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2. Far Ultraviolet Spectroscopic Explorer Spectroscopy of Absorption and Emission Lines from the Narrow-Line Seyfert 1 Galaxy NGC 4051

Author

Kaspi, Shai, Brandt, W. N., Collinge, M. J., Elvis, Martin, and Reynolds, Christopher S.

Subjects
Astrophysics
Abstract

We present three Far Ultraviolet Spectroscopic Explorer (FUSE) observations of the Narrow-Line Seyfert 1 galaxy NGC4051. The most prominent features in the far-ultraviolet (FUV) spectrum are the OVI emission and absorption lines and the HI Lyman series absorption lines which are detected up to the Lyman edge. We also identify weak emission from NIII, CIII, and HeII. The CIII line shows absorption while none is detected in the NIII and HeII lines. In HI and CIII we detect two main absorption systems at outflow velocities of -50+/-30 and -240+/-40 km/s, as well as a possible third one at ~ -450 km/s. These systems are consistent in velocity with the 10 absorption systems found previously in CIV, NV, and SiIV, though the individual systems are blended together in the FUV spectrum. We estimate column densities of the two main absorption systems and find that the HI column density is lower for systems with larger outflow velocity. We detect no flux or spectral variations of NGC4051 at FUV wavelengths during three epochs spanning one year. This is consistent with the optical light curve which shows no variations between the three epochs. It is also consistent with the X-ray light curve which shows consistent flux levels at the three epochs of the FUSE observations, although the X-ray light curve shows strong variations on much shorter timescales., Comment: 9 pages, 7 figures (5 in color), emulateapj, accepted for publication in The Astronomical Journal

Published
2004
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3. Candidate Type II Quasars from the Sloan Digital Sky Survey: I. Selection and Optical Properties of a Sample at 0.3<Z<0.83

Author

Zakamska, Nadia L., Strauss, Michael A., Krolik, Julian H., Collinge, M. J., Hall, P. B., Hao, L., Heckman, T. M., Ivezic, Z., Richards, G. T., Schlegel, D. J., Schneider, D. P., Strateva, I., Berk, D. E. Vanden, Anderson, S. F., and Brinkmann, J.

Subjects
Astrophysics
Abstract

Type II quasars are the long-sought luminous analogs of type II (narrow emission line) Seyfert galaxies, suggested by unification models of active galactic nuclei (AGN) and postulated to account for an appreciable fraction of the cosmic hard X-ray background. We present a sample of 291 type II AGN at redshifts 0.3

Published
2003
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4. An Initial Survey of White Dwarfs in the Sloan Digital Sky Survey

Author

Harris, H. C., Liebert, J., Kleinman, S. J., Nitta, A., Anderson, S. F., Knapp, G. R., Krzesinski, J., Schmidt, G., Strauss, M. A., Berk, D. Vanden, Eisenstein, D., Hawley, S., Margon, B., Munn, J. A., Silvestri, N. M., Smith, A., Szkody, P., Collinge, M. J., Dahn, C. C., Fan, X., Hall, P. B., Schneider, D. P., Brinkmann, J., Burles, S., Gunn, J. E., Hennessy, G. S., Hindsley, R., Ivezic, Z., Kent, S., Lamb, D. Q., Lupton, R. H., Nichol, R. C., Pier, J. R., Schlegel, D. J., SubbaRao, M., Uomoto, A., Yanny, B., and York, D. G.

Subjects
Astrophysics
Abstract

An initial assessment is made of white dwarf and hot subdwarf stars observed in the Sloan Digital Sky Survey. In a small area of sky (190 square degrees), observed much like the full survey will be, 269 white dwarfs and 56 hot subdwarfs are identified spectroscopically where only 44 white dwarfs and 5 hot subdwarfs were known previously. Most are ordinary DA (hydrogen atmosphere) and DB (helium) types. In addition, in the full survey to date, a number of WDs have been found with uncommon spectral types. Among these are blue DQ stars displaying lines of atomic carbon; red DQ stars showing molecular bands of C_2 with a wide variety of strengths; DZ stars where Ca and occasionally Mg, Na, and/or Fe lines are detected; and magnetic WDs with a wide range of magnetic field strengths in DA, DB, DQ, and (probably) DZ spectral types. Photometry alone allows identification of stars hotter than 12000 K, and the density of these stars for 15

Published
2003
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5. High-Resolution X-ray and Ultraviolet Spectroscopy of the Complex Intrinsic Absorption in NGC 4051 with Chandra and HST

Author

Collinge, M. J., Brandt, W. N., Kaspi, Shai, Crenshaw, D. Michael, Elvis, Martin, Kraemer, Steven B., Reynolds, Christopher S., Sambruna, Rita M., and Wills, Beverley J.

Subjects
Astrophysics
Abstract

We present the results from simultaneous observations of the Narrow-Line Seyfert 1 galaxy NGC 4051 with the Chandra High Energy Transmission Grating Spectrometer and the HST Space Telescope Imaging Spectrograph. The X-ray grating spectrum reveals absorption and emission lines from hydrogen-like and helium-like ions of O, Ne, Mg and Si. We resolve two distinct X-ray absorption systems: a high-velocity blueshifted system at -2340+/-130 km/s and a low-velocity blueshifted system at -600+/-130 km/s. In the UV spectrum we detect strong absorption, mainly from C IV, N V and Si IV, that is resolved into as many as nine different intrinsic absorption systems with velocities between -650 km/s and 30 km/s. Although the low-velocity X-ray absorption is consistent in velocity with many of the UV absorption systems, the high-velocity X-ray absorption seems to have no UV counterpart. In addition to the absorption and emission lines, we also observe rapid X-ray variability and a state of low X-ray flux during the last ~15 ks of the observation. NGC 4051 has a soft X-ray excess which we fit in both the high and low X-ray flux states. The high-resolution X-ray spectrum directly reveals that the soft excess is not composed of narrow emission lines and that it has significant spectral curvature. A power-law model fails to fit it, while a blackbody produces a nearly acceptable fit. We compare the observed spectral variability with the results of previous studies of NGC 4051., Comment: 16 pages, 13 figures included, LaTeX emulateapj5.sty, accepted for publication in The Astrophysical Journal (this version is the same as the first version)

Published
2001
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6. Compton-Thick X-ray Absorption in the Seyfert Galaxies Tololo 0109-383 and ESO 138-G1

Author

Collinge, M. J. and Brandt, W. N.

Subjects
Astrophysics
Abstract

We present analyses of the ASCA X-ray spectra of two Seyfert galaxies, Tololo 0109-383 and ESO 138-G1. In both cases, spectral fitting reveals two statistically acceptable continuum models: Compton reflection and partial covering. Both spectra have strong iron K-alpha lines, with equivalent widths greater than 1.5 keV. These large equivalent widths are suggestive of heavier obscuration than that directly indicated by the partial-covering models (approximately 2 x 10^23 cm^-2), with the actual column densities being `Compton-thick' (i.e. N_H > 1.5 x 10^24 cm^-2). We use the hard X-ray/[O III] flux correlation for Seyferts and data from the literature to provide additional support for this hypothesis. Since Tololo 0109-383 is known to have optical type 1 characteristics such as broad Balmer line components and Fe II emission, this result marks it as a notable object., Comment: 5 pages, 5 figures, accepted for publication in MNRAS, replaced to improve formatting

Published
2000
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7. The relationship between childhood abuse and delusions : an investigation based on delusional content

Author

Collinge, M. R.

Subjects
362.76
Abstract

Psychotic illness is associated in the literature with abuse in childhood (Read, van Os, Morrison, & Ross, 2005). This literature is reviewed, focussing on the relationship between childhood abuse and delusions. The review looks to the abuse literature to suggest ways that psychological sequelae of abuse might fit with existing theories of delusions to offer a more comprehensive understanding of their origins. It is argued that current psychological models of delusions do not deal adequately with the impact of childhood abuse. A greater appreciation of this relationship is theoretically important, but also has crucial implications for the accuracy of formulations and the appropriateness of treatment.

Published
2006

8. Cell-Mediated Immunity

Author

Kamperschroer, C., primary, Collinge, M., additional, Heyen, J.R., additional, Ji, C., additional, O’Donnell, L.M., additional, and Zhu, X., additional

Published
2018
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11. Història del retorn a les aules de primer cicle d’infantil: l’acompanyament des de l’Administració educativa

Author

Collinge, M. Magdalena, Font, Guillermo, Gual, Mateu, Mas, Rosa, Pascual, Arnau F., Rodríguez, Miguel, and Torrandell, Victòria

Subjects
Pandemic, Education
Abstract

[cat] Aquest article pretén fer memòria del procés d’acompanyament que des de l’Administració educativa s’ha fet als centres educatius de primer cicle d’educació infantil, de les xarxes pública i complementària, per a la seva obertura després del confinament establert per l’estat d’alarma i el seu posterior funcionament cohabitant amb les diferents situacions derivades de la pandèmia de la COVID-19. En aquest sentit, està escrit en termes cronològics per procurar al lector els contextos normatius i sanitaris de cada fase de la desescalada i fer entenedores les circumstàncies viscudes pels centres en cada moment., [spa] Este artículo pretende recordar el proceso de acompañamiento llevado a cabo desde la Administración educativa a los centros de primer ciclo de educación infantil, de las redes pública y complementaria, de cara a la apertura después del confinamiento establecido por el estado de alarma y su posterior funcionamiento conviviendo con las diferentes consecuencias de la pandemia de la COVID-19. En este sentido, está escrito en términos cronológicos para procurar al lector los contextos normativos y sanitarios de cada fase de la desescalada y hacer comprensibles las circunstancias vividas por los centros en cada momento.

Published
2021

16. Macrophage β(2) Integrin-Mediated, HuR-Dependent Stabilization of Angiogenic Factor-Encoding mRNAs in Inflammatory Angiogenesis

Author

Zhang J, Modi Y, Yarovinsky T, Yu J, Collinge M, Kyriakides T, Zhu Y, Sessa WC, Bender J.R., PARDI , RUGGERO, Zhang, J, Modi, Y, Yarovinsky, T, Yu, J, Collinge, M, Kyriakides, T, Zhu, Y, Sessa, Wc, Pardi, Ruggero, and Bender, J. R.

Abstract

HuR is a member of the Drosophila Elav protein family that binds mRNA degradation sequences and prevents RNase-mediated degradation. Such HuR-mediated mRNA stabilization, which is stimulated by integrin engagement and is controlled at the level of HuR nuclear export, is critically involved in T-cell cytokine production. However, HuR's role in macrophage soluble factor production, in particular in response to angiogenic stimuli, has not yet been established. We show that the labile transcripts that encode vascular endothelial growth factor and matrix metalloproteinase-9 are stabilized when murine macrophages adhere to the β(2) integrin ligand intercellular adhesion molecule-1. This mRNA stabilization response was absent in bone marrow-derived macrophages obtained from conditional macrophage-specific HuR knockout mice. The microvascular angiogenic response to an inflammatory stimulus (ie, subcutaneous polyvinyl alcohol sponge implantation) was markedly diminished in these macrophage HuR knockout mice despite the equal levels of macrophage localization to those observed in littermate wild-type controls. Furthermore, blood flow recovery and ischemic muscle neovascularization after femoral artery ligation were impaired in the conditional macrophage-specific HuR knockout mice. These results demonstrate that the dynamic effects on mRNA that are mediated by the RNA-binding and RNA-stabilizing protein HuR are required for macrophage production of angiogenic factors, which play critical roles in the neovascular responses to a variety of stimuli, including tissue ischemia.

Published
2012

17. T cell LFA-1 engagement induces HuR-dependent cytokine mRNA stabilization through a Vav-1, Rac1/2, p38MAPK and MKK3 signaling cascade

Author

RAMGOLAM VS, DEGREGORIO SD, RAO GK, COLLINGE M, SUBARAN SS, MARKOVIC PLESE S, BENDER J.R., PARDI , RUGGERO, Ramgolam, V, Degregorio, Sd, Rao, Gk, Collinge, M, Subaran, S, MARKOVIC PLESE, S, Pardi, Ruggero, and Bender, J. R.

Abstract

BACKGROUND: Engagement of the β2 integrin, lymphocyte function-associated antigen-1 (LFA-1), results in stabilization of T cell mRNA transcripts containing AU-rich elements (AREs) by inducing rapid nuclear-to-cytosolic translocation of the RNA-stabilizing protein, HuR. However, little is known regarding integrin-induced signaling cascades that affect mRNA catabolism. This study examines the role of the GTPases, Rac 1 and Rac 2, and their downstream effectors, in the LFA-1-induced effects on mRNA. METHODOLOGY/PRINCIPAL FINDINGS: Engagement of LFA-1 to its ligand, ICAM-1, in human peripheral T cells resulted in rapid activation of Rac1 and Rac2. siRNA-mediated knockdown of either Rac1 or Rac2 prevented LFA-1-stimulated stabilization of the labile transcripts encoding IFN-γ and TNF-α, and integrin mediated IFN-γ mRNA stabilization was absent in T cells obtained from Rac2 gene-deleted mice. LFA-1 engagement-induced translocation of HuR and stabilization of TNF- α mRNA was lost in Jurkat cells deficient in the Rac guanine nucleotide exchange factor Vav-1 (J.Vav1). The transfection of J.Vav1 cells with constitutively active Rac1 or Rac2 stabilized a labile β-globin reporter mRNA, in a HuR-dependent manner. Furthermore, LFA-1-mediated mRNA stabilization and HuR translocation in mouse splenic T cells was dependent on the phosphorylation of the mitogen-activated protein kinase kinase, MKK3, and its target MAP kinase p38MAPK, and lost in T cells obtained from MKK3 gene-deleted mice. CONCLUSIONS/SIGNIFICANCE: Collectively, these results demonstrate that LFA-1-induced stabilization of ARE-containing mRNAs in T cells is dependent on HuR, and occurs through the Vav-1, Rac1/2, MKK3 and p38MAPK signaling cascade. This pathway constitutes a molecular switch that enhances immune and pro-inflammatory gene expression in T cells undergoing adhesion at sites of activation and effector function.

Published
2010

18. LFA-1-Dependent HuR Nuclear Export and Cytokine mRNA Stabilization in T Cell Activation

Author

WANG JG, COLLINGE M, RAMGOLAM V, AYALON O, FAN XC, BENDER JR, PARDI , RUGGERO, Wang, Jg, Collinge, M, Ramgolam, V, Ayalon, O, Fan, Xc, Pardi, Ruggero, and Bender, Jr

Abstract

Lymphokine gene expression is a precisely regulated process in T cell-mediated immune responses. In this study we demonstrate that engagement of the beta(2) integrin LFA-1 in human peripheral T cells markedly extends the half-life of TNF-alpha, GM-CSF, and IL-3 mRNA, as well as a chimeric beta-globin mRNA reporter construct containing a strongly destabilizing class II AU-rich element from the GM-CSF mRNA 3'-untranslated region. This integrin-enhanced mRNA stability leads to augmented protein production, as determined by TNF-alpha ELISPOT assays. Furthermore, T cell stimulation by LFA-1 promotes rapid nuclear-to-cytoplasmic translocation of the mRNA-stabilizing protein HuR, which in turn is capable of binding an AU-rich element sequence in vitro. Abrogation of HuR function by use of inhibitory peptides, or marked reduction of HuR levels by RNA interference, prevents LFA-1 engagement-mediated stabilization of T cell TNF-alpha or IFN-gamma transcripts, respectively. Thus, HuR-mediated mRNA stabilization, stimulated by integrin engagement and controlled at the level of HuR nuclear export, is critically involved in T cell activation.

Published
2006

32. The Location of Calmodulin in the Pea Plasma Membrane

Author

Collinge, M and Trewavas, A J

Abstract

Plasma membrane has been prepared from pea seedlings in the presence of [ethylenebis(oxyethylenenitrilo)]tetraacetic acid (EGTA). Calmodulin has been detected in these plasma membrane preparations using calcium overlay techniques, immunoblots, quantitation with antibodies raised against spinach calmodulin, phosphodiesterase activation, mobility shift, and heat stability. EGTA-stable calmodulin represents 0.5–1% of the total plasma membrane protein, and it is the only detectable calcium-binding protein in plasma membrane isolated under these conditions. The anti-spinach calmodulin reacts only with the N-terminal region of spinach calmodulin representing residues 1–106. The positioning of EGTA-stable calmodulin in the plasma membrane has been probed with trypsin and anti-spinach calmodulin. The data suggest that the calmodulin N-terminal region representing residues 1–106 projects from the membrane and could be available for binding other proteins.

Published
1989
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33. Dynamics of Benzophenanthridine Alkaloid Production in Suspension Cultures of Eschscholtzia californica after Treatment with a Yeast Elicitor

Author

Collinge, M A, Brodelius, Peter, Collinge, M A, and Brodelius, Peter

Abstract

A number of benzophenanthridine alkaloids are induced in suspension cultures of Eschscholtzia californica after treatment with an elicitor prepared from yeast extract. The formation of the alkaloids sanguinarine, chelerythrine and macarpine has been studied in relation to; elicitor concentration, incubation time after elicitation, and culture age. A significant portion of these alkaloids is released into the medium. Sanguinarine and chelerythrine reach maximum levels a few hours after the time of elicitation. Thereafter, their levels decline and the amount of macarpine increases. Viability of elicited cells, as determined by their subsequent growth, is not significantly reduced. There is a good correlation between induced tyrosine decarboxylase activity and alkaloid formation.

Published
1989
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36. T cell LFA-1-induced proinflammatory mRNA stabilization is mediated by the p38 pathway kinase MK2 in a process regulated by hnRNPs C, H1 and K

Author

Matthias Gaestel, Ruggero Pardi, Joseph Sarhan, Jeffrey R. Bender, Vinod S. Ramgolam, Timur O. Yarovinsky, Mark Collinge, Albert J. Wong, Gautham K. Rao, Rao, G. K., Wong, A., Collinge, M., Sarhan, J., Yarovinsky, T. O., Ramgolam, V. S., Gaestel, M., Pardi, R., and Bender, J. R.

Subjects
0301 basic medicine, Integrins, Cytoplasm, Proteome, Physiology, Molecular biology, RNA Stability, T-Lymphocytes, Cell Culture Techniques, lcsh:Medicine, Protein-Serine-Threonine Kinase, Biochemistry, Heterogeneous-Nuclear Ribonucleoproteins, ELAV-Like Protein 1, White Blood Cells, Jurkat Cells, Animal Cells, Immune Physiology, Medicine and Health Sciences, Small interfering RNAs, Nuclear protein, lcsh:Science, Mice, Knockout, Innate Immune System, Multidisciplinary, T Cells, Kinase, Chemistry, Messenger RNA, Intracellular Signaling Peptides and Proteins, MRNA stabilization, Lymphocyte Function-Associated Antigen-1, Extracellular Matrix, Precipitation Techniques, Cell biology, Nucleic acids, RNA isolation, medicine.anatomical_structure, Cytokines, Cellular Types, Cellular Structures and Organelles, Cell Culture Technique, Human, Research Article, Signal Transduction, HNRNPC, Immune Cells, T cell, Immunology, Jurkat Cell, Protein Serine-Threonine Kinases, Biomolecular isolation, Proinflammatory cytokine, 03 medical and health sciences, Genetics, Cell Adhesion, medicine, Immunoprecipitation, Animals, Humans, RNA, Messenger, Non-coding RNA, Blood Cells, Animal, Activator (genetics), lcsh:R, Biology and Life Sciences, Cell Biology, Molecular Development, Gene regulation, Research and analysis methods, Mice, Inbred C57BL, Molecular biology techniques, 030104 developmental biology, Intracellular Signaling Peptides and Protein, Immune System, Heterogeneous-Nuclear Ribonucleoprotein, RNA, lcsh:Q, Gene expression, Developmental Biology
Abstract

Activation of the β2 integrin lymphocyte function-associated antigen-1 (LFA-1) in T cells induces stabilization of proinflammatory AU-rich element (ARE)-bearing mRNAs, by triggering the nuclear-to-cytoplasmic translocation of the mRNA-binding and -stabilizing protein HuR. However, the mechanism by which LFA-1 engagement controls HuR localization is not known. Here, we identify and characterize four key regulators of LFA-1-induced changes in HuR activity: the p38 pathway kinase MK2 and the constitutive nuclear proteins hnRNPs C, H1 and K. LFA-1 engagement results in rapid, sequential activation of p38 and MK2. Post-LFA-1 activation, MK2 inducibly associates with both hnRNPC and HuR, resulting in the dissociation of HuR from hnRNPs C, H1 and K. Freed from the three hnRNPs, HuR translocates from the nucleus to the cytoplasm, and mediates the stabilization of labile cytokine transcripts. Our results suggest that the modulation of T cell cytokine mRNA half-life is an intricate process that is negatively regulated by hnRNPs C, H1 and K and requires MK2 as a critical activator.

Published
2018
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37. The poly(ADP-ribose)-protein shuttle of chromatin

Author

M. C. Richard, Maria Malanga, C. Realini, Margaret A. Collinge, S. Bachmann, Phyllis L. Panzeter, B. Zweifel, S. H. Waser, Felix R. Althaus, Liane Höfferer, S. A. Braun, Althaus, F. R., Bachmann, S, Braun, S. A., Collinge, M. A., Hfferer, L, Malanga, Maria, Panzeter, P. L., Realini, C, Richard, M. C., Waser, S, and Zweifel, B.

Subjects
chemistry.chemical_compound, Histone, biology, Polynucleotide, Chemistry, biology.protein, Nucleosome, Binding site, Nuclear protein, DNA, Cell biology, Chromatin, Micrococcal nuclease
Abstract

Since the discovery of poly(ADP-ribose) in Paul Mandel’s laboratory in 196E (1), poly ADP-ribosylation has been classified as a posttranslational protein modification (for review see 2-4), While this definition is formally correct, it may not precisely reflect the primary function of poly(ADP-ribose). The term “posttranslational modification” projects the idea that the modifying residue modifies protein function by covalent modification of the target acceptor. Over the past five years, we have focussed on the possibility that ADP-ribose polymers may primarily act on protein function(s) by non-covalent interactions with nuclear proteins. The working hypothesis envisions poly(ADP-ribose) metabolism as a protein shuttle mechanism in chromatin. The results show that poly ADP-ribosylation may selectively regulate DNA template accessibility for proteins involved in DNA processing functions. In this mechanism, poly(ADP-ribose) assumes the function of an alternative polynucleotide binding site for histones in chromatin. Testing this concept in models of various complexities, we conclude that protein shuttling by poly ADP-ribosylation may be involved in local unfolding of nucleosomes during DNA excision repair (5,6).

Published
1992

38. mRNA-LNPs induce immune activation and cytokine release in human whole blood assays across diverse health conditions.

Author

Nguyen HM, Alexander KE, Collinge M, Hickey JC, Lanz TA, Li J, Sheehan MJ, Newman LC, and Thorn M

Abstract

RNA medicines have become a promising platform for therapeutic use in recent years. Understanding the immunomodulatory effects of novel mRNA-LNPs is crucial for future therapeutic development. An in vitro whole blood assay was developed to assess the impact of mRNA-LNPs on immune cell function, cytokine release, and complement activation. mRNA-LNPs significantly increased CD69 expression on T cells and natural killer (NK) cells, and CD80/CD86 on myeloid subsets, in a dose-dependent fashion. Furthermore, mRNA-LNPs elicited a robust release of pro-inflammatory cytokines, including TNF-α, IL-1β, MCP-1, IL-6, and IP-10, indicating a potent immune response. Notably, mRNA-LNPs stimulate early cytokine production prior to triggering immune cell activation, suggesting a temporal and biological relationship. Moreover, mRNA-LNPs induce complement activation via the alternative pathway, as evidenced by increased serum sC5b-9, C3a, and Bb which can amplify the inflammatory response and potentially impact safety. In vitro effects of mRNA-LNPs in whole blood of healthy human donors were compared to those from disease cohorts including systemic lupus erythematosus (SLE), type 2 diabetes mellitus (T2DM), and cancer donors. The differences in mRNA-LNPs effects on samples from healthy and diseased populations may impact therapeutic efficacy or toxicity, indicating a need for tailoring LNPs for specific target populations., (Copyright © 2024 The Author(s). Published by Elsevier Inc. All rights reserved.)

Published
2024
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39. Relationship between lymphocyte count and risk of infection in Japanese rheumatoid arthritis patients treated with tofacitinib.

Author

Tanaka Y, Takeuchi T, Valdez H, Collinge M, Zwillich SH, Toyoizumi S, Kwok K, and Hirose T

Subjects
Humans, Male, Female, Middle Aged, Lymphocyte Count, Aged, Japan epidemiology, Pyrroles therapeutic use, Pyrroles adverse effects, Adult, Antirheumatic Agents therapeutic use, Antirheumatic Agents adverse effects, Incidence, Infections epidemiology, Protein Kinase Inhibitors therapeutic use, Protein Kinase Inhibitors adverse effects, East Asian People, Arthritis, Rheumatoid drug therapy, Piperidines therapeutic use, Piperidines adverse effects, Pyrimidines therapeutic use, Herpes Zoster epidemiology, Herpes Zoster immunology
Abstract

Objectives: We characterised changes in absolute lymphocyte counts (ALCs) and lymphocyte subset counts (LSCs), and their relationship to incidence of serious infection events (SIEs) and herpes zoster (HZ) events in Japanese patients with moderate to severe rheumatoid arthritis enrolled in the tofacitinib clinical programme., Methods: Data included 765 patients receiving tofacitinib in Phase 2, Phase 3, and long-term extension studies. ALCs/LSCs and incidence rates (patients with events/100 patient-years) of SIEs and HZ were analysed over 75 months., Results: Median ALCs were generally stable over 75 months of treatment. Transient numerical increases from baseline in median LSCs were observed at Month 3; LSCs were generally lower than baseline for Months 36-75. SIE/HZ incidence rates were higher in patients with ALC <0.5 × 103 cells/mm3 versus those with ALC ≥0.5 × 103 cells/mm3 during tofacitinib treatment. Baseline LSCs were similar in patients with/without SIEs or HZ events., Conclusions: SIE/HZ risk was highest in patients with ALC <0.5 × 103 cells/mm3, supporting this threshold as clinically relevant for defining increased SIE/HZ risk in Japanese patients with rheumatoid arthritis receiving tofacitinib. However, SIEs and HZ events did not necessarily occur simultaneously with confirmed lymphopenia, preventing conclusions on possible causal relationships being drawn., (© Japan College of Rheumatology 2024. Published by Oxford University Press.)

Published
2024
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40. Challenges and gaps in immunosafety evaluation of therapeutics: An IQ DruSafe survey.

Author

Collinge M, Neff-LaFord H, Akella S, Fogal B, Fraser K, Jabbour J, Harper K, Maier CC, Malherbe L, Marshall N, Rao GK, Raman K, Skaggs H, Weber F, and Fuller CL

Subjects
Humans, Animals, Surveys and Questionnaires, Cytokines immunology, Risk Assessment, Drug Evaluation, Preclinical methods, Toxicity Tests methods, Immunologic Factors adverse effects, Immunologic Factors toxicity
Abstract

Immunotoxicology/immunosafety science is rapidly evolving, with novel modalities and immuno-oncology among the primary drivers of new tools and technologies. The Immunosafety Working Group of IQ/DruSafe sought to better understand some of the key challenges in immunosafety evaluation, gaps in the science, and current limitations in methods and data interpretation. A survey was developed to provide a baseline understanding of the needs and challenges faced in immunosafety assessments, the tools currently being applied across the industry, and the impact of feedback received from regulatory agencies. This survey also focused on current practices and challenges in conducting the T-cell-dependent antibody response (TDAR) and the cytokine release assay (CRA). Respondents indicated that ICH S8 guidance was insufficient for the current needs of the industry portfolio of immunomodulators and novel modalities and should be updated. Other challenges/gaps identified included translation of nonclinical immunosafety assessments to the clinic, and lack of relevant nonclinical species and models in some cases. Key areas of emerging science that will add future value to immunotoxicity assessments include development of additional in vitro and microphysiological system models, as well as application of humanized mouse models. Efforts are ongoing in individual companies and consortia to address some of these gaps and emerging science., Competing Interests: Declaration of competing interest The authors declare that they have no known competing financial interests or personal relationships that could have appeared to influence the work reported in this paper., (Copyright © 2024 Elsevier Inc. All rights reserved.)

Published
2024
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41. Current approaches to evaluate the function of cytotoxic T-cells in non-human primates.

Author

Kamperschroer C, Frank B, Genell C, Lebrec H, Mitchell-Ryan S, Molinier B, Newsome C, Piche MS, Weinstock D, Collinge M, Freebern W, and Rubio D

Subjects
Animals, Primates, Cytotoxicity, Immunologic, T-Lymphocytes, Cytotoxic, Neoplasms therapy
Abstract

Cytotoxic T-lymphocytes (CTL) are a subset of T-cells that play a critical role in protecting against intracellular infections and cancer, and have the ability to identify and kill infected or transformed cells expressing non-self peptides associated with major histocompatibility (MHC) Class I molecules. Conversely, aberrant CTL activity can contribute to immune-related pathology under conditions of overwhelming infection or autoimmunity. Disease-modifying therapeutics can have unintended effects on CTL, and a growing number of therapeutics are intended to either suppress or enhance CTL or their functions. The susceptibility of CTL to unintended effects from common therapeutic modalities underscores the need for a better understanding of the impact that such therapies have on CTL function and the associated safety implications. While there are reliable ways of quantifying CTL, notably via flow cytometric analysis of specific CTL markers, it has been a greater challenge to implement fit-for-purpose methods measuring CTL function in the context of safety studies of therapeutics. This review focuses on methods for measuring CTL responses in the context of drug safety and pharmacology testing, with the goals of informing the reader about current approaches, evaluating their pros and cons, and providing perspectives on the utility of these approaches for safety evaluation.

Published
2023
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42. A Novel C-C Chemoattractant Cytokine (Chemokine) Receptor 6 (CCR6) Antagonist (PF-07054894) Distinguishes between Homologous Chemokine Receptors, Increases Basal Circulating CCR6 + T Cells, and Ameliorates Interleukin-23-Induced Skin Inflammation.

Author

Li W, Crouse KK, Alley J, Frisbie RK, Fish SC, Andreyeva TA, Reed LA, Thorn M, DiMaggio G, Donovan CB, Bennett D, Garren J, Oziolor E, Qian J, Newman L, Vargas AP, Kumpf SW, Steyn SJ, Schnute ME, Thorarensen A, Hegen M, Stevens E, Collinge M, Lanz TA, Vincent F, Vincent MS, and Berstein G

Subjects
Humans, Animals, Mice, Receptors, CCR7, Ligands, T-Lymphocytes, Inflammation, Receptors, CCR6, Chemokines, CC genetics, Interleukin-23
Abstract

Blocking chemokine receptor C-C chemoattractant cytokine (chemokine) receptor (CCR) 6-dependent T cell migration has therapeutic promise in inflammatory diseases. PF-07054894 is a novel CCR6 antagonist that blocked only CCR6, CCR7, and C-X-C chemoattractant cytokine (chemokine) receptor (CXCR) 2 in a β -arrestin assay panel of 168 G protein-coupled receptors. Inhibition of CCR6-mediated human T cell chemotaxis by (R)-4-((2-(((1,4-Dimethyl-1H-pyrazol-3-yl)(1-methylcyclopentyl)methyl)amino)-3,4-dioxocyclobut-1-en-1-yl)amino)-3-hydroxy-N,N-dimethylpicolinamide (PF-07054894) was insurmountable by CCR6 ligand, C-C motif ligand (CCL) 20. In contrast, blockade of CCR7-dependent chemotaxis in human T cells and CXCR2-dependent chemotaxis in human neutrophils by PF-07054894 were surmountable by CCL19 and C-X-C motif ligand 1, respectively. [ 3 H]-PF-07054894 showed a slower dissociation rate for CCR6 than for CCR7 and CXCR2 suggesting that differences in chemotaxis patterns of inhibition could be attributable to offset kinetics. Consistent with this notion, an analog of PF-07054894 with fast dissociation rate showed surmountable inhibition of CCL20/CCR6 chemotaxis. Furthermore, pre-equilibration of T cells with PF-07054894 increased its inhibitory potency in CCL20/CCR6 chemotaxis by 10-fold. The functional selectivity of PF-07054894 for inhibition of CCR6 relative to CCR7 and CXCR2 is estimated to be at least 50- and 150-fold, respectively. When administered orally to naïve cynomolgus monkeys, PF-07054894 increased the frequency of CCR6 + peripheral blood T cells, suggesting that blockade of CCR6 inhibited homeostatic migration of T cells from blood to tissues. PF-07054894 inhibited interleukin-23-induced mouse skin ear swelling to a similar extent as genetic ablation of CCR6. PF-07054894 caused an increase in cell surface CCR6 in mouse and monkey B cells, which was recapitulated in mouse splenocytes in vitro. In conclusion, PF-07054894 is a potent and functionally selective CCR6 antagonist that blocks CCR6-mediated chemotaxis in vitro and in vivo. SIGNIFICANCE STATEMENT: The chemokine receptor, C-C chemoattractant cytokine (chemokine) receptor 6 (CCR6) plays a key role in the migration of pathogenic lymphocytes and dendritic cells into sites of inflammation. (R)-4-((2-(((1,4-Dimethyl-1H-pyrazol-3-yl)(1-methylcyclopentyl)methyl)amino)-3,4-dioxocyclobut-1-en-1-yl)amino)-3-hydroxy-N,N-dimethylpicolinamide (PF-07054894) is a novel CCR6 small molecule antagonist that illustrates the importance of binding kinetics in achieving pharmacological potency and selectivity. Orally administered PF-07054894 blocks homeostatic and pathogenic functions of CCR6, suggesting that it is a promising therapeutic agent for the treatment of a variety of autoimmune and inflammatory diseases., (Copyright © 2023 by The Author(s).)

Published
2023
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43. Application of Immunocompetent Microphysiological Systems in Drug Development: Current Perspective and Recommendations.

Author

Wang X, Kopec AK, Collinge M, David R, Grant C, Hardwick RN, Navratil A, Patel N, Rowan W, and Marshall N

Abstract

Immune responses are heavily involved in the regulation and pathogenesis of human diseases, including infectious diseases, inflammatory and autoimmune conditions, cancer, neurological disorders, and cardiometabolic syndromes. The immune system is considered a double-edged sword serving as a powerful host defense mechanism against infection and cancerous cells and causing detrimental tissue damage when the immune response is exaggerated or uncontrollable. One of the challenges in studying the efficacy and toxicity of drugs that target or modulate the immune system is the lack of suitable preclinical human models that are predictive of human response. Recent advancements in human microphysiological systems (MPS) have provided a promising in vitro platform to evaluate the response of immune organs ex vivo, to investigate the interaction of immune cells with non-lymphoid tissue cells, and to reduce the reliance on animals in preclinical studies. The development, regulation, trafficking, and responses of immune cells have been extensively studied in preclinical animal models and clinically, providing a wealth of knowledge by which to evaluate new in vitro models. Therefore, the application of immunocompetent MPS in drug discovery and development should first verify that the immune response in an MPS model recapitulates the complexity of the human immune physiology. This manuscript reviews biological functions of immune organ systems and tissue-resident immune cells and discusses contexts-of-use for commonly used immunocompetent and immune organ MPS models. Current perspective and recommendations are provided to guide the continued development of immune organ and immunocompetent MPS models and their application in drug discovery and development.

Published
2022
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44. Microphysiological systems in early stage drug development: Perspectives on current applications and future impact.

Author

Kopec AK, Yokokawa R, Khan N, Horii I, Finley JE, Bono CP, Donovan C, Roy J, Harney J, Burdick AD, Jessen B, Lu S, Collinge M, Sadeghian RB, Derzi M, Tomlinson L, and Burkhardt JE

Subjects
Animals, Biological Products, Drug Industry, Forecasting, Humans, Lab-On-A-Chip Devices, Drug Development methods, Drug Development trends, Microfluidic Analytical Techniques, Models, Biological
Abstract

Microphysiological systems (MPS) are making advances to provide more standardized and predictive physiologically relevant responses to test articles in living tissues and organ systems. The excitement surrounding the potential of MPS to better predict human responses to medicines and improving clinical translation is overshadowed by their relatively slow adoption by the pharmaceutical industry and regulators. Collaboration between multiorganizational consortia and regulators is necessary to build an understanding of the strengths and limitations of MPS models and closing the current gaps. Here, we review some of the advances in MPS research, focusing on liver, intestine, vascular system, kidney and lung and present examples highlighting the context of use for these systems. For MPS to gain a foothold in drug development, they must have added value over existing approaches. Ideally, the application of MPS will augment in vivo studies and reduce the use of animals via tiered screening with less reliance on exploratory toxicology studies to screen compounds. Because MPS support multiple cell types (e.g. primary or stem-cell derived cells) and organ systems, identifying when MPS are more appropriate than simple 2D in vitro models for understanding physiological responses to test articles is necessary. Once identified, MPS models require qualification for that specific context of use and must be reproducible to allow future validation. Ultimately, the challenges of balancing complexity with reproducibility will inform the promise of advancing the MPS field and are critical for realization of the goal to reduce, refine and replace (3Rs) the use of animals in nonclinical research.

Published
2021
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45. Cross-company evaluation of the human lymphocyte activation assay.

Author

Collinge M, Schneider P, Li D, Parish S, Dumont C, Freebern W, Ghanime J, Guimont-Derochers F, Langenkamp A, Lebron J, Li N, Marban C, Plitnick L, and Wheeler J

Subjects
Cells, Cultured, Cyclosporine pharmacology, Healthy Volunteers, Humans, Immunosuppressive Agents pharmacology, Influenza Vaccines immunology, Inhibitory Concentration 50, Leukocytes, Mononuclear, Lymphocyte Activation immunology, Mycophenolic Acid pharmacology, Reproducibility of Results, Biological Assay instrumentation, Cytotoxicity Tests, Immunologic methods, Drug Evaluation, Preclinical methods, Lymphocyte Activation drug effects
Abstract

Nonclinical immunotoxicity evaluation is an important component of safety assessment for pharmaceuticals. One in vitro assay that can be applied in a weight of evidence assessment is the human lymphocyte activation (HuLA) assay, an antigen recall assay, similar in many respects to the in vivo T-cell-dependent antibody response (TDAR) in that cooperation of multiple immune cell types are needed to produce responses. This assay uses human cells and is more amenable than the TDAR to compound ranking and mechanistic studies. The HuLA assay requires less time and drug than TDAR assays, uses a relevant antigen (influenza), reflects a human immune response, and applies principles of the 3Rs to non-clinical safety assessment. Peripheral blood mononuclear cells (PBMC) from flu-immunized donors are re-stimulated with flu-vaccine in the presence of test articles, and proliferation is measured. Published data demonstrate the applicability of the HuLA assay, but it has not been evaluated for reproducibility across testing sites. To evaluate assay reproducibility, scientists from a consortium of institutions conducted the assay in parallel, using a common pool of donor PBMC, influenza vaccine, and known immunosuppressant compounds (cyclosporine A and mycophenolic acid). The HuLA assay was highly reproducible in identification of inhibition of antigen-specific responses, and there was significant agreement across testing sites in the half maximal inhibitory concentration (IC 50 ) values. Intra-site variability was the largest contributor to the variability observed within the assay. The HuLA assay was demonstrated to be ideally suited to comparing multiple compounds (i.e. compound ranking or benchmarking) within the same assay. Overall, the data reported herein support the HuLA assay as a useful tool in mechanistic evaluations of antigen-specific immune responses.

Published
2020
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46. T cell LFA-1-induced proinflammatory mRNA stabilization is mediated by the p38 pathway kinase MK2 in a process regulated by hnRNPs C, H1 and K.

Author

Rao GK, Wong A, Collinge M, Sarhan J, Yarovinsky TO, Ramgolam VS, Gaestel M, Pardi R, and Bender JR

Subjects
Animals, Cell Culture Techniques, Cytoplasm metabolism, Humans, Intracellular Signaling Peptides and Proteins genetics, Jurkat Cells, Mice, Inbred C57BL, Mice, Knockout, Protein Serine-Threonine Kinases genetics, Proteome, RNA, Messenger metabolism, Signal Transduction, T-Lymphocytes cytology, ELAV-Like Protein 1 metabolism, Heterogeneous-Nuclear Ribonucleoproteins metabolism, Intracellular Signaling Peptides and Proteins metabolism, Lymphocyte Function-Associated Antigen-1 metabolism, Protein Serine-Threonine Kinases metabolism, RNA Stability physiology, T-Lymphocytes metabolism
Abstract

Activation of the β2 integrin lymphocyte function-associated antigen-1 (LFA-1) in T cells induces stabilization of proinflammatory AU-rich element (ARE)-bearing mRNAs, by triggering the nuclear-to-cytoplasmic translocation of the mRNA-binding and -stabilizing protein HuR. However, the mechanism by which LFA-1 engagement controls HuR localization is not known. Here, we identify and characterize four key regulators of LFA-1-induced changes in HuR activity: the p38 pathway kinase MK2 and the constitutive nuclear proteins hnRNPs C, H1 and K. LFA-1 engagement results in rapid, sequential activation of p38 and MK2. Post-LFA-1 activation, MK2 inducibly associates with both hnRNPC and HuR, resulting in the dissociation of HuR from hnRNPs C, H1 and K. Freed from the three hnRNPs, HuR translocates from the nucleus to the cytoplasm, and mediates the stabilization of labile cytokine transcripts. Our results suggest that the modulation of T cell cytokine mRNA half-life is an intricate process that is negatively regulated by hnRNPs C, H1 and K and requires MK2 as a critical activator., Competing Interests: The authors have declared that no competing interests exist.

Published
2018
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47. Reversibility of peripheral blood leukocyte phenotypic and functional changes after exposure to and withdrawal from tofacitinib, a Janus kinase inhibitor, in healthy volunteers.

Author

Weinhold KJ, Bukowski JF, Brennan TV, Noveck RJ, Staats JS, Lin L, Stempora L, Hammond C, Wouters A, Mojcik CF, Cheng J, Collinge M, Jesson MI, Hazra A, Biswas P, Lan S, Clark JD, and Hodge JA

Subjects
Adult, Aged, Arthritis, Rheumatoid drug therapy, Female, Healthy Volunteers, Humans, Leukocytes immunology, Lymphocyte Count, Male, Middle Aged, Phenotype, Piperidines adverse effects, Pyrimidines adverse effects, Pyrroles adverse effects, T-Lymphocytes drug effects, T-Lymphocytes immunology, Janus Kinase Inhibitors pharmacology, Leukocytes drug effects, Piperidines pharmacology, Pyrimidines pharmacology, Pyrroles pharmacology
Abstract

This study evaluated the short-term effects of tofacitinib treatment on peripheral blood leukocyte phenotype and function, and the reversibility of any such effects following treatment withdrawal in healthy volunteers. Cytomegalovirus (CMV)-seropositive subjects received oral tofacitinib 10 mg twice daily for 4 weeks and were followed for 4 weeks after drug withdrawal. There were slight increases in total lymphocyte and total T-cell counts during tofacitinib treatment, and B-cell counts increased by up to 26%. There were no significant changes in granulocyte or monocyte counts, or granulocyte function. Naïve and central memory T-cell counts increased during treatment, while all subsets of activated T cells were decreased by up to 69%. T-cell subsets other than effector memory cluster of differentiation (CD)4+, activated naïve CD4+ and effector CD8+ T-cell counts and B-cell counts, normalized 4 weeks after withdrawal. Following ex vivo activation, measures of CMV-specific T-cell responses, and antigen non-specific T-cell-mediated cytotoxicity and interferon (IFN)-γ production, decreased slightly. These T-cell functional changes were most pronounced at Day 15, partially normalized while still on tofacitinib and returned to baseline after drug withdrawal. Total natural killer (NK)-cell counts decreased by 33%, returning towards baseline after drug withdrawal. NK-cell function decreased during tofacitinib treatment, but without a consistent time course across measured parameters. However, markers of NK-cell-mediated cytotoxicity, antibody-dependent cellular cytotoxicity and IFN-γ production were decreased up to 42% 1 month after drug withdrawal. CMV DNA was not detectable in whole blood, and there were no cases of herpes zoster reactivation. No new safety concerns arose. In conclusion, the effect of short-term tofacitinib treatment on leukocyte composition and function in healthy CMV+ volunteers is modest and largely reversible 4 weeks after withdrawal., (Copyright © 2018 Pfizer Inc. Published by Elsevier Inc. All rights reserved.)

Published
2018
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48. Immunologic effects of chronic administration of tofacitinib, a Janus kinase inhibitor, in cynomolgus monkeys and rats - Comparison of juvenile and adult responses.

Author

Collinge M, Ball DJ, Bowman CJ, Nilson AL, Radi ZA, and Vogel WM

Subjects
Administration, Oral, Animals, Antigens immunology, Erythrocyte Count, Female, Hematocrit, Hemocyanins immunology, Hemoglobins analysis, Janus Kinase Inhibitors pharmacokinetics, Leukocyte Count, Leukocytes drug effects, Leukocytes immunology, Lymphoma, B-Cell chemically induced, Macaca fascicularis, Male, Organ Size drug effects, Piperidines pharmacokinetics, Pyrimidines pharmacokinetics, Pyrroles pharmacokinetics, Rats, Sprague-Dawley, Spleen drug effects, Spleen pathology, Thymus Gland drug effects, Thymus Gland pathology, Toxicity Tests, Chronic, Aging immunology, Janus Kinase Inhibitors toxicity, Piperidines toxicity, Pyrimidines toxicity, Pyrroles toxicity
Abstract

Tofacitinib, an oral Janus kinase (JAK) inhibitor for treatment of rheumatoid arthritis, targets JAK1, JAK3, and to a lesser extent JAK2 and TYK2. JAK1/3 inhibition impairs gamma common chain cytokine receptor signaling, important in lymphocyte development, homeostasis and function. Adult and juvenile cynomolgus monkey and rat studies were conducted and the impact of tofacitinib on immune parameters (lymphoid tissues and lymphocyte subsets) and function (T-dependent antibody response (TDAR), mitogen-induced T cell proliferation) assessed. Tofacitinib administration decreased circulating T cells and NK cells in juvenile and adult animals of both species. B cell decreases were observed only in rats. These changes and decreased lymphoid tissue cellularity are consistent with the expected pharmacology of tofacitinib. No differences were observed between juvenile and adult animals, either in terms of doses at which effects were observed or differential effects on immune endpoints. Lymphomas were observed in three adult monkeys. Tofacitinib impaired the primary TDAR in juvenile monkeys, although a recall response was generated. Complete or partial reversal of the effects on the immune system was observed., (Copyright © 2018 Elsevier Inc. All rights reserved.)

Published
2018
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49. Evaluation of a novel delayed-type hypersensitivity assay to Candida albicans in adult and neonatal rats.

Author

Thorn M, Hudson AW, Kreeger J, Kawabe TT, Bowman CJ, and Collinge M

Subjects
Animals, Chitosan chemistry, Female, Hypersensitivity, Delayed chemically induced, Mice, Rats, Rats, Sprague-Dawley, Candida albicans immunology, Candidiasis diagnosis, Candidiasis immunology, Chitosan immunology, Hypersensitivity, Delayed immunology
Abstract

Delayed-type hypersensitivity (DTH) is a T-cell-mediated immune response that may be used for immunotoxicity testing in non-clinical species. However, in some cases DTH assays using T-dependent antigens may be confounded by the production of antibodies to the antigen. The authors have previously modified a DTH assay, initially validated in the mouse, for use in juvenile rats to assess the effect of immunosuppressive drugs on the developing rat immune system. The assay measures footpad swelling induced by subcutaneous footpad injection of Candida albicans (C. albicans) derived-chitosan in rats previously sensitized with C. albicans. Antibodies to chitosan are not produced in this model. However, considerable inter-animal variability inherent in the footpad swelling assay can make it difficult to precisely quantify the magnitude of the immune response and inhibition by immunosuppressants, particularly if complete suppression is not observed. This report describes the development of an ex vivo assay to assess DTH in rats using interferon (IFN)-γ production by splenocytes, obtained from rats sensitized with C. albicans, as the quantifiable measure of the DTH response. Adult and neonatal rats administered dexamethasone (DEX), a known immunosuppressant, exhibited immunosuppression as evidenced by a reduction in ex vivo IFNγ production from splenocytes challenged with C. albicans-derived chitosan. Current data indicate that the ex vivo based DTH assay is more sensitive than the conventional footpad swelling assay due to a lower background response and the ability to detect a response as early as post-natal day (PND) 12. The ex vivo based rat DTH assay offers a highly sensitive and quantitative alternative to the footpad swelling assay for the assessment of the immunotoxic potential of drugs. The increased sensitivity of the ex vivo DTH assay may be useful for identifying smaller changes in response to immunotoxic drugs, as well as detecting responses earlier in animal development.

Published
2015
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50. Comparative nonclinical assessments of the proposed biosimilar PF-05280586 and rituximab (MabThera®).

Author

Ryan AM, Sokolowski SA, Ng CK, Shirai N, Collinge M, Shen AC, Arrington J, Radi Z, Cummings TR, Ploch SA, Stephenson SA, Tripathi NK, Hurst SI, Finch GL, and Leach MW

Subjects
Animals, Antigens, CD20 metabolism, B-Lymphocytes drug effects, B-Lymphocytes metabolism, Biosimilar Pharmaceuticals administration & dosage, Biosimilar Pharmaceuticals pharmacology, Dose-Response Relationship, Drug, Endpoint Determination, Female, Macaca fascicularis, Male, Reproducibility of Results, Rituximab, Antibodies, Monoclonal, Murine-Derived administration & dosage, Antibodies, Monoclonal, Murine-Derived pharmacokinetics
Abstract

Comparative nonclinical studies were conducted with the proposed biosimilar PF-05280586 and rituximab-EU (MabThera®). In side-by-side analyses, peptide maps and complement-dependent cytotoxicity assay results were similar. Sexually-mature cynomolgus monkeys were administered PF-05280586 or rituximab-EU as a single dose of 0, 2, 10, or 20 mg/kg on day 1 and observed for 92 days (single-dose study) or as 5 weekly injections of 0 or 20 mg/kg and necropsied on day 30, the day after the 5th dose, or on day 121 (repeat-dose study). The pharmacokinetic and pharmacodynamic profiles for both molecules were similar. Marked depletion of peripheral blood B cells 4 days after dosing was followed by near or complete repletion (single-dose study) or partial repletion (repeat-dose study). In the single-dose study, anti-drug antibodies (ADA) were detected by day 29 in all animals administered PF-05280586 or rituximab-EU and persisted through day 85, the last day tested. In the repeat-dose study, ADA were detected on day 121 in 50% of animals administered PF-05280586 or rituximab-EU. Both molecules were well tolerated at all doses. In all endpoints evaluated, PF-05280586 exhibited similarity to rituximab-EU., (© 2014 by The Author(s).)

Published
2014
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