, Li+, or choline does not. Electron micrographs of K+ liposomes show a wide variation in liposome sizes. Ficoll density gradient fractionation of K+ liposomes shows that the largest vesicles are lipid rich, have the lowest density, and have the highest level of Na+-dependent amino acid transport. Liposomes formed in Na+ have a 34% smaller trapped volume than K+ liposomes and lack a population of large vesicles. A second freeze-thaw in K+ restores activity to Na+ liposomes which now contain large low density active vesicles. Fluorescence measurements of freeze-thaw-induced mixing of vesicle lipids indicates that the absence of large vesicles in Na+ liposomes is due to inhibition by Na+ of lipid vesicle fusion events during freezing and thawing. The large vesicle fraction is enriched in a 125-kDa peptide. It has not yet been established whether this peptide is part of the transport system for neutral amino acids.

Published
1985
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152. Selective externalization of an ATP-binding protein structurally related to the clathrin-uncoating ATPase/heat shock protein in vesicles containing terminal transferrin receptors during reticulocyte maturation.

Author

Davis, J Q, Dansereau, D, Johnstone, R M, and Bennett, V

Abstract

Transferrin receptors are lost from reticulocytes in vesicles that are released during the final stage of erythrocyte maturation (Pan, B. T., and Johnstone, R. M. (1983) Cell 33, 967-977). Transferrin receptor-containing vesicles have a major protein component present in a 1:1 ratio with the receptor that migrates on sodium dodecyl sulfate gels as two polypeptides of Mr = 71,000 and 72,000. The Mr = 71,000/72,000 doublet is indistinguishable from the clathrin-uncoating ATPase/heat shock protein based on cross-reaction with affinity-purified antibody against the uncoating protein, by comparison of peptide maps of the Mr = 72,000 and 71,000 polypeptides and the uncoating protein, and by selective binding of these polypeptides to ATP-agarose. This finding suggests a possible activity of proteins related to the uncoating/heat shock protein family in the disposal of aged membrane proteins by a pathway independent of lysosomes.

Published
1986
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153. Star Formation in Cooling Flows (Invited Paper)

Author

Nulsen, P. E. J., Johnstone, R. M., and Fabian, A. C.

Abstract

AbstractX-ray data show that substantial quantities of hot gas are cooling near the centres of many clusters and groups of galaxies. The existence of such cooling flows has been challenged because of the lack of evidence for star formation from the cooled gas. Spectra of cooling flow galaxies show filling in of the continuum shortward of the break at 4000 Å relative to normal elliptical galaxies. This is consistent with some continuing star formation. Extended regions of line emission are commonly associated with cooling flows. If the initial-mass-function of the newly formed stars which affect the 4000 Å break is like that which applies in the solar neighbourhood, then these stars can also power the line emission. The strength of the 4000 Å break is shown to correlate with the Hßflux in the manner expected when this is the case. This allows us to esimate the star formation rate from the line luminosity.The rate of star formation required to account for the line emission still falls well short of the rate at which gas is inferred to be cooling. It is argued that, nevertheless, the cooling gas is probably forming into stars. The overall initial-mass-function must be different from that which applies in the solar neighbourhood, but this should not be surprising given the different ambient conditions in a cooling flow.

Published
1987
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154. Protein kinase C does not phosphorylate the externalized form of the transferrin receptor

Author

Adam, M A and Johnstone, R M

Abstract

We have investigated the phosphorylation of transferrin receptors both in intact sheep reticulocytes and in isolated plasma membranes. Phosphorylation of the receptor in intact cells or isolated plasma membranes is stimulated by phorbol diesters, suggesting that protein kinase C may be involved. Identical [32P] phosphopeptide tryptic maps are formed in the presence and absence of phorbol diesters. Using heat-treated membranes (which are devoid of endogenous kinase activity) exogenous protein kinase C phosphorylates the same peptides as the endogenous kinase(s). During maturation of reticulocytes to erythrocytes, the transferrin receptor is released to the medium in vesicular form. In cells labelled with [32P]Pi, the released receptor is not labelled with 32P and the exocytosed vesicles do not phosphorylate receptor with [gamma-32P]ATP. The absence of 32P in the released receptor appears to be due to a change in the receptor, since, even in the presence of exogenous protein kinase C, the exocytosed receptor is phosphorylated to approximately 8% of the level obtained with receptors from the plasma membrane. These data suggest that during maturation and externalization the receptor is altered so that it loses its capacity to act as a substrate for exogenous protein kinase C as well as the endogenous kinase(s). This change may be a signal which segregates the receptor for externalization from the receptor pool remaining for transferrin recycling during the final stages of red cell maturation.

Published
1987
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155. Loss of the transferrin receptor during the maturation of sheep reticulocytes in vitro. An immunological approach

Author

Pan, B T, Blostein, R, and Johnstone, R M

Abstract

Sheep reticulocyte-specific antiserum absorbed with mature sheep red cells has been used to isolate and identify reticulocyte-specific plasma-membrane proteins and to monitor their loss during incubation in vitro. Specific precipitation of labelled plasma-membrane proteins is obtained when detergent-solubilized extracts of 125I-labelled reticulocyte plasma membranes are incubated with this antiserum and Staphyloccus aureus, but not when mature-cell plasma membranes are treated similarly. During maturation of reticulocytes in vitro (up to 4 days at 37 degrees C), there is a marked decrease in the immunoprecipitable material. The anti-reticulocyte-specific antibodies have been identified as anti-(transferrin receptor) antibodies. By using these antibodies as a probe, the transferrin receptor has been shown to have a subunit molecular weight of 93 000. The data are consistent with reported molecular weights of this receptor and with the proposal that the receptor may exist as a dimer, since [125I]iodotyrosyl-peptide maps of the 93 000- and 186 000-mol.wt. components isolated are shown to be identical. Evidence is presented for the transmembrane nature of the receptor and for the presence of different binding sites for transferrin and these antibodies on the receptor.

Published
1983
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156. A ROSATstudy of the cores of clusters of galaxies — I. Cooling flows in an X‐ray flux‐limited sample

Author

Peres, C. B., Fabian, A. C., Edge, A. C., Allen, S. W., Johnstone, R. M., and White, D. A.

Abstract

This is the first part of a study of the detailed X‐ray properties of the cores of nearby clusters. We have used the flux‐limited sample of 55 clusters listed by Edge et al., and archival and proprietary data from the ROSATobservatory. In this paper an X‐ray spatial analysis based on the surface‐brightness‐deprojection technique is applied to the clusters in the sample with the aim of studying their cooling flow properties. We determine the fraction of cooling flows in this sample to be 70–90 per cent, and estimate the contribution of the flow region to the cluster X‐ray luminosity. We show that the luminosity within a strong cooling flow can account for up to 70 per cent of a cluster X‐ray bolometric luminosity. Our analysis indicates that about 40 per cent of the clusters in the sample have flows depositing more than 100 M⊙ yr−1throughout the cooling region, and that these possibly have been undisturbed for many Gyr, confirming that cooling flows are the natural state of cluster cores. New cooling flows in the sample are presented, and previously ambiguous ones are clarified. We have constructed a catalogue of some intracluster medium properties for the clusters in this sample. The profiles of the mass deposited from cooling flows are analysed, and evidence is presented for the existence of breaks in some of the profiles. Comparison is made to recent optical and radio data. We cross‐correlate our sample with the Green Bank, NVSS and FIRST surveys, and with the volume‐limited sample of brightest cluster galaxies presented by Lauer &38; Postman. Although weak trends exist, no strong correlation between optical magnitude or radio power of the brightest cluster galaxy and the strength of the flow is found.

Published
1998
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157. Vesicle formation during reticulocyte maturation. Association of plasma membrane activities with released vesicles (exosomes).

Author

Johnstone, R M, Adam, M, Hammond, J R, Orr, L, and Turbide, C

Abstract

Vesicles are released during the in vitro culture of sheep reticulocytes which can be harvested by centrifugation at 100,000 X g for 90 min. These vesicles contain a number of activities, characteristic of the reticulocyte plasma membrane, which are known to diminish or disappear upon reticulocyte maturation. The activities include acetylcholinesterase, cytochalasin B binding (glucose transporter) nucleoside binding (i.e. nucleoside transporter), Na+-independent amino acid transport, and the transferrin receptor. Enzymes of cytosolic origin are not detectable or are present at low activity in the vesicles. Cultures of whole blood, mature red cells, or white cells do not yield comparable levels of these activities, supporting the conclusion that the activities arise from the reticulocytes. In addition, the lipid composition of the vesicles shows the high sphingomyelin content characteristic of sheep red cell plasma membranes, but not white cell or platelet membranes, also consistent with the conclusion that the vesicles are of reticulocyte origin. It is suggested that vesicle externalization may be a mechanism for shedding of specific membrane functions which are known to diminish during maturation of reticulocytes to erythrocytes.

Published
1987
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158. Simple and effective purification of a Na+-dependent amino acid transport system from Ehrlich ascites cell plasma membrane.

Author

McCormick, J I and Johnstone, R M

Abstract

A reconstitution assay was used to measure transport activity during purification of a Na+-dependent amino acid transporter from Ehrlich cell plasma membrane. Cholate/urea-solubilized membranes were fractionated on a Sepharose 6B column and transport activity was recovered in the column void volume. Centrifugation of the void volume fraction at 105,000 X g and reextraction of the pellet with 1% octyl glucoside led to recovery of an extract whose specific transport activity was nearly 30-fold higher than that of the original solubilized extract with a recovery of 38% of the original activity. The properties of amino acid uptake in the purified reconstituted transporter were identical to those in native plasma membrane vesicles. The major component present in the purified fraction had a molecular mass of 120-130 kDa. Strong evidence that this 120- to 130-kDa peptide contains a component of the amino acid transporter was obtained by immunoprecipitation of transport activity from solubilized membranes with an antibody against the 120- to 130-kDa peptide. This study tentatively identifies a component of the Na+-dependent amino acid transporter as a peptide with an apparent molecular mass of 120-130 kDa.

Published
1988
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159. Electron microscopic evidence for externalization of the transferrin receptor in vesicular form in sheep reticulocytes.

Author

Pan, B T, Teng, K, Wu, C, Adam, M, and Johnstone, R M

Abstract

Using ferritin-labeled protein A and colloidal gold-labeled anti-rabbit IgG, the fate of the sheep transferrin receptor has been followed microscopically during reticulocyte maturation in vitro. After a few minutes of incubation at 37 degrees C, the receptor is found on the cell surface or in simple vesicles of 100-200 nm, in which the receptor appears to line the limiting membrane of the vesicles. With time (60 min or longer), large multivesicular elements (MVEs) appear whose diameter may reach 1-1.5 micron. Inside these large MVEs are round bodies of approximately 50-nm diam that bear the receptor at their external surfaces. The limiting membrane of the large MVEs is relatively free from receptor. When the large MVEs fuse with the plasma membrane, their contents, the 50-nm bodies, are released into the medium. The 50-nm bodies appear to arise by budding from the limiting membrane of the intracellular vesicles. Removal of surface receptor with pronase does not prevent exocytosis of internalized receptor. It is proposed that the exocytosis of the approximately 50-nm bodies represents the mechanism by which the transferrin receptor is shed during reticulocyte maturation.

Published
1985
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160. In vitro acylation of the transferrin receptor.

Author

Adam, M, Rodriguez, A, Turbide, C, Larrick, J, Meighen, E, and Johnstone, R M

Abstract

In vitro fatty acylation of the transferrin receptor with [3H]tetradecanoate or [3H]tetradecanoyl-CoA has been demonstrated for isolated sheep reticulocyte plasma membranes. Although less than 5% of the receptor was labeled in vitro, the acylated protein could be readily observed after sodium dodecyl sulfate-gel electrophoresis. The acylated transferrin receptor in the reticulocyte membrane was specifically precipitated with a monoclonal antibody and was absent from mature red cell membranes. Incorporation of fatty acid was dependent on ATP, and fatty acid was 5-10 times less effective as an acyl donor than the acyl-CoA derivative, pointing out the strong potential of this reagent for in vitro acylation of membrane proteins. During in vitro maturation of reticulocytes, the receptor is released in vesicles into the incubation medium. Using reticulocytes labeled with [3H]tetradecanoate, it can be shown that the 3H-labeled receptor is transferred from the cells to the vesicles without loss of acyl groups, suggesting that the vesiculation process does not involve deacylation.

Published
1984
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161. Solubilization and reconstitution of a nucleoside-transport system from Ehrlich ascites-tumour cells

Author

Hammond, J R and Johnstone, R M

Abstract

Uptake of [3H]uridine by Ehrlich cells was mediated by both nitrobenzylthioinosine (NBMPR)-sensitive (75%) and NBMPR-insensitive (25%) mechanisms. Each cell contained approx. 26,000 high-affinity (KD = 0.19 nM) recognition sites for [3H]NBMPR, and binding was inhibited by dipyridamole and adenosine at concentrations similar to those required for inhibition of [3H]uridine uptake. Calculations show that each cell contains a total of about 35,000 nucleoside transporters. Photoaffinity labelling of a partially purified preparation of plasma membranes with [3H]NBMPR resulted in a single broad 3H-labelled band on SDS/polyacrylamide gels, with an apparent molecular-mass peak of 42 kDa. This is in contrast with human erythrocyte membranes, where [3H]NBMPR photolabelled two broad bands with peaks at 55 and 80 kDa. Treatment of photoaffinity-labelled membranes with endoglycosidase F decreased the apparent molecular masses of both the Ehrlich-cell and erythrocyte [3H]NBMPR-labelled proteins to approx. 40 kDa. These results suggest that the human erythrocyte [3H]NBMPR-binding polypeptides are more extensively glycosylated than the corresponding Ehrlich-cell polypeptides. Octyl beta-D-glucopyranoside [1.0% (w/v) + asolectin] solubilized over 90% of the [3H]NBMPR-binding sites, with near-complete retention of [3H]NBMPR-binding characteristics. The only major change was a 65-fold decrease in affinity for dipyridamole, which was partly reversed upon incorporation of the solubilized proteins into asolectin membranes. Proteoliposomes, prepared by using asolectin and the octyl glucoside-solubilized plasma membranes, were capable of accumulating [3H]uridine via a protein-dependent dipyridamole/nitrobenzylthioguanosine/dilazep-sensitive mechanism. We have thus demonstrated the efficient solubilization and functional reconstitution of a nucleoside-transport system from Ehrlich ascites-tumour cells.

Published
1989
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162. Phosphorylation of choline and ethanolamine in Ehrlich ascites-carcinoma cells

Author

Sung, Cheng-Po and Johnstone, R. M.

Abstract

1. Ehrlich ascites-cell extracts convert choline and ethanolamine approximately equally well into their respective phosphoryl derivatives. 2. Choline is a potent inhibitor of ethanolamine phosphorylation, but ethanolamine has little effect on choline phosphorylation. 3. 2,3-Dimercaptopropanol, cysteine and Ca2+ inhibit ethanolamine phosphorylation, but have no detectable effect on choline phosphorylation. 4. Choline-phosphorylating activity in Ehrlich ascites-cell extracts is more stable during storage than ethanolamine-phosphorylating activity. 5. Choline phosphorylation is stimulated in the presence of benzoylcholine, succinylcholine, butyrylcholine and propionylcholine, whereas ethanolamine phosphorylation is inhibited. This relationship is reciprocal: the compounds causing the greatest stimulation of choline phosphorylation bring about the greatest inhibition of ethanolamine phosphorylation.

Published
1967
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163. ACTIVE TRANSPORT OF ASCORBIC ACID IN ADRENAL CORTEX AND BRAIN CORTEX IN VITRO AND THE EFFECTS OF ACTH AND STEROIDS

Author

Sharma, Shail K., Johnstone, R. M., and Quastel, J. H.

Abstract

Uptake of ascorbic acid-1-C14in brain cortex and adrenal cortex slices is an energy-dependent process. Concentration ratios (i.e. ratios of tissue ascorbic acid-1-C14to medium ascorbic acid-1-C14) greater than 4 have been obtained with both tissues in vitro. Ouabain as well as 2, 4-dinitrophenol suppresses ascorbic acid uptake into brain cortex slices.ACTH inhibits the uptake of ascorbic acid-1-C14in adrenal cortex, but not in brain cortex slices. The presence of glucose is necessary for the inhibition. Several cortical steroids, as well as adenosine-3′,5′-monophosphate, at small concentrations inhibit the uptake. The results are consistent with the interpretation that ACTH inhibits the uptake of ascorbic acid in the adrenal cortex through the steroids produced in its presence.

Published
1963
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164. ARGININE UPTAKE AND ARGINASE ACTIVITY IN EHRLICH ASCITES CARCINOMA CELLS

Author

Johnstone, R. M.

Abstract

Anaerobic glycolysis in Ehrlich ascites tumor cells exposed to amino acids leads to an increased uptake of a number of the amino acids to levels comparable with those obtained under aerobic conditions. The arginine uptake in the cell is not increased by glucose. Anaerobically the arginase activity is inhibited when glucose is present. The inhibition appears to be the result of an increased retention in the cell of the ornithine produced by arginase activity.

Published
1959
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165. Mastery Learning in Modern Languages - a Case Study

Author

Parkinson, B. L., Mitchell, R. F., and Johnstone, R. M.

Abstract

Five teachers of French in first year classes, using a package of mastery learning materials devised by the researchers, were followed through two units of instruction (approximately ten weeks). This paper describes the materials used, and the data collected by systematic lesson observation, by analysis of test results and by interviews with the teachers, and offers tentative conclusions on the effectiveness of mastery learning as a strategy for foreign language teaching in the Scottish school context.

Published
1971
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166. Specificity of action of adrenocorticotrophin in vitro on ascorbate transport in rat adrenal glands

Author

Clayman, M., Tsang, D., De Nicola, A. F., and Johnstone, R. M.

Abstract

The inhibition of ascorbate transport by rat adrenal quarters in response to steroidogenesis in vitro was shown to be highly specific with respect to tissue, substrate and steroidogenic agent. The transport system in vitro is capable of net accumulation of ascorbate. The evidence is consistent with the conclusion that ascorbate `depletion' in the adrenal gland is due to a specific block by corticoids of the uptake of ascorbate.

Published
1970
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193. Critical perspectives on modern languages in Scottish further education 2000-2002

Author

Doughty, Hannelore and Johnstone, R. M.

Subjects
378, Languages, Modern - Study and teaching - Scotland, modern languages, scotland, further education, policy, motivation, critical theory, self-determination theory
Abstract

The research in this thesis focuses on issues surrounding modern language provision within Scottish further education during the period 2000-2002. The study analyses the arguments regarding the place of modern language study within Scottish further education (FE) as expressed in formal and informal discourses, and assesses the influence of socio-cultural and socio-historical assumptions on these discourses. To this end, a multi-strand and multi-level research model was adopted, examining official and other public documents, together with views expressed by stakeholders from five Scottish FE colleges and from industry. These were analysed both on their own terms and by taking into account changes in the external context. The initial focus of the study centred on the motivational characteristics of student participants. However, changes in the external context prompted the inclusion of further data into the research design and a shift of methodological emphasis, exploring the ways in which assumptions underlying data collection procedures related to labour market information and uptake of individual FE subjects may be contributing to a continuous re-affirmation that 'English is enough'. The validity of this assertion and the authority accorded to it are called into question. It is argued that the belief will increasingly limit Scottish FE students' potential to participate as self-confident and self-determining individuals in a global and multilingual economy for which their vocational education and training is ostensibly trying to prepare them. Some suggestions, arising from the research, for a more inclusive language education policy are considered.

Published
2005

194. Attitudes to and motivation for learning English in Japan

Author

Seki, Taeko and Johnstone, R. M.

Subjects
428.071152, College students Japan Attitudes, English language Study and teaching Foreign speakers, English language Study and teaching Japan, Japan, EFL, English education, TEFL, ELT, attitudes, motivation, language teaching
Abstract

The aim of this research is to determine Japanese first-year university students’ attitudes to and motivation for learning English. A successful English-language education system is crucial for Japan, under great pressure to internationalise during her most prolonged recession ever. To help make the education system successful, knowledge of learners’ attitudes and motivation is essential. Chapter 1 discusses Japan as a stage for English-language education. Japan is identified as uniquely homogenous and insular. Internationalisation of industry and a drop in the college-age population forcing universities to compete for students are identified as recent phenomena driving reform in the English-language education system. Chapter 2 describes the roughly 130-year history of Japanese English-language education from first contact to the present day. Changes in the English-language education policies of successive Japanese governments are discussed through examination of the Ministry of Education ‘Course of Study’ guidelines. Chapter 3 surveys the theoretical literature on attitudes and motivation in foreign and second language learning. Significant and relevant empirical research from Japan and other countries is reviewed. Chapter 4 determines an approach to the main research question through a number of subsidiary questions, using the theoretical framework from Chapter 3. A detailed research design (methods, schedule, and data collection procedures) is drawn up and discussed. Chapter 5 presents and analyses the findings of the two questionnaires which form the main data collection method. The computer program SPSS is used in analysis. Chapter 6 presents and analyses the findings of the two group interviews and two individual interviews by categorising and descriptive explanation. Chapter 7, the final chapter, reviews the research process and answers the subsidiary and main research questions. Key themes are that Japanese students are highly motivated to learn English for communication, and that the English classes currently offered at universities do not meet the demands of Japanese students. These answers and themes are used as the basis for some recommendations for English-language education in Japan.

Published
2004

195. HST imaging of the dusty filaments and nucleus swirl in NGC4696 at the centre of the Centaurus Cluster.

Author

Fabian, A. C., Walker, S. A., Russell, H. R., Pinto, C., Canning, R. E. A., Salome, P., Sanders, J. S., Taylor, G. B., Zweibel, E. G., Conselice, C. J., Combes, F., Crawford, C. S., Ferland, G. J., Gallagher III, J. S., Hatch, N. A., Johnstone, R. M., and Reynolds, C. S.

Subjects
*IMAGING systems in astronomy, *BLACK holes, *GALAXY clusters, *GAS flow, *CENTAURUS (Constellation)
Abstract

Narrow-band HST imaging has resolved the detailed internal structure of the 10 kpc diameter H α+[N II] emission line nebulosity in NGC4696, the central galaxy in the nearby Centaurus cluster, showing that the dusty, molecular, filaments have a width of about 60 pc. Optical morphology and velocity measurements indicate that the filaments are dragged out by the bubbling action of the radio source as part of the active galactic nucleus feedback cycle. Using the drag force we find that the magnetic field in the filaments is in approximate pressure equipartition with the hot gas. The filamentary nature of the cold gas continues inwards, swirling around and within the Bondi accretion radius of the central black hole, revealing the magnetic nature of the gas flows in massive elliptical galaxies. HST imaging resolves the magnetic, dusty, molecular filaments at the centre of the Centaurus cluster to a swirl around and within the Bondi radius. [ABSTRACT FROM AUTHOR]

Published
2016
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196. Characteristics of the interaction between Hsc70 and the transferrin receptor in exosomes released during reticulocyte maturation.

Author

Géminard C, Nault F, Johnstone RM, and Vidal M

Subjects
Adenosine Triphosphatases metabolism, Animals, Binding, Competitive, Blotting, Western, Brain metabolism, Chromatography, Agarose, Cytosol metabolism, Electrophoresis, Polyacrylamide Gel, HSC70 Heat-Shock Proteins, Hot Temperature, Immunoblotting, Immunosuppressive Agents pharmacology, Luciferases metabolism, Molecular Chaperones metabolism, Precipitin Tests, Protein Binding, Protein Structure, Tertiary, Rats, Recombinant Proteins metabolism, Sheep, Temperature, Time Factors, HSP70 Heat-Shock Proteins metabolism, Receptors, Transferrin metabolism, Reticulocytes metabolism
Abstract

The transferrin receptor (TfR) of reticulocytes is released in vesicular form (exosomes) during their maturation to erythrocytes. The heat shock cognate 70-kDa protein (Hsc70) has been demonstrated to interact with the cytosolic domain of the TfR and could thus trigger the receptor toward this secretion pathway. We investigated the characteristics of the interaction between Hsc70 and the TfR in exosomes with an in vitro binding assay using TfR immobilized on Sepharose beads and purified Hsc70. The results show that Hsc70 binds to exosomal TfR with characteristics expected of a chaperone/peptide interaction. We demonstrated that heat-denatured luciferase competed for in vitro binding, dependent on the nucleotide bound to Hsc70, and that this interaction activates the ATPase activity of Hsc70. Moreover, we used immunosuppressive agents that interact with Hsc70, thus decreasing Hsc70 binding to TfR in our in vitro binding assay and enabling us to assess the role of this interaction in vivo during reticulocyte maturation.

Published
2001
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197. Mutated-gamma-actin restores growth to a yeast amino acid transport defective mutant.

Author

Khamessan A, Naghibalhossaini F, Vedadi M, and Johnstone RM

Subjects
Amino Acid Sequence genetics, Amino Acid Transport Systems, Base Sequence genetics, Carrier Proteins metabolism, Cell Division drug effects, Cell Line, Transformed, Cycloheximide pharmacology, DNA Transposable Elements, Ions, Molecular Sequence Data, Proline pharmacology, Protein Synthesis Inhibitors pharmacology, Quaternary Ammonium Compounds pharmacology, RNA, Messenger genetics, RNA, Messenger metabolism, Yeasts cytology, Yeasts drug effects, Yeasts metabolism, Actins genetics, Actins pharmacology, Carrier Proteins genetics, Mutation, Yeasts genetics
Abstract

A mutated yeast cell 22574d lacking all three proline transporters, PUT4, UGA4, and GAP1, and incapable of growth on proline recovers its lost ability to grow on proline as sole nitrogen source when transformed with a mutagenized mouse gamma-actin cDNA (M-gamma-A). Native mouse gamma-actin cDNA is ineffective. The 3'-region of gamma-actin cDNA was mutagenized to resemble E51 cDNA previously isolated from Ehrlich tumor cells. The E51 cDNA has an extended reading frame in the 3'-region compared to that in native gamma-actin. The extension of the open reading frame in E51 cDNA, was found to be due to an additional pair of bases (TG) at position 1104 of E51 cDNA. After site-directed mutagenesis of the 3'-region of native gamma-actin cDNA to resemble that of E51 cDNA, the construct, M-gamma-A cDNA, was expressed in the 22574d yeast. While the transformation with M-gamma-A increased the uptake of both proline and gamma-amino butyric acid, the transport of five other solutes was not changed by this transformation. Northern blotting of the nontransformed and the M-gamma-A-transformed 22574d cells with gene-specific probes for the three proline transporters showed the expression of an mRNA for UGA4 in both transformed and nontransformed cells but no evidence for the expression of GAP1 or PUT4. The mRNA for UGA4 was expressed at a lower level in strain 22574d than in the parent yeast sigma1278b. Furthermore, the message in the mutated cells is smaller in size by about 15%. These results are consistent with the synthesis of a mutated transporter which requires the coexpression of M-gamma-A, but not native gamma-actin, to restore physiological function, i.e., proline or gamma-amino acid transport.

Published
2001
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198. Loss of glucose transport in developing avian red cells.

Author

Johnstone RM, Mathew A, Setchenska MS, Grdisa M, and White MK

Subjects
Animals, Biological Transport, Active, Bone Marrow Cells cytology, Butyrates pharmacology, Butyric Acid, Cell Line, Chickens, Deoxyglucose metabolism, Erythroblasts metabolism, Erythrocytes cytology, Glucose genetics, Glucose Transporter Type 3, Hemin pharmacology, Monosaccharide Transport Proteins biosynthesis, Monosaccharide Transport Proteins genetics, Nucleosides metabolism, RNA, Messenger biosynthesis, RNA, Messenger drug effects, RNA, Messenger metabolism, Temperature, Bone Marrow Cells metabolism, Erythrocytes metabolism, Erythropoiesis, Glucose metabolism, Nerve Tissue Proteins
Abstract

Although red cells are generally associated with significant glucose transport and dependence on glycolysis, the mature red cells of some species (e.g. pig) show very low glucose transport. The generally low level of glucose transport in mature mammalian red cells is the result of maturational development, since it has been shown that even in red cells which have negligible glucose transport (e.g. pig red cells) the corresponding reticulocytes have significant glucose transport activity. The reticulocytes of the chicken, however, show minimal glucose transport activity. But this also is the result of maturational development, since chicken bone marrow red cells do transport glucose which diminishes upon cell maturation in vitro. The erythroblast chicken cell line, HD3, has high glucose transport activity which is lost upon induction to the red cell phenotype. Growing HD3 cells have much higher levels of transport than native chicken bone marrow cells and this is associated in part with elevation of glucose transporter (GLUT) mRNAs as a consequence of the expression of the v-erbA and v-erbB oncogenes. Both native bone marrow red cells and HD3 cells, when incubated in vitro under conditions where maturation occurs, show substantial losses of GLUT mRNA and GLUT proteins. To assess whether the inducers of maturation (hemin and butyrate) affect only the normally expressed GLUTs, chicken GLUT3 expressed from a different promoter was introduced into the HD3 cell by retroviral infection. Both the endogenous and exogenous transporters were lost upon cell differentiation and maturation, leaving a cell with low glucose transport activity. Conversely, in growing cells, butyrate had a pronounced effect on the elevation of the GLUT3 mRNA, especially on the exogenous GLUT3 mRNA, and elevated glucose transport prior to differentiation. These results are consistent with the conclusion that chicken red cell development involves a requirement to reduce glucose transport activity. The near absence of glucose transport in the embryonic chicken red cell is thus due to a loss of this transporter during early development which occurs at an earlier developmental stage in the chicken red cell than in the mammalian red cell.

Published
1998
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199. Expression cloning of a mammalian amino acid transporter or modifier by complementation of a yeast transport mutant.

Author

Lin G, Cai X, and Johnstone RM

Subjects
Amino Acid Sequence, Amino Acid Transport Systems, Aminoisobutyric Acids metabolism, Animals, Base Sequence, Biological Transport, Carrier Proteins biosynthesis, Carrier Proteins chemistry, Cell Line, Cloning, Molecular, DNA, Complementary, Gene Library, Genetic Complementation Test, Kinetics, Leucine metabolism, Male, Mammals, Mice, Molecular Sequence Data, Muscle, Skeletal, Organ Specificity, Polymerase Chain Reaction, Proline metabolism, Protein Biosynthesis, RNA, Messenger biosynthesis, Rats, Recombinant Proteins biosynthesis, Recombinant Proteins chemistry, Recombinant Proteins metabolism, Saccharomyces cerevisiae genetics, Transcription, Genetic, Carrier Proteins metabolism, Saccharomyces cerevisiae growth & development
Abstract

A cDNA clone named L21 was isolated from L6 rat muscle cells by complementation of a yeast proline transport mutant. L21 cDNA has 2,268 bp and codes for a peptide of 228 amino acids with four potential transmembrane domains. The amino acid sequence of L21 shows no homology to any known proteins. Expression of L21 cDNA enables the mutant yeast to grow in proline as the sole nitrogen source and to transport proline, alpha-aminoisobutyric acid (AIB) and leucine. The Km for proline is about 1.0 mM. The substrate specificity of L21 expressed in yeast shows no striking similarity to known mammalian amino acid transporters.

Published
1997
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200. Cleavage of the transferrin receptor by human granulocytes: differential proteolysis of the exosome-bound TFR.

Author

Johnstone RM

Subjects
Acetylcholinesterase metabolism, Affinity Labels metabolism, Animals, Blotting, Western, Cell Membrane enzymology, Cytoplasm metabolism, Enzyme Stability, Humans, Membrane Proteins metabolism, Organelles metabolism, Protease Inhibitors pharmacology, Sheep, Temperature, Thioinosine analogs & derivatives, Thioinosine metabolism, Transferrin metabolism, Trypsin metabolism, Endopeptidases metabolism, Granulocytes enzymology, Receptors, Transferrin metabolism, Reticulocytes metabolism
Abstract

In contrast with other mammalian granulocytes, human granulocytes rapidly cleave the transferrin receptor (TFR) from sheep exosomes. Proteolysis of TFR from exosomes is more rapid and more extensive than that from the sheep reticulocyte cell surface itself, although little difference in cleavage is seen when immunoprecipitates or when immobilized, solubilized receptors from the two sources are compared. Circulating exosomes but not the plasma membrane fraction from seven species of immature red cells or erythropoietic cells show the presence of a peptide of approximately 18 kD recognized by an antibody to the cytoplasmic domain of the TFR. This 18 kD peptide is virtually absent from the corresponding cellular plasma membranes including human reticulocyte membranes. Taken together, the data are consistent with the conclusion that the exosomes released to the circulation from maturing red cells are the principal source of the soluble, circulating, truncated TFR. The granulocyte protease appears to be present on the cell surface and not released into the medium after short (30 min) periods of incubation at 37 degrees C. The protease is inhibited by PMSF but only at high (1 mM) concentrations. Using sheep exosome bound-TFR as substrate, human granulocytes exceed other granulocytes in their capacity to cleave TFR, suggesting that this may be a key factor for the prominent amount of circulating, soluble receptor found in human sera during periods of elevated reticulocyte levels. Human exosomes, unlike those from other species, contain little native size TFR. Truncated receptor containing the cytoplasmic domain being predominant in human exosomes.

Published
1996
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