Your search keyword '"Howard R. Morris"' showing total 367 results

351. Quantitation of luekotrienes C4, D4 amd E4 released by pathophysiological stimuli

Author

John R. Tippins, Howard R. Morris, and B.C. Beaubien

Subjects

medicine.medical_specialty, Leukotriene, biology, Stimulation, Radioimmunoassay, respiratory system, Biochemistry, chemistry.chemical_compound, Lipoxygenase, Endocrinology, Biosynthesis, chemistry, Internal medicine, Parenchyma, Muscarinic acetylcholine receptor, medicine, biology.protein, Cyclooxygenase

Abstract

In order to examine the modulation of leukotriene (LT) release, the PAF-acether-mediated stimulation of these compounds in rat lung was studied. Release of LTC 4 , LTD 4 and LTE 4 in both perfused and chopped lung preparations was measured using HPLC and radioimmunoassay. Pre-incubation or pre-infusion of the tissue with indomethacin and PGE 2 was conducted to investigate the effect of cyclooxygenase inhibitors and products on the lipoxygenase pathway. In addition, the effects of LT levels of pre-incubation with vasoactive intenstinal polypeptide (VIP) in chopped lung were observed. In perfused rat lung, indomethacin reduced the levels of LTC 4 relative to LTD 4 as measured in the first 2 min after stimulation of the lung by PAF-acether. Chopped lung preparations, incubated for 15 min. exhibited higher levels of LTC 4 and LTD 4 in indomethacin-treated samples, this increases being effectively reversed by PGE 2 . In the VIP pre-incubation experiments clear inhibition of peptido -leukotriene synthesis was observed, with no LTC 4 and only low levels of LTD 4 and LTE 4 observed in VIP-incubated samples. In preliminary experiments using rabbit C5a des arg and PAF-acether on rabbit lung parenchyma strips to stimulaet LT release, disodium cromoglycate pre-incubation was observed to inhibit this release. Inhibition of the 5-lipoxygenase pathway of PGE 2 is supported by these experiments. VIP appears to act as an inhibitor of LTC 4 and LTD 4 biosynthesis or release in this model. Too little is known that peptidergic actions to postulate a mechanism by which a neuroendocrine peptide exerts control of release of arachidonate metabolites; however, VIP is associated with muscarinic stimulation (1) and has been found in mast cells (2).

Published

1984

352. PAF-mediated leukotriene biosynthesis in lungs : Control by the neuropeptidergic system

Author

Howard R. Morris, John R. Tippins, and V. Di Marzo

Subjects

Leukotriene biosynthesis, Endocrinology, Biochemistry, Chemistry, Pharmacology

Published

1987

353. Structural modifications of human CGRP and their effect on osteoclastic bone resorption

Author

T.J. Chambers, Howard R. Morris, Mone Zaidi, John R. Tippins, and I. Maclntyre

Subjects

medicine.medical_specialty, Histology, Endocrinology, Physiology, Chemistry, Endocrinology, Diabetes and Metabolism, Internal medicine, Bone cell, medicine, Calcitonin gene-related peptide, Bone resorption

Published

1987

354. Recent advances in organic mass spectrometry in analytical chemistry

Author

J. H. Beynon, Howard R. Morris, K. R. Jennings, James A. Ballantine, and David E. Games

Subjects

Materials science, Computational chemistry, Analytical Chemistry (journal), Mass spectrometry, Analytical Chemistry

Published

1980

355. Mass spectrometry for biochemists

Author

Howard R. Morris

Subjects

Multidisciplinary, Chromatography, Volume (thermodynamics), Chemistry, Mass spectrometry, Mass spectrometry imaging

Abstract

Biochemical Applications of Mass Spectrometry: First Supplementary Volume. Edited by George R. Waller and Otis C. Dermer, Pp. 1,279. (Wiley-Interscience: 1980.) 79.80, 187.50.

Published

1981

356. The plasma-calcium modulating effects of calcitonin gene-related peptide

Author

M. Attinger, I. Maclntyre, Howard R. Morris, M. Azria, C.J. Hillyard, Peter J.R. Bevis, and C. Lynch

Subjects

medicine.medical_specialty, Histology, Endocrinology, Physiology, Plasma calcium, Chemistry, Endocrinology, Diabetes and Metabolism, Internal medicine, medicine, Calcitonin receptor, Calcitonin gene-related peptide

Published

1986

357. β-Cell-tropin: relationship of structure to biological activity

Author

Graham W. Taylor, Howard R. Morris, John Morton, Simon J. Dunmore, and Anne Beloff-Chain

Subjects

medicine.anatomical_structure, Chemistry, Cell, medicine, Biophysics, Biological activity, Biochemistry

Published

1983

358. β-Cell-tropin: characterization as corticotropin-(22–39)-peptide

Author

John Morton, Anne Beloff-Chain, Howard R. Morris, Simon J. Dunmore, and Graham W. Taylor

Subjects

chemistry.chemical_classification, medicine.anatomical_structure, chemistry, Biochemistry, Cell, medicine, Peptide

Published

1983

359. Detection and measurement of CGRP-like substance in man

Author

T. Etienne, I. Maclntyre, John R. Tippins, S. I. Girgis, Maria Panico, and Howard R. Morris

Subjects

medicine.medical_specialty, Histology, Endocrinology, Physiology, Chemistry, Endocrinology, Diabetes and Metabolism, Internal medicine, medicine, Calcitonin gene-related peptide

Published

1985

360. The purification and sequence analysis of rat neuromedin U

Author

Howard R. Morris, S.R. Bloom, L. Thim, V. DiMarzo, Conlon Jm, and Jan Domin

Subjects

Cellular and Molecular Neuroscience, Endocrinology, Physiology, Sequence analysis, Chemistry, Clinical Biochemistry, Biochemistry, Molecular biology, Neuromedin U

Published

1988

361. The identification of a mutant peptide of an abnormal haemoglobin by mass spectrometry

Author

Dudley H. Williams and Howard R. Morris

Subjects

chemistry.chemical_classification, Chromatography, chemistry, Protein mass spectrometry, Biochemistry, Mutant, Abnormal haemoglobin, Molecular Medicine, Peptide, Mass spectrometry

Abstract

A mutant peptide from an abnormal haemoglobin, contaminated by a second peptide, has been sequenced by mass spectrometry; the spectrum of one derivatised mixture allowed the sequences Leu-Leu-Gly-Asn-Val-Leu-Phe and Leu-Leu-Val-Val-Tyr-Pro-Trp to be determined.

Published

1972

362. Towards GAG glycomics: Analysis of highly sulfated heparins by MALDI-TOF mass spectrometry.

Author

Bérangère Tissot, Nijole Gasiunas, Andrew K Powell, Yassir Ahmed, Zheng-liang Zhi, Stuart M Haslam, Howard R Morris, Jeremy E Turnbull, John T Gallagher, and Anne Dell

Subjects

GLYCOMICS, TISSUES, CELLS, IONIZATION (Atomic physics)

Abstract

Glycomics is a developing field that provides structural information on complex populations of glycans isolated from tissues, cells and organs. Strategies employing matrix-assisted laser desorption ionization time-of-flight mass spectrometry (MALDI-TOF MS) are central to glycomic analysis. Current MALDI-based glycomic strategies are capable of efficiently analyzing glycoprotein and glycosphingolipid glycomes but little attention has been paid to devising glycomic methodologies suited to the analysis of glycosaminoglycan (GAG) polysaccharides which pose special problems for MALDI analysis because of their high level of sulfation and large size. In this paper, we describe MALDI strategies that have been optimized for the analysis of highly sulfated GAG-derived oligosaccharides. A crystalline matrix norharmane, as well as an ionic liquid 1-methylimidazolium α-cyano-4-hydroxycinnamate (ImCHCA), have been used for the analysis of heparin di-, tetra-, hexa- and decasaccharides carrying from 2 to 13 sulfate groups. Information about the maximum number of sulfate groups is obtained using the ionic liquid whereas MALDI-TOF/TOF MS/MS experiments using norharmane allowed the determination of the nature of the glycosidic backbone, and more precise information about the presence and the position in the sequence of N-acetylated residues. [ABSTRACT FROM AUTHOR]

Published

2007

363. Integrated mass spectrometric strategy for characterizing the glycans from glycosphingolipids and glycoproteins: direct identification of sialyl Lex in mice.

Author

Simon Parry, Victoria Ledger, Bérangère Tissot, Stuart M. Haslam, James Scott, Howard R. Morris, and Anne Dell

Subjects

MASS spectrometry, GLUCANS, GLYCOSPHINGOLIPIDS, GLYCOPROTEINS

Abstract

The current interest in applying systems biology approaches to studying an organisms form or function promises to reveal further insights into the role of glycosylation in cells and whole organisms. This has prompted the development of a rapid, sensitive method of profiling the glycan component of both glycosphingolipids and glycoproteins from a single sample. Here we report a new mass spectrometric screening strategy for characterizing glycosphingolipid-derived oligosaccharides, which can be integrated into an existing highly sensitive glycoprotein glycomics strategy. Using ceramide glycanase to release the glycans from glycosphingolipids, this method provides a reliable profile of the glycosphingolipid-derived glycans present in a sample and has revealed new glycan structures. Glycoproteins are also efficiently recovered using this method, allowing the subsequent analysis of glycoprotein-derived glycans by mass spectrometry. The high sensitivity of this glycomic screening method allowed us to directly characterize the sialyl Lex epitope from mouse brain for the first time, where it was observed on an O-mannose structure. Thus, we present a mass spectrometric method that allows glycomic screening of N- and O-glycans as well as glycosphingolipid-derived glycans from a single tissue. [ABSTRACT FROM AUTHOR]

Published

2007

364. Analysis of protein-linked glycosylation in a sperm-somatic cell adhesion system.

Author

Mark Sutton-Smith, Nyet Kui Wong, Kay-Hooi Khoo, Sz-Wei Wu, Shin-Yi Yu, Manish S Patankar, Richard Easton, Frank A Lattanzio, Howard R Morris, Anne Dell, and Gary F Clark

Subjects

GLYCOSYLATION, SOMATIC cells, CELL adhesion, SPERM-ovum interactions

Abstract

Murine sperm initiate fertilization by binding to the specialized extracellular matrix of their complementary eggs, known as the zona pellucida. On the basis of data reported in this study, mouse sperm also bind to rabbit erythrocytes with higher affinity than they do to murine eggs. This unusual interaction between a germ cell and a somatic cell (“sperm–somatic cell adhesion system”) is also carbohydrate dependent based on its sensitivity to mild periodate oxidation. To determine what types of carbohydrate sequences could be involved in this interaction, the protein-linked oligosaccharides of rabbit erythrocytes were sequenced using novel matrix-assisted laser desorption/ionization time-of-flight tandem mass spectrometry methods that enabled the analysis of individual components up to m/z 9000. The N-glycans are primarily complex biantennary and triantennary types terminated with Galα1–3Gal sequences. The majority of these oligosaccharides also possess one antenna consisting of a highly branched polylactosamine-type sequence that is also associated with many glycosphingolipids that coat rabbit erythrocytes. These erythrocytes also express Core 1 and Core 2 O-glycans terminated primarily with Galα1–3Gal sequences and to a lesser extent sialic acid. These results confirm that rabbit erythrocytes and mouse eggs present very different types of carbohydrate sequences on their surfaces. However, oligosaccharides terminated with β1–6-linked N-acetyllactosamine or its α1–3 galactosylated analog are expressed on both the mouse zona pellucida and this somatic cell type. The far more abundant presentation of such sequences on rabbit erythrocytes compared with murine eggs could explain why mouse sperm display such exceptional affinity for this somatic cell type. [ABSTRACT FROM AUTHOR]

Published

2007

365. Amino acid sequence of the factor XIII a acceptor site in bovine plasma fibronectin

Author

McDonagh, R.P., McDonagh, Jan, Petersen, Torben E., Thøgersen, Hans C., Skorstengaard, Karna, Sottrup-Jensen, Lars, Magnusson, Staffan, Dell, Anne, and Howard R, Morris

Published

1981

366. Gp120 on HIV-1 Virions Lacks O-Linked Carbohydrate.

Author

Elizabeth Stansell, Maria Panico, Kevin Canis, Poh-Choo Pang, Laura Bouché, Daniel Binet, Michael-John O'Connor, Elena Chertova, Julian Bess, Jeffrey D Lifson, Stuart M Haslam, Howard R Morris, Ronald C Desrosiers, and Anne Dell

Subjects

Medicine, Science

Abstract

As HIV-1-encoded envelope protein traverses the secretory pathway, it may be modified with N- and O-linked carbohydrate. When the gp120s of HIV-1 NL4-3, HIV-1 YU2, HIV-1 Bal, HIV-1 JRFL, and HIV-1 JRCSF were expressed as secreted proteins, the threonine at consensus position 499 was found to be O-glycosylated. For SIVmac239, the corresponding threonine was also glycosylated when gp120 was recombinantly expressed. Similarly-positioned, highly-conserved threonines in the influenza A virus H1N1 HA1 and H5N1 HA1 envelope proteins were also found to carry O-glycans when expressed as secreted proteins. In all cases, the threonines were modified predominantly with disialylated core 1 glycans, together with related core 1 and core 2 structures. Secreted HIV-1 gp140 was modified to a lesser extent with mainly monosialylated core 1 O-glycans, suggesting that the ectodomain of the gp41 transmembrane component may limit the accessibility of Thr499 to glycosyltransferases. In striking contrast to these findings, gp120 on purified virions of HIV-1 Bal and SIV CP-MAC lacked any detectable O-glycosylation of the C-terminal threonine. Our results indicate the absence of O-linked carbohydrates on Thr499 as it exists on the surface of virions and suggest caution in the interpretation of analyses of post-translational modifications that utilize recombinant forms of envelope protein.

Published

2015

367. Transglutaminase-mediated semen coagulation controls sperm storage in the malaria mosquito.

Author

David W Rogers, Francesco Baldini, Francesca Battaglia, Maria Panico, Anne Dell, Howard R Morris, and Flaminia Catteruccia

Subjects

Biology (General), QH301-705.5

Abstract

Insect seminal fluid proteins are powerful modulators of many aspects of female physiology and behaviour including longevity, egg production, sperm storage, and remating. The crucial role of these proteins in reproduction makes them promising targets for developing tools aimed at reducing the population sizes of vectors of disease. In the malaria mosquito Anopheles gambiae, seminal secretions produced by the male accessory glands (MAGs) are transferred to females in the form of a coagulated mass called the mating plug. The potential of seminal fluid proteins as tools for mosquito control demands that we improve our limited understanding of the composition and function of the plug. Here, we show that the plug is a key determinant of An. gambiae reproductive success. We uncover the composition of the plug and demonstrate it is formed through the cross-linking of seminal proteins mediated by a MAG-specific transglutaminase (TGase), a mechanism remarkably similar to mammalian semen coagulation. Interfering with TGase expression in males inhibits plug formation and transfer, and prevents females from storing sperm with obvious consequences for fertility. Moreover, we show that the MAG-specific TGase is restricted to the anopheline lineage, where it functions to promote sperm storage rather than as a mechanical barrier to re-insemination. Taken together, these data represent a major advance in our understanding of the factors shaping Anopheles reproductive biology.

Published

2009