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Author

J H, Keen

Subjects
Time Factors, Drug Therapy, Injections, Intravenous, Humans, Emergency Nursing
Published
1995
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3. Modulation of the arrestin-clathrin interaction in cells. Characterization of beta-arrestin dominant-negative mutants

Author

J G, Krupnick, F, Santini, A W, Gagnon, J H, Keen, and J L, Benovic

Subjects
Arrestin, GTP-Binding Proteins, COS Cells, Mutagenesis, Site-Directed, Animals, Humans, Cattle, Receptors, Adrenergic, beta-2, Clathrin, Endocytosis, Cell Line, Genes, Dominant, Protein Binding
Abstract

We recently demonstrated that nonvisual arrestins interact via a C-terminal binding domain with clathrin and function as adaptor proteins to promote beta2-adrenergic receptor (beta2AR) internalization. Here, we investigated the potential utility of a mini-gene expressing the clathrin-binding domain of beta-arrestin (beta-arrestin (319-418)) to function as a dominant-negative with respect to beta2AR internalization and compared its properties with those of beta-arrestin and beta-arrestin-V53D, a previously reported dominant-negative mutant. In vitro studies demonstrated that beta-arrestin-V53D bound better to clathrin than beta-arrestin but was significantly impaired in its interaction with phosphorylated G protein-coupled receptors. In contrast, whereas beta-arrestin (319-418) also bound well to clathrin it completely lacked receptor binding activity. When coexpressed with the beta2AR in HEK293 cells, beta-arrestin (319-418) effectively inhibited agonist-promoted receptor internalization, whereas beta-arrestin-V53D was only modestly effective. However, both constructs significantly inhibited the stimulation of beta2AR internalization by beta-arrestin in COS-1 cells. Interestingly, immunofluorescence microscopy analysis reveals that both beta-arrestin (319-418) and beta-arrestin-V53D are constitutively localized in clathrin-coated pits in COS-1 cells. These results indicate the potential usefulness of beta-arrestin (319-418) to effectively block arrestin-clathrin interaction in cells and suggest that this construct may prove useful in further defining the mechanisms involved in G protein-coupled receptor trafficking.

Published
1998

4. Role of arrestins in G-protein-coupled receptor endocytosis

Author

O B, Goodman, J G, Krupnick, F, Santini, V V, Gurevich, R B, Penn, A W, Gagnon, J H, Keen, and J L, Benovic

Subjects
Arrestins, Cell Membrane, Transfection, Models, Biological, Clathrin, Endocytosis, Recombinant Proteins, Cell Line, GTP-Binding Proteins, Cricetinae, COS Cells, Animals, Humans, Receptors, Adrenergic, beta-2, Adrenergic alpha-Agonists, Signal Transduction
Published
1997

5. Arrestin/clathrin interaction. Localization of the clathrin binding domain of nonvisual arrestins to the carboxy terminus

Author

J G, Krupnick, O B, Goodman, J H, Keen, and J L, Benovic

Subjects
Alanine, Binding Sites, Transcription, Genetic, Arrestins, Recombinant Fusion Proteins, Molecular Sequence Data, Transfection, Clathrin, Kinetics, Protein Biosynthesis, COS Cells, Mutagenesis, Site-Directed, Animals, Cattle, Amino Acid Sequence, Receptors, Adrenergic, beta-2, Glutathione Transferase, Sequence Deletion
Abstract

We have recently demonstrated that the nonvisual arrestins, beta-arrestin and arrestin3, interact with high affinity and stoichiometrically with clathrin, and we postulated that this interaction mediates internalization of G protein-coupled receptors (Goodman, O. B., Jr., Krupnick, J. G., Santini, F., Gurevich, V. V., Penn, R. B., Gagnon, A. W., Keen, J. H., and Benovic, J. L. (1996) Nature 383, 447-450). In this study, we localized the clathrin binding domain of arrestin3 using a variety of approaches. Truncation mutagenesis demonstrated that the COOH-terminal half of arrestin3 is required for clathrin interaction. Assessment of the clathrin binding properties of various glutathione S-transferase-arrestin3 fusion proteins indicated that the predominant clathrin binding domain is contained within residues 367-385. Alanine scanning mutagenesis further localized this domain to residues 371-379, and site-directed mutagenesis demonstrated the critical importance of both hydrophobic (Leu-373, Ile-374, and Phe-376) and acidic (Glu-375 and Glu-377) residues in the arrestin3/clathrin interaction. These results are complementary to the observation that hydrophobic and basic residues in clathrin are critical for its interaction with nonvisual arrestins (Goodman, O. B. , Jr., Krupnick, J. G., Gurevich, V. V., Benovic, J. L., and Keen, J. H. (1997) J. Biol. Chem. 272, 15017-15022). Lastly, an arrestin3 mutant in which Leu-373, Ile-374, and Phe-376 were mutated to Ala was significantly defective in its ability to promote beta2-adrenergic receptor internalization in COS-1 cells when compared with wild-type arrestin3. Taken together, these results implicate a discrete region of arrestin3 in high affinity binding to clathrin, an interaction critical for agonist-promoted internalization of the beta2-adrenergic receptor.

Published
1997

6. Arrestin/clathrin interaction. Localization of the arrestin binding locus to the clathrin terminal domain

Author

O B, Goodman, J G, Krupnick, V V, Gurevich, J L, Benovic, and J H, Keen

Subjects
Alanine, Arrestin, Arrestins, Glutamine, Lysine, Recombinant Fusion Proteins, Molecular Sequence Data, Polymerase Chain Reaction, Clathrin, Escherichia coli, Mutagenesis, Site-Directed, Animals, Cattle, Amino Acid Sequence, Cloning, Molecular, Sequence Alignment, Conserved Sequence, beta-Arrestins, Glutathione Transferase, Sequence Deletion
Abstract

Previously we demonstrated that nonvisual arrestins exhibit a high affinity interaction with clathrin, consistent with an adaptor function in the internalization of G protein-coupled receptors (Goodman, O. B., Jr., Krupnick, J. G., Santini, F., Gurevich, V. V., Penn, R. B., Gagnon, A. W., Keen, J. H., and Benovic, J. L. (1996) Nature 383, 447-450). In this report we show that a short sequence of highly conserved residues within the globular clathrin terminal domain is responsible for arrestin binding. Limited proteolysis of clathrin cages results in the release of terminal domains and concomitant abrogation of arrestin binding. The nonvisual arrestins, beta-arrestin and arrestin3, but not visual arrestin, bind specifically to a glutathione S-transferase-clathrin terminal domain fusion protein. Deletion analysis and alanine scanning mutagenesis localize the binding site to residues 89-100 of the clathrin heavy chain and indicate that residues 1-100 can function as an independent arrestin binding domain. Site-directed mutagenesis identifies an invariant glutamine (Glu-89) and two highly conserved lysines (Lys-96 and Lys-98) as residues critical for arrestin binding, complementing hydrophobic and acidic residues in arrestin3 which have been implicated in clathrin binding (Krupnick, J. G., Goodman, O. B., Jr., Keen, J. H., and Benovic, J. L. (1997) J. Biol. Chem. 272, 15011-15016). Despite exhibiting high affinity clathrin binding, arrestins do not induce coat assembly. The terminal domain is oriented toward the plasma membrane in coated pits, and its binding of both arrestins and AP-2 suggests that this domain is the anchor responsible for adaptor-receptor recruitment to the coated pit.

Published
1997

7. Mapping of the molecular determinants involved in the interaction between eps15 and AP-2

Author

G, Iannolo, A E, Salcini, I, Gaidarov, O B, Goodman, J, Baulida, G, Carpenter, P G, Pelicci, P P, Di Fiore, and J H, Keen

Subjects
Binding Sites, Base Sequence, Calcium-Binding Proteins, Molecular Sequence Data, Intracellular Signaling Peptides and Proteins, Membrane Proteins, 3T3 Cells, Phosphoproteins, Peptide Mapping, Peptide Fragments, Recombinant Proteins, Adaptor Proteins, Vesicular Transport, Mice, Adaptor Protein Complex alpha Subunits, Animals, Adaptor Proteins, Signal Transducing
Abstract

eps15, a substrate for the epidermal growth factor receptor and other receptor tyrosine kinases, possesses a discrete domain structure with protein-binding properties. It interacts with a number of cellular proteins through an evolutionarily conserved protein-binding domain, the eps15 homology domain, located in its NH2-terminal region. In addition, a proline-rich region, located in the COOH-terminal portion of eps15, can bind to the Src homology 3 domain of the crk proto-oncogene product in vitro. Recently, coimmunoprecipitation between eps15 and AP-2, a major component of coated pits, was reported. Here, we characterize the molecular determinants of the eps15/AP-2 interaction. The AP-2 binding region of eps15 is localized in its COOH-terminal region and spans approximately 80 amino acids. At least three molecular determinants, located at residues 650-660, 680-690, and 720-730, are involved in the binding. AP-2 binds to eps15 through its alpha subunit (alpha-adaptin); in particular, the COOH-terminal region of alpha-adaptin, the so-called alpha-ear, contains the eps15 binding region.

Published
1997

8. Giving medications to different age groups

Author

J H, Keen

Subjects
Adult, Adolescent, Drug Therapy, Child, Preschool, Body Weight, Age Factors, Infant, Newborn, Humans, Infant, Middle Aged, Child, Mathematics, Aged
Published
1994

9. Clathrin assembly protein AP-3 is phosphorylated and glycosylated on the 50-kDa structural domain

Author

J E, Murphy, J A, Hanover, M, Froehlich, G, DuBois, and J H, Keen

Subjects
Binding Sites, Glycosylation, Protein Conformation, Galactose, Nerve Tissue Proteins, Phosphoproteins, Clathrin, Acetylglucosamine, Rats, Adaptor Proteins, Vesicular Transport, Monomeric Clathrin Assembly Proteins, Animals, Cattle, Phosphorylation, Protein Processing, Post-Translational, Cells, Cultured
Abstract

AP-3 (AP180) in rat sympathetic neurons maintained in culture was analyzed by pulse-chase labeling with [35S]methionine to look for post-translational modifications. At early times, two lower molecular weight precursors of the mature species were detected. By 10 min, all of the AP-3 was found in the mature form which is stable for at least 9 h. We show here that at least one of these processing events is due to the addition of O-linked N-acetylglucosamine (GlcNAc) which is present on the mature form of the protein. Wheat germ agglutinin, a GlcNAc-specific probe, bound to AP-3 and the binding was blocked by excess GlcNAc but not by excess mannose. Purified AP-3, and AP-3 in coated vesicles derived from bovine brain, served as substrates for beta-D-galactosyltransferase which is specific for terminal GlcNAc residues. Analysis of the disaccharide released by beta-elimination indicated that single GlcNAc residues are attached to AP-3 through an O-glycosidic linkage to threonine or serine residues. In vivo 32P-labeled AP-3, the result of serine phosphorylation (Keen, J. H., and Black, M.M. (1986) J. Cell Biol. 102, 1325-1333), bound to wheat germ agglutinin-Sepharose indicating that phosphorylation and glycosylation can occur simultaneously on the same molecule. Both modifications have been mapped to the central 50-kDa structural domain that is responsible for the anomalous migration of AP-3. Consistent with localization to the nonclathrin binding domain, the O-GlcNAc modification does not play a discernible role in the interaction of AP-3 with clathrin.

Published
1994

10. Recognition sites for clathrin-associated proteins AP-2 and AP-3 on clathrin triskelia

Author

J E, Murphy and J H, Keen

Subjects
Adaptor Proteins, Vesicular Transport, Binding Sites, Protein Conformation, Hydrolysis, Monomeric Clathrin Assembly Proteins, Electrophoresis, Polyacrylamide Gel, Trypsin, Phosphoproteins, Clathrin
Abstract

AP-2 and AP-3 are cellular proteins that drive the in vitro polymerization of clathrin triskelia into cage structures. The interaction of these two types of assembly proteins (APs) with preassembled clathrin cages has been studied in order to identify the sites on the triskelia required for binding. Comparing binding of the APs to intact or to proteolytically clipped cages, we attempted to distinguish between binding to the terminal domain, the globular end of the heavy chain, and binding to the hub of the clathrin triskelia, the portion that remains assembled after trypsin treatment. AP-3 binds to intact clathrin cages but not to those that were treated with trypsin. AP-3 also bound to cages consisting solely of clathrin heavy chains; proteolysis of these cages also eliminated AP-3 binding. In addition, AP-3 did not bind to either isolated hubs or terminal domains that had been immobilized on Sepharose. These data indicate that clathrin light chains are not required for binding of AP-3, and that neither terminal domain nor hubs alone will suffice. However, an intact heavy chain is both necessary and sufficient for the binding of AP-3. Previous work has demonstrated one binding site for AP-2 on proteolyzed cages containing only clathrin hubs; the existence of a second binding site associated with the terminal domain was hypothesized. Here we provide direct evidence for recognition by AP-2 of isolated terminal domains immobilized on Sepharose and show that the core of the AP-2 molecule is responsible for this interaction. These results provide the first demonstration of a functional role for the conserved terminal domain of the clathrin heavy chain.

Published
1992

11. Clathrin domains involved in recognition by assembly protein AP-2

Author

J H, Keen, K A, Beck, T, Kirchhausen, and T, Jarrett

Subjects
Polyphosphates, Animals, Cattle, Coated Pits, Cell-Membrane, Electrophoresis, Polyacrylamide Gel, Carrier Proteins, Clathrin
Abstract

The domains on clathrin responsible for interaction with the plasma membrane-associated assembly protein AP-2 have been studied using a novel cage binding assay. AP-2 bound to pure clathrin cages but not to coat structures already containing AP that had been prepared by coassembly. Binding to preassembled cages also occurred in the presence of elevated Tris-HCl concentrations (greater than or equal to 200 mM) which block AP-2 interactions with free clathrin. AP-2 interactions with assembled cages could also be distinguished from AP-2 binding to clathrin trimers by sodium tripolyphosphate (NaPPPi), which binds to the alpha subunit of AP-2 (Beck, K., and Keen, J. H. (1991) J. Biol. Chem. 266, 4442-4447). At concentrations of 1-5 mM, NaPPPi blocked clathrin-triskelion binding; in contrast, interactions with cages persisted in the presence of 25 mM NaPPPi. To begin to identify the region(s) of the clathrin molecule important in recognition by AP-2, clathrin cages were proteolyzed to remove heavy chain terminal domains and portions of the distal leg as well as all of the light chains. AP-2 bound to these "clipped cages"; however, unlike the interaction with native cages, binding of AP-2 to clipped cages was sensitive to the lower concentrations of both Tris-HCl and NaPPPi which disrupt interactions of AP-2 with clathrin trimers. Reconstitution of the clipped cages with clathrin light chains did not restore resistance of AP-2 binding to Tris-HCl. We conclude that one binding site for AP-2 resides on the hub and/or proximal part of the clathrin triskelion whereas a second site is likely to involve the terminal domain and/or distal leg; the second site is manifested only in the assembled lattice structure. We suggest that these two distinct binding interactions may be mediated by the two unique large subunits within the AP-2 complex, acting sequentially during assembly.

Published
1991

12. Self-association of the plasma membrane-associated clathrin assembly protein AP-2

Author

K A, Beck and J H, Keen

Subjects
Adaptor Proteins, Vesicular Transport, Structure-Activity Relationship, Macromolecular Substances, Monomeric Clathrin Assembly Proteins, Animals, Cattle, Coated Pits, Cell-Membrane, Hydrogen-Ion Concentration, In Vitro Techniques, Phosphoproteins, Clathrin, Peptide Fragments, Protein Binding
Abstract

A self-association reaction involving the plasma membrane-associated clathrin assembly protein AP-2 has been detected by incubating AP-2 alone under solution conditions that would favor the assembly of complete coat structures if clathrin were present. Self-association was rapid, unaffected by nonionic detergents, readily reversible, and gave rise to sedimentable aggregates. Only the AP subtype AP-2 exhibited self-association: the structurally or functionally related assembly proteins AP-1 and AP-3 and unrelated proteins neither self-associated nor were incorporated into the AP-2 aggregate. AP-2 interactions responsible for self-association were of high affinity, with an apparent Kd of approximately 10(-8)M. By proteolytic dissection, the self-association domain was localized to the core of the molecule containing the intact 50- and 16-kDa polypeptides in association with the truncated 60-66-kDa moieties of the parent alpha/beta polypeptides. Self-association of the intact AP-2 molecule was pH-dependent, exhibiting an apparent pKa approximately 7.4. While it is unlikely that the large AP-2 aggregates formed in solution are themselves biologically relevant structures, the AP-2 interactions involved in their formation have properties consistent with their occurrence in intact cells and thus may be important in cellular functions of the plasma membrane-localized assembly protein.

Published
1991

13. Interaction of phosphoinositide cycle intermediates with the plasma membrane-associated clathrin assembly protein AP-2

Author

K A, Beck and J H, Keen

Subjects
Phosphatidylinositol 4,5-Diphosphate, Phytic Acid, Macromolecular Substances, Affinity Labels, Coated Pits, Cell-Membrane, Inositol 1,4,5-Trisphosphate, In Vitro Techniques, Phosphatidylinositols, Phosphoproteins, Clathrin, Adaptor Proteins, Vesicular Transport, Structure-Activity Relationship, Adenosine Triphosphate, Animals, Cattle, Magnesium, Protein Binding
Abstract

Several components of the phosphoinositide cycle have been found to interact specifically and at physiological concentrations with the plasma membrane-associated clathrin assembly (adaptor) protein AP-2. These include phosphatidylinositol 4,5-bisphosphate and inositol 1,4,5-trisphosphate, which are present at the plasma membrane, as well as other polyphosphoinositols. ATP and other polyphosphate molecules complete with the polyphosphoinositols, however, they are at least 80-fold less potent. Also, the effect of ATP, unlike the polyphosphoinositols, is blocked by physiological concentrations of Mg2+. Photoaffinity labeling of AP-2 by [alpha-32P]8-azidoadenosine 5'-triphosphate and its competition by polyphosphoinositols has been used to identify the alpha subunit of the AP-2 complex as the site of specific interaction with the polyphosphoinositols and to confirm direct ultrafiltration binding experiments. Proteolytic dissection of the labeled AP-2 demonstrated that binding occurred exclusively on the N-terminal portion of the alpha subunit. Interaction of purified AP-2 with sub-microM concentrations of polyphosphoinositols has inhibitory effects on a novel AP-2 self-association described in the accompanying paper (Beck, K. A., and Keen, J. H., J. Biol. Chem. 266, 4437-4441), and at higher concentrations on the binding of AP-2 to dissociated clathrin trimers as well as AP-2-mediated clathrin coat assembly. Review of the literature shows that several physiological stimuli that are known to result in increased coat pit formation in intact cells correlate with increased phosphoinositide turnover. These in vivo correlations and the in vitro observations reported here suggest that coated membrane and phosphoinositide cycles may be interdependent within cells.

Published
1991

14. Clathrin assembly protein AP-3. The identity of the 155K protein, AP 180, and NP185 and demonstration of a clathrin binding domain

Author

J E, Murphy, I T, Pleasure, S, Puszkin, K, Prasad, and J H, Keen

Subjects
Antibodies, Monoclonal, In Vitro Techniques, Phosphoproteins, Peptide Mapping, Clathrin, Peptide Fragments, Molecular Weight, Adaptor Proteins, Vesicular Transport, Monomeric Clathrin Assembly Proteins, Immunologic Techniques, Animals, Cattle, Electrophoresis, Gel, Two-Dimensional, Trypsin
Abstract

Three independently isolated clathrin-associated proteins have been reported that have molecular weights of approximately 155,000-185,000 on sodium dodecyl sulfate-polyacrylamide gel electrophoresis: the 155K protein (Keen, J. H., and Black, M. M. (1986) J. Cell Biol. 102, 1325-1333), AP 180 (Ahle, S., and Ungewickell, E. (1986) EMBO J. 5, 3143-3149), and NP185 (Kohtz, D. S., and Puszkin, S. (1988) J. Biol. Chem. 263, 7418-7425). Using two-dimensional isoelectric focusing polyacrylamide gel electrophoresis and one- and two-dimensional immunoblots with two different monoclonal antibodies, we show that these three proteins are identical. The term AP-3 is used to denote this protein. A preliminary analysis of the domain structure of AP-3 was done by controlled proteolysis. Trypsin treatment of AP-3 yields two distinct classes of products. The larger fragments obtained (100,000-135,000 apparent Mr) are acidic and behave anomalously on gel electrophoresis, yielding aberrantly high Mr and exhibiting poor dye binding; these characteristics are shared with intact AP-3. Trypsin also generates a smaller neutral species of approximately 30,000 Da which migrates appropriately on sodium dodecyl sulfate-gel electrophoresis, binds dye comparatively strongly, and behaves as a monomeric globular species in solution. In addition, this species, which is also released by a variety of other proteases, binds specifically and reversibly to clathrin-Sepharose, identifying it as a clathrin recognition domain.

Published
1991

15. Peltigera membranacea

Author

J. H. Keen, J. H. Keen, J. H. Keen, and J. H. Keen

Abstract

Lichens, http://name.umdl.umich.edu/IC-HERB00IC-X-118272%5DMICH-F-118272, https://quod.lib.umich.edu/cgi/i/image/api/thumb/herb00ic/118272/MICH-F-118272/!250,250, The University of Michigan Library provides access to these materials for educational and research purposes. Some materials may be protected by copyright. If you decide to use any of these materials, you are responsible for making your own legal assessment and securing any necessary permission. If you have questions about the collection, please contact the Herbarium professional staff: herb-dlps-help@umich.edu. If you have concerns about the inclusion of an item in this collection, please contact Library Information Technology: libraryit-info@umich.edu., https://www.lib.umich.edu/about-us/policies/copyright-policy

Published
1898

16. Mechanism for the several activities of the glutathione S-transferases

Author

J H Keen, William H. Habig, and William B. Jakoby

Subjects
chemistry.chemical_classification, Thiocyanate, Stereochemistry, Cell Biology, Glutathione, Biochemistry, Enzyme catalysis, Catalysis, chemistry.chemical_compound, chemistry, Nucleophile, Thioether, Electrophile, Thiol, Molecular Biology
Abstract

The catalyzed reactions of GSH with organic nitrate and thiocyanate esters and with a series of chloronitrobenzene substrates have been investigated and the results used to formulate a mechanism for glutathione S-transferase catalysis. All the homogeneous preparations of the glutathione transferases that have been tested catalyze the reaction of GSH with organic nitrates and thiocyanates. The nature of the reaction with nitrate esters, resulting in the formation of GSSG rather than a thioether, has been investigated further. The presence of an additional nonsubstrate thiol decreased the formation of GSSG to an extent that cannot be explained by disulfide interchange. These results are interpreted to reflect the enzymatic formation of an unstable glutathione sulfenyl nitrite that undergoes subsequent non-enzymatic decomposition. Hammett plots of the catalytic constants of rat liver transferases B and C obtained with a series of 4-substituted 1-chloro-2-nitrobenzene substrates demonstrate a linear relationship with sigma- substituent constants, reflecting the nucleophilic nature of the enzymatic reactions and their strong dependence on the electrophilicity of the nonthiol substrate. These data suggest that the many diverse reactions catalyzed by the glutathione transferases may be formulated as a nucleophilic attack of enzyme-bound GSH on the electrophilic center of the second substrate. The final products observed reflect this primary event and the existence of subsequent nonenzymatic reactions.

Published
1976
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17. Clathrin and coated vesicle proteins Immunological characterization

Author

J H Keen, Mark C. Willingham, and Ira Pastan

Subjects
Antiserum, Molecular mass, medicine.diagnostic_test, biology, Immunoprecipitation, Coated vesicle, Coated Pit, Cell Biology, Immunofluorescence, Biochemistry, Molecular biology, Clathrin, Isoelectric point, medicine, biology.protein, Molecular Biology
Abstract

Antisera to a purified extract of bovine brain coated vesicles have been prepared. The extract contained clathrin (greater than 90%) and polypeptides of 35,000 (less than 5%) and 38,000 (less than 5%) molecular weight. Antibodies to clathrin were affinity purified on a homogeneous clathrin-Sepharose column and demonstrated to be monospecific by sensitive immunoprecipitation and immunofluorescence experiments. These antibodies give a fluorescence pattern consistent with coated pit localization in cultured cells from diverse species indicating extensive cross-reaction, and, thus, conservation of the clathrin antigen. Antibodies to the lower molecular weight proteins (LMWP) present in the clathrin preparation were also affinity purified on a column containing these polypeptides but devoid of clathrin. These antibodies cross-reacted completely and immunoprecipitated only clathrin from 3T3 cell extracts. Although the molecular weights and isoelectric points of the LMWP presented are quite similar to tropomyosins, these immunological results and limited protease digestion data indicate that tropomyosin and the LMWP are not related. Rather, the latter may be breakdown products of clathrin.

Published
1981
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18. Deep-etch visualization of 27S clathrin: a tetrahedral tetramer

Author

R E Lippoldt, John E. Heuser, L M Amende, K Prasad, and J H Keen

Subjects
Models, Molecular, Macromolecular Substances, Protein Conformation, Clathrin, chemistry.chemical_compound, Protein structure, Tetramer, Animals, Molecule, biology, Freeze Etching, Brain, Coated Pits, Cell-Membrane, Articles, Cell Biology, Molecular Weight, Microscopy, Electron, Crystallography, Biochemistry, chemistry, Ionic strength, Polylysine, biology.protein, Tetrahedron, Cattle, Mica
Abstract

It has recently been reported that 8S clathrin trimers or "triskelions" form larger 27S oligomers upon dialysis into low ionic strength buffers (Prasad, K., R. E. Lippoldt, H. Edelhoch, and M. S. Lewis, 1986, Biochemistry, 25:5214-5219). Here, deep-etch electron microscopy of the 27S species reveals that they are closed tetrahedra composed of four clathrin triskelions. This was determined by two approaches. First, standard quick-freezing and freeze-etching of unfixed 27S species suspended in 2 mM 2-(N-morpholino)ethane sulfonic acid (MES) buffer, pH 5.9, yielded unambiguous images of tetrahedra that measured 33 nm on each edge. Second, the technique of freeze-drying molecules on mica (Heuser, J. E., 1983, J. Mol. Biol., 169:155-195) was modified to overcome the low affinity of mica in 2 mM MES, by pretreating the mica with polylysine. Thereafter, 27S species adsorbed avidly to it and collapsed into characteristic configurations containing four globular domains, each linked to the others by three approximately 33-nm struts. The globular domains look like vertices of deep-etched clathrin triskelions and the links, numbering 12 in all, look like four sets of triskelion legs. New light scattering and equilibrium centrifugation data confirm that 27S polymer is four times as massive as one clathrin triskelion. We conclude that in conditions that do not favor the formation of standard clathrin cages, low affinity interactions lead to closed, symmetrical assemblies of four triskelions, each of which assumes a unique puckered, straight-legged configuration to create the edges of a tetrahedron. Tetrahedra are similar in construction to the cubic octomers of clathrin recently found in ammonium sulfate solutions (Sorger, P. K., R. A. Crowther, J. T. Finch, and B. M. F. Pearse, 1986, J. Cell Biol., 103:1213-1219) but are still smaller, involving only half as many clathrin triskelions.

Published
1987
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19. Glutathione transferases. Catalysis of nucleophilic reactions of glutathione

Author

W B Jakoby and J H Keen

Subjects
chemistry.chemical_classification, Maleic acid, Stereochemistry, Cell Biology, Glutathione, Biochemistry, Catalysis, chemistry.chemical_compound, Enzyme, chemistry, Nucleophile, Electrophile, Organic chemistry, Binding site, Molecular Biology, Isomerization
Abstract

Homogeneous preparations of the glutathione transferases from rat liver have been tested for their ability to catalyze a number of diverse nucleophilic reactions of GSH. Although disulfide interchange with GSSG or L-cystine, and cis-trans isomerization of maleic acid, are clearly promoted by thiols in solution, the reactions were not catalyzed by the glutathione transferases. In contrast, certain more hydrophobic analogs of these compounds were found to serve as substrates. The transferases also catalyze the glutathione-dependent release of p-nitrophenol from p-nitrophenyl acetate and p-nitrophenyl trimethylacetate. These observations are consistent with the formulation that catalysis may result from close juxtaposition of sufficiently electrophilic, nonpolar compounds with GSH on the enzyme surface.

Published
1978
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20. Assembly polypeptides from coated vesicles mediate reassembly of unique clathrin coats

Author

J H Keen and S Zaremba

Subjects
Endosome, Coated vesicle, Endosomes, Biology, Clathrin binding, Clathrin, symbols.namesake, Animals, Vesicle, Temperature, Coated Pits, Cell-Membrane, Articles, Cell Biology, Hydrogen-Ion Concentration, Golgi apparatus, Molecular Weight, Sedimentation coefficient, Microscopy, Electron, Membrane, Biochemistry, symbols, Biophysics, biology.protein, Cattle, Electrophoresis, Polyacrylamide Gel, Peptides
Abstract

A protein activity has been identified in extracts of coated vesicles that enables purified clathrin triskelions to reassemble in vitro into coat structures of uniform size. Coats formed in the presence of this preparation, regardless of the buffer system employed, are uniform in size with a mean diameter of 78 nm (+/- 5 nm SD) and a sedimentation coefficient (S20,w) of approximately 250S. Analysis of the reassembled coats on dodecyl sulfate acrylamide gels reveals that they have specifically incorporated three polypeptides from the preparation: those of Mr congruent to 52,000, 100,000, and 110,000. The 52,000-, 100,000-, and 110,000-mol-wt polypeptides are incorporated in molar ratios of 0.85, 1.11, and 0.26, respectively, per three clathrin monomers (equivalent to one triskelion). We therefore designate these as assembly polypeptides (AP). In contrast, coats formed from clathrin alone, under permissive buffer conditions, are larger (400S), more heterogeneous in size (101 nm +/- 15 nm SD), and are composed only of clathrin and its associated light chains. These biochemical and biophysical characteristics distinguish AP-reassembled coats from coats formed by triskelions alone. AP-reassembled coats can be isolated, dissociated, then reassembled in the absence of any other factors. This recycling indicates that all the information needed for reassembly is present in the coat-incorporated polypeptides themselves. Reassembly is stoichiometric and saturable with respect to both clathrin and AP concentration. In the presence of AP, significant coat reassembly occurs at clathrin concentrations as low as 0.06 mg/ml. AP-mediated reassembly proceeds at 4 degrees, 22 degrees, and 37 degrees C. Coat formation also proceeds efficiently at intracellular pH values (7.2-7.5) in the presence of AP. In its absence, reassembly does not occur at all above pH 6.7. In summary, AP promotes clathrin reassembly into coat structures of uniform size and distinctive composition under physiologically relevant salt, temperature, and pH conditions. In addition, the close similarity in size between AP-reassembled coats in vitro and coated membranes in the Golgi region in vivo raises the possibility that AP in the cell may be associated with this subpopulation of coat structures.

Published
1983
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21. Deep-etch visualization of proteins involved in clathrin assembly

Author

J H Keen and John E. Heuser

Subjects
Polymers, Coated vesicle, Biology, Endocytosis, Clathrin coat, Clathrin, Chromatography, Affinity, Adaptor Protein Complex alpha Subunits, Freezing, Animals, Brain Chemistry, Pancreatic Elastase, Freeze Etching, Vesicle, Proteins, Cell Biology, Articles, Microscopy, Electron, Membrane, Freeze Drying, Biochemistry, Biophysics, biology.protein, Clathrin adaptor proteins, Aluminum Silicates, Cattle
Abstract

Assembly proteins were extracted from bovine brain clathrin-coated vesicles with 0.5 M Tris and purified by clathrin-Sepharose affinity chromatography, then adsorbed to mica and examined by freeze-etch electron microscopy. The fraction possessing maximal ability to promote clathrin polymerization, termed AP-2, was found to be a tripartite structure composed of a relatively large central mass flanked by two smaller mirror-symmetric appendages. Elastase treatment quantitatively removed the appendages and clipped 35 kD from the molecule's major approximately 105-kD polypeptides, indicating that the appendages are made from portions of these polypeptides. The remaining central masses no longer promote clathrin polymerization, suggesting that the appendages are somehow involved in the clathrin assembly reaction. The central masses are themselves relatively compact and brick-shaped, and are sufficiently large to contain two copies of the molecule's other major polypeptides (16- and 50-kD), as well as two copies of the approximately 70-kD protease-resistant portions of the major approximately 105-kD polypeptides. Thus the native molecule seems to be a dimeric, bilaterally symmetrical entity. Direct visualization of AP-2 binding to clathrin was accomplished by preparing mixtures of the two molecules in buffers that marginally inhibit AP-2 aggregation and cage assembly. This revealed numerous examples of AP-2 molecules binding to the so-called terminal domains of clathrin triskelions, consistent with earlier electron microscopic evidence that in fully assembled cages, the AP's attach centrally to inwardly-directed terminal domains of the clathrin molecule. This would place AP-2s between the clathrin coat and the enclosed membrane in whole coated vesicles. AP-2s linked to the membrane were also visualized by enzymatically removing the clathrin from brain coated vesicles, using purified 70 kD, uncoating ATPase plus ATP. This revealed several brick-shaped molecules attached to the vesicle membrane by short stalks. The exact stoichiometry of APs to clathrin in such vesicles, before and after uncoating, remains to be determined.

Published
1988

22. Structural and functional division into two domains of the large (100- to 115-kDa) chains of the clathrin-associated protein complex AP-2

Author

A. Vaisberg, J. H. Keen, William Matsui, Alvin E. Davis, C. Burne, E. P. Chow, Katherine L. Nathanson, and Tomas Kirchhausen

Subjects
Adaptor Protein Complex sigma Subunits, Macromolecular Substances, Molecular Sequence Data, Adaptor Protein Complex 2, Coated vesicle, Clathrin binding, Clathrin, Adaptor Protein Complex alpha Subunits, Animals, Amino Acid Sequence, Cloning, Molecular, Peptide sequence, Multidisciplinary, Base Sequence, biology, Vesicle, Coated Pits, Cell-Membrane, DNA, Phosphoproteins, Adaptor Protein Complex mu Subunits, Peptide Fragments, Rats, Molecular Weight, Adaptor Proteins, Vesicular Transport, Biochemistry, biology.protein, Biophysics, Cattle, Research Article
Abstract

The clathrin-associated protein complex 2 (AP-2 complex) is a group of proteins associated with clathrin-coated vesicles and believed to interact with cytoplasmic domains of receptors found in the plasma membrane. AP-2 was purified as an assembly of several polypeptide chains (alpha, beta, AP50, and AP17), of which only the alpha and beta chains (100-115 kDa) show significant heterogeneity. We have obtained cDNA clones for two distinct rat brain beta chains. We have also studied the domain organization of bovine brain AP-2 complexes by selective proteolysis. Results of these studies show that the alpha and beta chains have a similar two-domain organization. Their amino-terminal domains are relatively invariant whereas their carboxyl-terminal domains are variable in both sequence and length. We propose that the variable domains select receptors for inclusion in coated vesicles.

Published
1989
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23. LIST OF COLEOPTERA COLLECTED AT MASSETT, QUEEN CHARLOTTE ISLANDS, B. C

Author

J. H. Keen

Subjects
Geography, Physiology, Structural Biology, Insect Science, Molecular Biology, Archaeology, Ecology, Evolution, Behavior and Systematics, Queen (playing card)
Abstract

The beetles enumerated below were all taken within a circle of five miles' radius from Massett, on the Northern Shore of Graham Island—the most northerly of the Queen Charlotte group. This area, though small, is considerably diversified, and favourable to coleopterous life. The island here is flat, and covered with a forest of spruce and hemlock, with a sprinkling of alder. The soil is sandy, and for the most part dry. The coastline includes a stretch of level sand reached only by the highest tides, and strewn with driftwood; a protected pebbly beach and a tract of rough stones, also covered by the high tides. The sandy beach I find most productive, many even inland insects appearing to fall on the loose sand, and, being unable to rise, crawl for shelter under the driftwood. Hills and fresh-water streams (of any size) are absent, and I quite expect these situations, which occur in other parts of the island, to yield, when examined, several additional species.

Published
1895
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24. Significance of hypocalcaemia in neonatal convulsions

Author

J. H. Keen

Subjects
Male, Pediatrics, medicine.medical_specialty, Hypoglycemia, Infant, Newborn, Diseases, Milk products, Pregnancy, Seizures, Neonatal convulsions, medicine, Animals, Humans, Hypocalcaemia, Infant Nutritional Physiological Phenomena, Hypocalcemia, business.industry, Age Factors, Infant, Newborn, Infant, medicine.disease, Infant newborn, Milk, England, Blood chemistry, Pediatrics, Perinatology and Child Health, Calcium, Female, Seasons, business, Research Article
Published
1969
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25. THREE INTERESTING STAPHYLINIDÆ FROM QUEEN CHARLOTTE ISLANDS

Author

J. H. Keen

Subjects
Geography, Physiology, Structural Biology, Insect Science, Ancient history, Molecular Biology, Ecology, Evolution, Behavior and Systematics, Queen (playing card)
Abstract

At the request of Dr. James Fletcher, I am writing a few notes to accompany the three figures which have been made at his instance, and kindly presented by him. They represent three Staphylinidæ taken by me at Massett, on the Queen Charlotte Islands, and were prepared under the direction of Mons. A. Fauvel, the well-known specialist in that order, to whom also I am indebted for the determination of the beetles themselves.

Published
1897
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26. Farber's disease (lysosomal acid ceramidase deficiency)

Author

J. H. Keen, R. A. Jameson, and P. J. L. Holt

Subjects
medicine.medical_specialty, Acid Ceramidase, Immunology, Arthritis, Disease, Lipidoses, Gastroenterology, General Biochemistry, Genetics and Molecular Biology, Cachexia, Amidohydrolases, Rheumatology, Internal medicine, Convulsion, medicine, Ceramidases, Immunology and Allergy, Humans, Farber disease, business.industry, Infant, Syndrome, medicine.disease, Acid Ceramidase Deficiency, Endocrinology, Hoarse voice, Female, medicine.symptom, business, Lysosomes, Research Article
Abstract

The patient presented with progressive joint deformity, a hoarse voice, subsequent cachexia, and myoclonic seizures. She was first seen aged 22 months and died aged 6 years. A diagnosis of Farber's disease was made by demonstrating a deficiency of acid ceramidase both in leucocytes and fibroblasts.

Published
1987

27. The clathrin coat assembly polypeptide complex. Autophosphorylation and assembly activities

Author

J H, Keen, M H, Chestnut, and K A, Beck

Subjects
Macromolecular Substances, Adaptor Protein Complex 2, Brain, Coated Pits, Cell-Membrane, Endosomes, Phosphoproteins, Clathrin, Adaptor Protein Complex mu Subunits, Molecular Weight, Adaptor Proteins, Vesicular Transport, Kinetics, Adenosine Triphosphate, Animals, Cattle, Phosphorylation, Phosphorus Radioisotopes
Abstract

A 50-kDa polypeptide that is rapidly phosphorylated on addition of [gamma-32P]ATP to isolated clathrin-coated vesicles is shown here to be identical to the 50-kDa component (AP50) of the clathrin assembly protein (AP), a complex that promotes the assembly of clathrin coat structures under physiological conditions of pH and ionic strength. Phosphorylation of the AP50 occurred readily at 0 degrees C, almost exclusively on a threonyl residue(s). This reaction is attributable to autophosphorylation, since the AP50 was able to covalently incorporate 32P from [gamma-32P]ATP after separation by either one- or two-dimensional sodium dodecyl sulfate gel electrophoresis. Kinetic studies in solution were consistent with an intramolecular phosphorylation event; in addition, a concentration-dependent increase in AP50 phosphorylation was observed that may reflect intermolecular AP-AP activation of autophosphorylation. The phosphorylated AP50 was resistant to several inorganic phosphatases tested but was a substrate for protein phosphatases 1 and 2A, suggesting that a physiological phosphorylation-dephosphorylation cycle may exist. The phosphorylation state of the AP50 did not affect the ability of the AP to promote in vitro clathrin coat assembly. These and other data suggest that unique structural domains of the assembly protein are responsible for assembly (the 100-kDa components) and autophosphorylation (the AP50) and that the latter may be active as a protein kinase in the intact cell.

Published
1987

28. The milk of human kindness

Author

J H, Keen

Subjects
Celiac Disease, Breast Feeding, Hypercalcemia, Infant, Newborn, Humans, Infant Food, Obesity, Infant Nutritional Physiological Phenomena, Infant Nutrition Disorders
Published
1975

29. Care of the Child with Diabetes

Author

J H Keen

Subjects
medicine.medical_specialty, Text mining, business.industry, Family medicine, Diabetes mellitus, Pediatrics, Perinatology and Child Health, medicine, business, medicine.disease, Book Review
Published
1987

30. The child's perception of the disease and the experience of pain in juvenile chronic arthritis

Author

J G, Beales, J H, Keen, and P J, Holt

Subjects
Male, Adolescent, Humans, Pain, Female, Perception, Psychology, Child, Child, Arthritis, Juvenile
Abstract

Interviews conducted among 39 children with juvenile chronic arthritis supported the hypothesis that the meaning which the child attributes to sensations originating in his joints influences the extent to which those sensations constitute pain. Children in both 6-11 and 12-17 age groups reported similar qualities of sensation from their affected joints, but the older children attributed a more unpleasant meaning to their sensations because of their greater understanding of the significance of internal pathology. By association, the 12-17s consequently reported joint sensations specifically, as more unpleasant and stronger than did the 6-11s.

Published
1983

32. Case conferences-for child abuse

Author

J H Keen

Subjects
Child abuse, medicine.medical_specialty, business.industry, Family medicine, Pediatrics, Perinatology and Child Health, Correspondence, medicine, business
Published
1987

33. Receptor-mediated endocytosis of diphtheria toxin by cells in culture

Author

J. H. Keen, M. C. Hardegree, Frederick R. Maxfield, and W. H. Habig

Subjects
media_common.quotation_subject, Drug Resistance, Receptors, Cell Surface, Biology, Endocytosis, medicine.disease_cause, Mice, Immunotoxin, medicine, Animals, Humans, Diphtheria Toxin, Receptors, Cholinergic, alpha-Macroglobulins, Internalization, Cells, Cultured, media_common, Fluorescent Dyes, Diphtheria toxin, Multidisciplinary, Toxin, Diphtheria, Receptor-mediated endocytosis, medicine.disease, Molecular biology, Cell culture, Intercellular Signaling Peptides and Proteins, Heparin-binding EGF-like Growth Factor, Research Article
Abstract

The binding and uptake of fluorescently labeled diphtheria toxin by cells in culture has been examined by using epifluorescence video intensification microscopy. Rhodamine-labeled diphtheria toxin retained significant toxicity on bioassay and in cell culture and was tested for uptake by human WI-38 and mouse 3T3 fibroblasts grown in culture. When added to cells at 37 degrees C, toxin was observed to become concentrated and internalized in discrete vesicles in both cell lines. The appearance of fluorescent clusters could be prevented by addition of excess unlabeled diphtheria toxin to the medium or by addition of ATP (which has been shown to block toxin binding to cells), indicating that the rhodamine-labeled toxin was binding to diphtheria toxin-specific cell surface binding sites. When the simultaneous uptake of rhodamine-labeled diphtheria toxin and fluorescein-labeled alpha 2-macroglobulin was monitored, the two proteins appeared in the same clusters indicating that the toxin undergoes receptor-mediated endocytosis. Despite the difference in susceptibility to diphtheria toxin of cells derived from sensitive (human) and resistant (mouse) tissues, the behavior of the rhodamine-labeled derivative in both cell lines was indistinguishable in terms of toxin required for formation of clusters or inhibition by unlabeled toxin or by ATP. These results demonstrate that diphtheria toxin-specific cell surface binding sites occur on both insensitive and sensitive cells and suggest that toxin is processed similarly by both cell types during its initial cell surface binding and internalization by this pathway. The possible involvement of this uptake system in the mechanism of action of diphtheria toxin in cells is discussed.

Published
1982

34. The Emory prospective randomized trial: selective versus nonselective shunt to control variceal bleeding. Ten year follow-up

Author

R B Smith rd, W. D. Warren, Atef A. Salam, William J. Millikan, J T Galambos, J H Keen, J. M. Henderson, and Michael Kutner

Subjects
Male, medicine.medical_specialty, Cirrhosis, Population, Esophageal and Gastric Varices, Random Allocation, Liver Function Tests, Occlusion, medicine, Humans, Portasystemic Shunt, Surgical, Prospective Studies, Prospective cohort study, education, education.field_of_study, Clinical Trials as Topic, medicine.diagnostic_test, business.industry, Middle Aged, medicine.disease, Surgery, Anesthesia, Hepatic Encephalopathy, Female, Liver function, business, Liver function tests, Gastrointestinal Hemorrhage, Perfusion, Shunt (electrical), Splenorenal Shunt, Surgical, Liver Circulation, Research Article
Abstract

From 1971 to 1975, 55 patients with variceal bleeding secondary to cirrhosis were entered into a prospective randomized trial comparing distal splenorenal (selective) and H-graft interposition (nonselective) shunt. This 10-year follow-up documents that selective shunt is better (p less than 0.05) in four of the five variables monitored. Control of bleeding: selective shunt prevented variceal bleeding better than interposition shunt due to the higher (0.05 less than p less than 0.1) occlusion rate (30%) of interposition shunt. Selective shunt maintained postoperative portal perfusion better (p less than 0.01) than patent interposition shunt. Seventy-five per cent of selective shunt survivors have portal perfusion at 10 years: no patient with a patent nonselective shunt perfuses the liver. Quantitative liver function was better preserved (p less than 0.01) 10 years after selective shunt than nonselective shunt. Postoperative encephalopathy occurred in fewer (p less than 0.01) selective (27%) than nonselective (75%) shunt patients over the 10 years. Survival: in the randomized population, the improved survival in the selective shunt subgroup did not reach statistical significance. However, improved survival was confirmed in nonalcoholics. Five of eight nonalcoholics operated with selective shunt are alive at 10 years with patent shunts. No nonalcoholic, of seven total, operated with nonselective shunt survived 10 years with a patent shunt. These data show that selective shunt was superior to nonselective shunt. There was less rebleeding and encephalopathy after distal splenorenal shunt; postoperative portal perfusion and hepatic function were maintained.

Published
1985

35. Children with juvenile chronic arthritis: their beliefs about their illness and therapy

Author

J H Keen, V P Mellor, P J Holt, and J G Beales

Subjects
Male, medicine.medical_specialty, Adolescent, Immunology, education, Self-concept, Arthritis, medicine.disease_cause, Fantasy, General Biochemistry, Genetics and Molecular Biology, Rheumatology, medicine, Immunology and Allergy, Psychological stress, Humans, Psychiatry, Child, Clinical treatment, business.industry, Age Factors, Juvenile chronic arthritis, medicine.disease, Self Concept, Arthritis therapy, Female, business, Medical therapy, Attitude to Health, Stress, Psychological, Research Article
Abstract

Seventy-five patients aged 7 to 17 with juvenile chronic arthritis were interviewed to identify their beliefs about the physical nature of their illness and the relevance and modes of action of their clinical treatment. Children in the 7-11 age group were found to perceive their arthritis largely in terms of its immediately manifestations, to have little conception of internal pathology, and to be less aware of the value of their medical therapy. Children in the 12-17 age group showed a greater tendency to recognize arthritis as a condition of internal pathology, to experience distressing fantasies about the internal appearance of their affected joints, and to appreciate the purpose of their therapy.

Published
1983

36. Glutathione transferases. Catalysis of nucleophilic reactions of glutathione

Author

J H, Keen and W B, Jakoby

Subjects
Binding Sites, Liver, Animals, Humans, Glutathione, Glutathione Transferase, Protein Binding, Rats, Substrate Specificity
Abstract

Homogeneous preparations of the glutathione transferases from rat liver have been tested for their ability to catalyze a number of diverse nucleophilic reactions of GSH. Although disulfide interchange with GSSG or L-cystine, and cis-trans isomerization of maleic acid, are clearly promoted by thiols in solution, the reactions were not catalyzed by the glutathione transferases. In contrast, certain more hydrophobic analogs of these compounds were found to serve as substrates. The transferases also catalyze the glutathione-dependent release of p-nitrophenol from p-nitrophenyl acetate and p-nitrophenyl trimethylacetate. These observations are consistent with the formulation that catalysis may result from close juxtaposition of sufficiently electrophilic, nonpolar compounds with GSH on the enzyme surface.

Published
1978

37. Outbreak of Infantile Gastro-enteritis Caused by Escherichia coli O114

Author

B. Wolman, S. I. Jacobs, J. H. Keen, V. Miller, R. J. Gross, Joan Taylor, and A. Holzel

Subjects
medicine.medical_specialty, Pediatrics, Parenteral Nutrition, Vomiting, education, medicine.disease_cause, Gastro enteritis, Disease Outbreaks, medicine, Humans, Escherichia coli, Escherichia coli Infections, business.industry, Colistin, Infant, Newborn, Outbreak, Infant, Articles, Surgery, Gastroenteritis, Parenteral nutrition, England, Liver, Pediatrics, Perinatology and Child Health, Diarrhea, Infantile, Odorants, Carbohydrate Metabolism, Gentamicin, Liver function, medicine.symptom, Gentamicins, business, psychological phenomena and processes, medicine.drug
Abstract

An outbreak of infantile gastro-enteritis occurred at Booth Hall Children9s Hospital as part of a general incident in north-western England, caused by Esch. coli O114K90H2. The organism, which could not be identified with routinely used antisera, caused an unusually prolonged illness after an insidious onset, and was characterized by severe vomiting, together with the passage of very watery stools which became mucuslike and which had a distinctive smell. 29 children were affected and 20 required intravenous feeding for a mean period of 10 days. 7 children died late in the illness, but all were young and debilitated by other acquired or congenital anomalies. Sugar intolerance was prominent, and there was difficulty in returning the children to their routine formulae. Gentamicin and colistin sulphate may have had some effect in reducing the mortality caused by the illness. Liver function abnormality was common, suggesting that Esch. coli O114 might have produced a substance with widespread visceral effects.

Published
1970

38. Beetles From Northern British Columbia

Author

J. H. Keen

Subjects
Geography, Physiology, Structural Biology, Insect Science, Molecular Biology, Ecology, Evolution, Behavior and Systematics
Abstract

About ten years ago (see Can. Ent., Vol. XXXVII, Nos. 7 and 8) I published a list of beetles taken by me on the Queen Charlotte Islands. The beetles enumerated below were, except where otherwise designated, taken on the mainland of British Columbia, on the coast between the mouths of the Naas and Skeena Rivers. Some of them were determined for me through the kindness of Dr. James Fletcher, the Dominion Entomologist, whose valuable help and advice I have now for many years enjoyed; the remaider by Professor H.F. Wickham, of Iowa University, to whose skill and courtesy I am deeply indebted.

Published
1905

40. Sequelae of neonatal convulsions. Study of 112 infants

Author

D Lee and J H Keen

Subjects
Blood Glucose, Pediatrics, medicine.medical_specialty, Intelligence, Hemiplegia, Hypoglycemia, Electroencephalography, Motor Activity, Quadriplegia, Infant, Newborn, Diseases, Recurrence, Seizures, Neonatal convulsions, Medicine, Humans, Meningitis, Motor activity, Hypoxia, Cerebral Hemorrhage, medicine.diagnostic_test, Hypocalcemia, business.industry, Follow up studies, Age Factors, Infant, Newborn, Brain, medicine.disease, Infant newborn, Pediatrics, Perinatology and Child Health, Calcium, business, Follow-Up Studies, Research Article
Published
1973

42. Inflicted burns and scalds in children

Author

B Wolman, J Lendrum, and J H Keen

Subjects
Male, Child abuse, medicine.medical_specialty, Poison control, Suicide prevention, Occupational safety and health, Injury prevention, medicine, Humans, Child Abuse, Buttocks, Child, General Environmental Science, business.industry, General Engineering, Infant, Human factors and ergonomics, General Medicine, Surgery, Perineum, medicine.anatomical_structure, Child, Preschool, Family medicine, Wounds and Injuries, General Earth and Planetary Sciences, Female, Burns, business, Social Welfare, Research Article
Abstract

Ten children who had been burnt and six who had been scalded by parents or those caring for them were seen over three years. In no case did the thermal injury affect more than 5% of the body surface and there were no deaths. In seven the perineum or buttocks were in the burnt area. In 12 children there was evidence of other inflicted injury including six recent fractures. Staff caring for burnt children should be aware of this type of inflicted injury. X-ray skeletal surveys should be carried out in doubtful cases and a case conference initiated with the appropriate social work services to consider supervising the family after the child's discharge or taking legal care proceedings.

Published
1975
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43. ÆGIALITES DEBILIS, MANN

Author

J. H. Keen and B. C. Metlakatla

Subjects
Physiology, Structural Biology, Insect Science, Molecular Biology, Ecology, Evolution, Behavior and Systematics
Abstract

Leconte and Horn, in their “Classification,” say of this beetle: “It is of such extreme rarity as to have been by but few entomologists.” It was with considerable interest, therefore, that I captured my first specimen one March afternoon in 1894. I came upon Æ. debilis on the under side of a stone. From Leconte'e description I felt prety sure that my identification was correct, and it was subsequently confirmed by Dr.Fletcher, or Ottawa. Leconte says the beetle is black, but he had probably seen only dried specimens. Freshly-taken specimens show a distinctly green tinge. The insect is about .15inch long, and in general shape suggests a small carabid.

Published
1903
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44. A NEW CYCHRINID

Author

J. H. Keen

Subjects
Physiology, Structural Biology, Insect Science, Molecular Biology, Ecology, Evolution, Behavior and Systematics
Abstract

This fine plum-coloured beetle–superficially resembling Cychrus marginatus—was taken by me in 1896, and kindly named for me by Captain Casey, whose description of it, published in his Coleopterological Notices, No. VII, page 334, I take the liberty of transcribing below for the benefit of Canadian students who may not see Captain Casey's books. The beetle occurs sparingly, under loose bark or under logs on the gournd, along the mainland of British Columbia from Fort Simpson to Rivers Inlet, and probably farther, if sought for. I have never met with a specimen on the Queen Charlotte Islands.

Published
1898
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46. SOME BRITISH COLUMBIA COLEOPTERA

Author

J. H. Keen

Subjects
Physiology, Structural Biology, Insect Science, Molecular Biology, Ecology, Evolution, Behavior and Systematics
Abstract

Last year (1890) I spent the months of July and August at Inverness—a saimon-canning station at the mouth of the River Skeena, and paid what attention I could spare to the beetles of the locality, a list of which I give below. For the identification of my specimens I am indebted to the courtesy of the British Museum authorities at South Kensington.

Published
1891
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