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21 results on '"Gangatirkar P"'

1. An immunohistochemical atlas of necroptotic pathway expression

Author

Chiou, Shene, Al-Ani, Aysha H, Pan, Yi, Patel, Komal M, Kong, Isabella Y, Whitehead, Lachlan W, Light, Amanda, Young, Samuel N, Barrios, Marilou, Sargeant, Callum, Rajasekhar, Pradeep, Zhu, Leah, Hempel, Anne, Lin, Ann, Rickard, James A, Hall, Cathrine, Gangatirkar, Pradnya, Yip, Raymond KH, Cawthorne, Wayne, Jacobsen, Annette V, Horne, Christopher R, Martin, Katherine R, Ioannidis, Lisa J, Hansen, Diana S, Day, Jessica, Wicks, Ian P, Law, Charity, Ritchie, Matthew E, Bowden, Rory, Hildebrand, Joanne M, O’Reilly, Lorraine A, Silke, John, Giulino-Roth, Lisa, Tsui, Ellen, Rogers, Kelly L, Hawkins, Edwin D, Christensen, Britt, Murphy, James M, and Samson, André L

Published
2024
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2. MLKL deficiency protects against low-grade, sterile inflammation in aged mice

Author

Tovey Crutchfield, Emma C., Garnish, Sarah E., Day, Jessica, Anderton, Holly, Chiou, Shene, Hempel, Anne, Hall, Cathrine, Patel, Komal M., Gangatirkar, Pradnya, Martin, Katherine R., Li Wai Suen, Connie S. N., Garnham, Alexandra L., Kueh, Andrew J., Wicks, Ian P., Silke, John, Nachbur, Ueli, Samson, Andre L., Murphy, James M., and Hildebrand, Joanne M.

Published
2023
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3. Automated grading of enlarged perivascular spaces in clinical imaging data of an acute stroke cohort using an interpretable, 3D deep learning framework

Author

Williamson, Brady J., Khandwala, Vivek, Wang, David, Maloney, Thomas, Sucharew, Heidi, Horn, Paul, Haverbusch, Mary, Alwell, Kathleen, Gangatirkar, Shantala, Mahammedi, Abdelkader, Wang, Lily L., Tomsick, Thomas, Gaskill-Shipley, Mary, Cornelius, Rebecca, Khatri, Pooja, Kissela, Brett, and Vagal, Achala

Published
2022
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7. A missense mutation in the MLKL brace region promotes lethal neonatal inflammation and hematopoietic dysfunction

Author

Hildebrand, Joanne M., Kauppi, Maria, Majewski, Ian J., Liu, Zikou, Cox, Allison J., Miyake, Sanae, Petrie, Emma J., Silk, Michael A., Li, Zhixiu, Tanzer, Maria C., Brumatti, Gabriela, Young, Samuel N., Hall, Cathrine, Garnish, Sarah E., Corbin, Jason, Stutz, Michael D., Di Rago, Ladina, Gangatirkar, Pradnya, Josefsson, Emma C., Rigbye, Kristin, Anderton, Holly, Rickard, James A., Tripaydonis, Anne, Sheridan, Julie, Scerri, Thomas S., Jackson, Victoria E., Czabotar, Peter E., Zhang, Jian-Guo, Varghese, Leila, Allison, Cody C., Pellegrini, Marc, Tannahill, Gillian M., Hatchell, Esme C., Willson, Tracy A., Stockwell, Dina, de Graaf, Carolyn A., Collinge, Janelle, Hilton, Adrienne, Silke, Natasha, Spall, Sukhdeep K., Chau, Diep, Athanasopoulos, Vicki, Metcalf, Donald, Laxer, Ronald M., Bassuk, Alexander G., Darbro, Benjamin W., Fiatarone Singh, Maria A., Vlahovich, Nicole, Hughes, David, Kozlovskaia, Maria, Ascher, David B., Warnatz, Klaus, Venhoff, Nils, Thiel, Jens, Biben, Christine, Blum, Stefan, Reveille, John, Hildebrand, Michael S., Vinuesa, Carola G., McCombe, Pamela, Brown, Matthew A., Kile, Benjamin T., McLean, Catriona, Bahlo, Melanie, Masters, Seth L., Nakano, Hiroyasu, Ferguson, Polly J., Murphy, James M., Alexander, Warren S., and Silke, John

Published
2020
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11. Proinflammatory microenvironment promotes lymphoma progression in mice with high megakaryocyte and TPO levels.

Author

Au AE, Corbin J, Lebois M, Gangatirkar P, Yassinson F, Hyslop SR, Cannon P, Mason KD, Li-Wai-Suen CSN, Garnham AL, Moujalled D, Cimmino L, Alexander WS, and Josefsson EC

Subjects
Mice, Animals, Humans, Megakaryocytes metabolism, Receptors, Thrombopoietin, Blood Platelets metabolism, Tumor Microenvironment, Thrombocytopenia genetics, Lymphoma genetics
Abstract

Platelets have been shown to enhance the survival of lymphoma cell lines. However, it remains unclear whether they play a role in lymphoma. Here, we investigated the potential role of platelets and/or megakaryocytes in the progression of Eμ-myc lymphoma. Eμ-myc tumor cells were transplanted into recipient wild-type (WT) control, Mpl-/-, or TpoTg mice, which exhibited normal, low, and high platelet and megakaryocyte counts, respectively. TpoTg mice that underwent transplantation exhibited enhanced lymphoma progression with increased white blood cell (WBC) counts, spleen and lymph node weights, and enhanced liver infiltration when compared with WT mice. Conversely, tumor-bearing Mpl-/- mice had reduced WBC counts, lymph node weights, and less liver infiltration than WT mice. Using an Mpl-deficient thrombocytopenic immunocompromised mouse model, our results were confirmed using the human non-Hodgkin lymphoma GRANTA cell line. Although we found that platelets and platelet-released molecules supported Eμ-myc tumor cell survival in vitro, pharmacological inhibition of platelet function or anticoagulation in WT mice transplanted with Eμ-myc did not improve disease outcome. Furthermore, transient platelet depletion or sustained Bcl-xL-dependent thrombocytopenia did not alter lymphoma progression. Cytokine analysis of the bone marrow fluid microenvironment revealed increased levels of the proinflammatory molecule interleukin 1 in TpoTg mice, whereas these levels were lower in Mpl-/- mice. Moreover, RNA sequencing of blood-resident Eμ-myc lymphoma cells from TpoTg and WT mice after tumor transplantation revealed the upregulation of hallmark gene sets associated with an inflammatory response in TpoTg mice. We propose that the proinflammatory microenvironment in TpoTg mice promotes lymphoma progression., (© 2023 by The American Society of Hematology. Licensed under Creative Commons Attribution-NonCommercial-NoDerivatives 4.0 International (CC BY-NC-ND 4.0), permitting only noncommercial, nonderivative use with attribution. All other rights reserved.)

Published
2023
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12. The RNA-binding protein SRSF3 has an essential role in megakaryocyte maturation and platelet production.

Author

Heazlewood SY, Ahmad T, Mohenska M, Guo BB, Gangatirkar P, Josefsson EC, Ellis SL, Ratnadiwakara M, Cao H, Cao B, Heazlewood CK, Williams B, Fulton M, White JF, Ramialison M, Nilsson SK, and Änkö ML

Subjects
Animals, Mice, Mice, Knockout, Blood Platelets metabolism, Megakaryocytes metabolism, RNA, Messenger genetics, RNA, Messenger metabolism, Serine-Arginine Splicing Factors genetics, Serine-Arginine Splicing Factors metabolism, Thrombocytopenia genetics, Thrombocytopenia metabolism, Thrombopoiesis genetics
Abstract

RNA processing is increasingly recognized as a critical control point in the regulation of different hematopoietic lineages including megakaryocytes responsible for the production of platelets. Platelets are anucleate cytoplasts that contain a rich repertoire of RNAs encoding proteins with essential platelet functions derived from the parent megakaryocyte. It is largely unknown how RNA binding proteins contribute to the development and functions of megakaryocytes and platelets. We show that serine-arginine-rich splicing factor 3 (SRSF3) is essential for megakaryocyte maturation and generation of functional platelets. Megakaryocyte-specific deletion of Srsf3 in mice led to macrothrombocytopenia characterized by megakaryocyte maturation arrest, dramatically reduced platelet counts, and abnormally large functionally compromised platelets. SRSF3 deficient megakaryocytes failed to reprogram their transcriptome during maturation and to load platelets with RNAs required for normal platelet function. SRSF3 depletion led to nuclear accumulation of megakaryocyte mRNAs, demonstrating that SRSF3 deploys similar RNA regulatory mechanisms in megakaryocytes as in other cell types. Our study further suggests that SRSF3 plays a role in sorting cytoplasmic megakaryocyte RNAs into platelets and demonstrates how SRSF3-mediated RNA processing forms a central part of megakaryocyte gene regulation. Understanding SRSF3 functions in megakaryocytes and platelets provides key insights into normal thrombopoiesis and platelet pathologies as SRSF3 RNA targets in megakaryocytes are associated with platelet diseases., (© 2022 by The American Society of Hematology. Licensed under Creative Commons Attribution-NonCommercial-NoDerivatives 4.0 International (CC BY-NC-ND 4.0), permitting only noncommercial, nonderivative use with attribution. All other rights reserved.)

Published
2022
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13. Membrane budding is a major mechanism of in vivo platelet biogenesis.

Author

Potts KS, Farley A, Dawson CA, Rimes J, Biben C, de Graaf C, Potts MA, Stonehouse OJ, Carmagnac A, Gangatirkar P, Josefsson EC, Anttila C, Amann-Zalcenstein D, Naik S, Alexander WS, Hilton DJ, Hawkins ED, and Taoudi S

Subjects
Animals, Blood Platelets metabolism, Blood Platelets ultrastructure, Bone Marrow Cells cytology, Cell Lineage, Cell Membrane ultrastructure, Databases as Topic, Embryo, Mammalian cytology, Fetus cytology, Gene Expression Regulation, Imaging, Three-Dimensional, Integrases metabolism, Liver embryology, Megakaryocytes cytology, Megakaryocytes metabolism, Mice, Inbred C57BL, Ploidies, Reproducibility of Results, Skull cytology, Blood Platelets cytology, Cell Membrane metabolism
Abstract

How platelets are produced by megakaryocytes in vivo remains controversial despite more than a century of investigation. Megakaryocytes readily produce proplatelet structures in vitro; however, visualization of platelet release from proplatelets in vivo has remained elusive. We show that within the native prenatal and adult environments, the frequency and rate of proplatelet formation is incompatible with the physiological demands of platelet replacement. We resolve this inconsistency by performing in-depth analysis of plasma membrane budding, a cellular process that has previously been dismissed as a source of platelet production. Our studies demonstrate that membrane budding results in the sustained release of platelets directly into the peripheral circulation during both fetal and adult life without induction of cell death or proplatelet formation. In support of this model, we demonstrate that in mice deficient for NF-E2 (the thrombopoietic master regulator), the absence of membrane budding correlates with failure of in vivo platelet production. Accordingly, we propose that membrane budding, rather than proplatelet formation, supplies the majority of the platelet biomass., Competing Interests: Disclosures: The authors declare no competing interests exist., (© 2020 Potts et al.)

Published
2020
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14. Intrinsic apoptosis circumvents the functional decline of circulating platelets but does not cause the storage lesion.

Author

Pleines I, Lebois M, Gangatirkar P, Au AE, Lane RM, Henley KJ, Kauppi M, Corbin J, Cannon P, Bernardini J, Alwis I, Jarman KE, Ellis S, Metcalf D, Jackson SP, Schoenwaelder SM, Kile BT, and Josefsson EC

Subjects
Animals, Biomarkers, Bleeding Time, Blood Cell Count, Blood Coagulation, Caspases metabolism, Cell Survival genetics, Female, Genotype, Male, Mice, Mice, Knockout, Mitochondria metabolism, Signal Transduction, bcl-2-Associated X Protein genetics, bcl-2-Associated X Protein metabolism, bcl-X Protein genetics, bcl-X Protein metabolism, Apoptosis genetics, Blood Platelets metabolism, Disease Susceptibility
Abstract

The circulating life span of blood platelets is regulated by the prosurvival protein BCL-X L It restrains the activity of BAK and BAX, the essential prodeath mediators of intrinsic apoptosis. Disabling the platelet intrinsic apoptotic pathway in mice by deleting BAK and BAX results in a doubling of platelet life span and concomitant thrombocytosis. Apoptotic platelets expose phosphatidylserine (PS) via a mechanism that is distinct from that driven by classical agonists. Whether there is any role for apoptotic PS in platelet function in vivo, however, is unclear. Apoptosis has also been associated with the platelet storage lesion (PSL), the constellation of biochemical deteriorations that occur during blood bank storage. In this study, we investigated the role of BAK/BAX-mediated apoptosis in hemostasis and thrombosis and in the development of the PSL. We show that although intrinsic apoptosis is rapidly induced during storage at 37°C, it is not detected when platelets are kept at the standard storage temperature of 22°C. Remarkably, loss of BAK and BAX did not prevent the development of the PSL at either temperature. BAK/BAX-deficient mice exhibited increased bleeding times and unstable thrombus formation. This phenotype was not caused by impaired PS exposure, but was associated with a defect in granule release from aged platelets. Strikingly, rejuvenation of BAK/BAX-deficient platelets in vivo completely rescued the observed hemostatic defects. Thus, apoptotic culling of old platelets from the bloodstream is essential to maintain a functional, hemostatically reactive platelet population. Inhibiting intrinsic apoptosis in blood banked platelets is unlikely to yield significant benefit., (© 2018 by The American Society of Hematology.)

Published
2018
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15. Altered B-lymphopoiesis in mice with deregulated thrombopoietin signaling.

Author

Au AE, Lebois M, Sim SA, Cannon P, Corbin J, Gangatirkar P, Hyland CD, Moujalled D, Rutgersson A, Yassinson F, Kile BT, Mason KD, Ng AP, Alexander WS, and Josefsson EC

Subjects
Animals, B-Lymphocytes metabolism, Cell Cycle, Female, Lymphoid Progenitor Cells metabolism, Male, Mice, Mice, Inbred C57BL, B-Lymphocytes cytology, Lymphoid Progenitor Cells cytology, Lymphopoiesis, Signal Transduction, Thrombopoietin metabolism
Abstract

Thrombopoietin (TPO) is the master cytokine regulator of megakaryopoiesis. In addition to regulation of megakaryocyte and platelet number, TPO is important for maintaining proper hematopoietic stem cell (HSC) function. It was previously shown that a number of lymphoid genes were upregulated in HSCs from Tpo -/- mice. We investigated if absent or enhanced TPO signaling would influence normal B-lymphopoiesis. Absent TPO signaling in Mpl -/- mice led to enrichment of a common lymphoid progenitor (CLP) signature in multipotential lineage-negative Sca-1 + c-Kit + (LSK) cells and an increase in CLP formation. Moreover, Mpl -/- mice exhibited increased numbers of PreB2 and immature B-cells in bone marrow and spleen, with an increased proportion of B-lymphoid cells in the G1 phase of the cell cycle. Conversely, elevated TPO signaling in Tpo Tg mice was associated with reduced B-lymphopoiesis. Although at steady state, peripheral blood lymphocyte counts were normal in both models, Mpl -/- Eµ-myc mice showed an enhanced preneoplastic phase with increased numbers of splenic PreB2 and immature B-cells, a reduced quiescent fraction, and augmented blood lymphocyte counts. Thus, although Mpl is not expressed on lymphoid cells, TPO signaling may indirectly influence B-lymphopoiesis and the preneoplastic state in Myc-driven B-cell lymphomagenesis by lineage priming in multipotential progenitor cells.

Published
2017
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16. Differential requirement for Nfil3 during NK cell development.

Author

Seillet C, Huntington ND, Gangatirkar P, Axelsson E, Minnich M, Brady HJ, Busslinger M, Smyth MJ, Belz GT, and Carotta S

Subjects
Animals, Animals, Newborn, Basic-Leucine Zipper Transcription Factors genetics, Basic-Leucine Zipper Transcription Factors metabolism, Cell Differentiation genetics, Cell Lineage genetics, Cells, Cultured, Flow Cytometry, Gene Expression immunology, Killer Cells, Natural metabolism, Liver cytology, Liver immunology, Liver metabolism, Mice, Mice, Knockout, Mice, Transgenic, Reverse Transcriptase Polymerase Chain Reaction, T-Box Domain Proteins genetics, T-Box Domain Proteins immunology, T-Box Domain Proteins metabolism, TNF-Related Apoptosis-Inducing Ligand genetics, TNF-Related Apoptosis-Inducing Ligand immunology, TNF-Related Apoptosis-Inducing Ligand metabolism, Thymus Gland cytology, Thymus Gland immunology, Thymus Gland metabolism, Basic-Leucine Zipper Transcription Factors immunology, Cell Differentiation immunology, Cell Lineage immunology, Killer Cells, Natural immunology
Abstract

NK cells can be grouped into distinct subsets that are localized to different organs and exhibit a different capacity to secrete cytokines and mediate cytotoxicity. Despite these hallmarks that reflect tissue-specific specialization in NK cells, little is known about the factors that control the development of these distinct subsets. The basic leucine zipper transcription factor Nfil3 (E4bp4) is essential for bone marrow-derived NK cell development, but it is not clear whether Nfil3 is equally important for all NK cell subsets or how it induces NK lineage commitment. In this article, we show that Nfil3 is required for the formation of Eomes-expressing NK cells, including conventional medullary and thymic NK cells, whereas TRAIL(+) Eomes(-) NK cells develop independently of Nfil3. Loss of Nfil3 during the development of bone marrow-derived NK cells resulted in reduced expression of Eomes and, conversely, restoration of Eomes expression in Nfil3(-/-) progenitors rescued NK cell development and maturation. Collectively, these findings demonstrate that Nfil3 drives the formation of mature NK cells by inducing Eomes expression and reveal the differential requirements of NK cell subsets for Nfil3.

Published
2014
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17. Functional characterization of quiescent keratinocyte stem cells and their progeny reveals a hierarchical organization in human skin epidermis.

Author

Schlüter H, Paquet-Fifield S, Gangatirkar P, Li J, and Kaur P

Subjects
Animals, Antigens, CD metabolism, Cell Physiological Phenomena, Flow Cytometry, Foreskin cytology, Gene Expression Profiling, Humans, Infant, Newborn, Keratinocytes physiology, Keratinocytes transplantation, Male, Mice, Mice, SCID, Oligonucleotide Array Sequence Analysis, Rats, Receptors, Transferrin metabolism, Regeneration, Skin Physiological Phenomena, Trachea pathology, Transplantation, Heterologous, Epidermis physiology, Keratinocytes cytology, Skin cytology, Stem Cells physiology
Abstract

Although homeostatic renewal of human skin epidermis is achieved by the combined activity of quiescent stem cells (SCs) and their actively cycling progeny, whether these two populations are equipotent in their capacity to regenerate tissue has not been determined in biological assays that mimic lifelong renewal. Using fluorescence activated cell separation strategy validated previously by us, human epidermis was fractionated into three distinct subsets: that is, α 6briCD71(dim) , α 6briCD71(bri) , and α 6dim with characteristics of keratinocyte stem, transient amplifying, and early differentiating cells, respectively. The global gene expression profile of these fractions was determined by microarray, confirming that the α 6briCD71(dim) subset was quiescent, the α 6briCD71(bri) was actively cycling, and the α 6dim subset expressed markers of differentiation. More importantly, functional evaluation of these populations in an in vivo model for tissue reconstitution at limiting cell dilutions revealed that the quiescent α 6briCD71(dim) fraction was the most potent proliferative and tissue regenerative population of the epidermis, capable of long-term (LT) epidermal renewal from as little as 100 cells for up to 10 weeks. In contrast, the cycling α 6briCD71(bri) fraction was the first to initiate tissue reconstitution, although this was not sustained in the LT, while differentiating α 6dim cells possessed the lowest demonstrable tissue regenerative capacity. Our data suggest that in human skin, the epidermal proliferative compartment is not composed of equipotent cells, but rather is organized in a functionally hierarchical manner with the most potent quiescent SCs at its apex (i.e., α 6briCD71(dim) ) followed by cycling progenitors (i.e., α 6briCD71(bri) ) and finally early differentiating keratinocytes (i.e., α 6dim)., (Copyright © 2011 AlphaMed Press.)

Published
2011
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18. A role for pericytes as microenvironmental regulators of human skin tissue regeneration.

Author

Paquet-Fifield S, Schlüter H, Li A, Aitken T, Gangatirkar P, Blashki D, Koelmeyer R, Pouliot N, Palatsides M, Ellis S, Brouard N, Zannettino A, Saunders N, Thompson N, Li J, and Kaur P

Subjects
Base Sequence, Cell Differentiation, Cells, Cultured, Coculture Techniques, Epidermal Cells, Epidermis metabolism, Gene Expression, Humans, Keratinocytes cytology, Keratinocytes metabolism, Laminin genetics, Laminin metabolism, Mesenchymal Stem Cells cytology, Mesenchymal Stem Cells physiology, Oligonucleotide Array Sequence Analysis, Pericytes cytology, RNA, Messenger genetics, RNA, Messenger metabolism, Regeneration genetics, Pericytes physiology, Regeneration physiology, Skin Physiological Phenomena
Abstract

The cellular and molecular microenvironment of epithelial stem and progenitor cells is poorly characterized despite well-documented roles in homeostatic tissue renewal, wound healing, and cancer progression. Here, we demonstrate that, in organotypic cocultures, dermal pericytes substantially enhanced the intrinsically low tissue-regenerative capacity of human epidermal cells that have committed to differentiate and that this enhancement was independent of angiogenesis. We used microarray analysis to identify genes expressed by human dermal pericytes that could potentially promote epidermal regeneration. Using this approach, we identified as a candidate the gene LAMA5, which encodes laminin alpha5, a subunit of the ECM component laminin-511/521 (LM-511/521). LAMA5 was of particular interest as we had previously shown that it promotes skin regeneration both in vitro and in vivo. Analysis using immunogold localization revealed that pericytes synthesized and secreted LAMA5 in human skin. Consistent with this observation, coculture with pericytes enhanced LM-511/521 deposition in the dermal-epidermal junction of organotypic cultures. We further showed that skin pericytes could also act as mesenchymal stem cells, exhibiting the capacity to differentiate into bone, fat, and cartilage lineages in vitro. This study suggests that pericytes represent a potent stem cell population in the skin that is capable of modifying the ECM microenvironment and promoting epidermal tissue renewal from non-stem cells, a previously unsuspected role for pericytes.

Published
2009
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19. Combination therapy of established cancer using a histone deacetylase inhibitor and a TRAIL receptor agonist.

Author

Frew AJ, Lindemann RK, Martin BP, Clarke CJ, Sharkey J, Anthony DA, Banks KM, Haynes NM, Gangatirkar P, Stanley K, Bolden JE, Takeda K, Yagita H, Secrist JP, Smyth MJ, and Johnstone RW

Subjects
Animals, Antibodies, Monoclonal pharmacology, CASP8 and FADD-Like Apoptosis Regulating Protein biosynthesis, Cell Line, Tumor, Down-Regulation drug effects, Gene Expression Regulation, Neoplastic drug effects, Histone Deacetylases metabolism, Humans, Hydroxamic Acids pharmacology, Mammary Neoplasms, Experimental metabolism, Mice, Mice, Inbred BALB C, Mice, SCID, Neoplasm Proteins metabolism, Receptors, TNF-Related Apoptosis-Inducing Ligand metabolism, Vorinostat, Antineoplastic Combined Chemotherapy Protocols pharmacology, Apoptosis drug effects, Histone Deacetylase Inhibitors, Mammary Neoplasms, Experimental drug therapy, Neoplasm Proteins agonists, Neoplasm Proteins antagonists & inhibitors, Receptors, TNF-Related Apoptosis-Inducing Ligand agonists
Abstract

Histone deacetylase inhibitors (HDACi) and agents such as recombinant tumor necrosis factor-related apoptosis-inducing ligand (TRAIL) and agonistic anti-TRAIL receptor (TRAIL-R) antibodies are anticancer agents that have shown promise in preclinical settings and in early phase clinical trials as monotherapies. Although HDACi and activators of the TRAIL pathway have different molecular targets and mechanisms of action, they share the ability to induce tumor cell-selective apoptosis. The ability of HDACi to induce expression of TRAIL-R death receptors 4 and 5 (DR4/DR5), and induce tumor cell death via the intrinsic apoptotic pathway provides a molecular rationale to combine these agents with activators of the TRAIL pathway that activate the alternative (death receptor) apoptotic pathway. Herein, we demonstrate that the HDACi vorinostat synergizes with the mouse DR5-specific monoclonal antibody MD5-1 to induce rapid and robust tumor cell apoptosis in vitro and in vivo. Importantly, using a preclinical mouse breast cancer model, we show that the combination of vorinostat and MD5-1 is safe and induces regression of established tumors, whereas single agent treatment had little or no effect. Functional analyses revealed that rather than mediating enhanced tumor cell apoptosis via the simultaneous activation of the intrinsic and extrinsic apoptotic pathways, vorinostat augmented MD5-1-induced apoptosis concomitant with down-regulation of the intracellular apoptosis inhibitor cellular-FLIP (c-FLIP). These data demonstrate that combination therapies involving HDACi and activators of the TRAIL pathway can be efficacious for the treatment of cancer in experimental mouse models.

Published
2008
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20. Establishment of 3D organotypic cultures using human neonatal epidermal cells.

Author

Gangatirkar P, Paquet-Fifield S, Li A, Rossi R, and Kaur P

Subjects
Cell Differentiation physiology, Collagen, Fibroblasts, Flow Cytometry methods, Humans, Infant, Newborn, Cell Culture Techniques methods, Epidermal Cells, Keratinocytes cytology
Abstract

This protocol describes an ex vivo three-dimensional coculture system optimized to study the skin regenerative ability of primary human keratinocytes grown at the air-liquid interface on collagen matrices embedded with human dermal fibroblasts. An option for enrichment of keratinocyte stem cells and their progeny using fluorescence-activated cell sorting is also provided. Initially, dermal equivalents, comprising human passaged fibroblasts seeded in a collagen matrix, are grown on porous filters (3 mum) placed in transwells. After 1 week, primary human keratinocytes are seeded on this base. One week later, an air-lift transition is performed, leading to the differentiation of the keratinocytes, which are macroscopically visible as artificial skin after a couple of days. The cultures can be harvested 1 week after the air-lift and processed for immunohistochemistry or gene expression analysis. The overall procedure can be completed in 3 weeks, including the preparation of the dermal equivalent and the seeding of the primary keratinocytes.

Published
2007
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21. Monoclonal antibodies to gonadotropin-releasing hormone (GnRH) inhibit binding of the hormone to its receptor.

Author

Gangatirkar P, Gangadharan S, Narendranath A, Nagpal S, Salunke DM, and Karande AA

Subjects
Amino Acid Sequence, Animals, Cell Line, Cells, Cultured, Epitope Mapping, Epitopes chemistry, Epitopes genetics, Gonadotropin-Releasing Hormone chemistry, Gonadotropin-Releasing Hormone genetics, Hybridomas immunology, Luteinizing Hormone metabolism, Mice, Molecular Sequence Data, Neutralization Tests, Pituitary Gland metabolism, Proto-Oncogene Proteins c-fos metabolism, Rats, Antibodies, Monoclonal, Gonadotropin-Releasing Hormone immunology, Gonadotropin-Releasing Hormone metabolism, Receptors, LHRH metabolism
Abstract

Monoclonal antibodies (MAbs) specific to gonadotropin-releasing hormone (GnRH) were obtained using different strategies of conjugation of the peptide to carrier protein and immunization. Of several antibodies obtained, two, namely F1D3C5 and E2D2 bound GnRH in solution phase. Though the epitopes corresponding to the two overlapped, there was a one amino acid shift in the core epitope. These two antibodies were characterized with respect to inhibition of GnRH induced responses in rat pituitary cultures and alpha-T3.1 mouse gonadotrope cell line.

Published
2002
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