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1. Ceramide-induced integrated stress response overcomes Bcl-2 inhibitor resistance in acute myeloid leukemia

Author

Lewis, Alexander C., Pope, Victoria S., Tea, Melinda N., Li, Manjun, Nwosu, Gus O., Nguyen, Thao M., Wallington-Beddoe, Craig T., Moretti, Paul A.B., Anderson, Dovile, Creek, Darren J., Costabile, Maurizio, Ali, Saira R., Thompson-Peach, Chloe A.L., Dredge, B. Kate, Bert, Andrew G., Goodall, Gregory J., Ekert, Paul G., Brown, Anna L., D'Andrea, Richard, Robinson, Nirmal, Pitman, Melissa R., Thomas, Daniel, Ross, David M., Gliddon, Briony L., Powell, Jason A., and Pitson, Stuart M.

Published
2022
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4. Endogenous bystander killing mechanisms enhance the activity of novel FAP‐specific CAR‐T cells against glioblastoma.

Author

Yu, Wenbo, Truong, Nga TH, Polara, Ruhi, Gargett, Tessa, Tea, Melinda N, Pitson, Stuart M, Cockshell, Michaelia P, Bonder, Claudine S, Ebert, Lisa M, and Brown, Michael P

Subjects
GLIOBLASTOMA multiforme, NEURAL stem cells, TUMOR growth, CYTOTOXINS
Abstract

Objectives: CAR‐T cells are being investigated as a novel immunotherapy for glioblastoma, but clinical success has been limited. We recently described fibroblast activation protein (FAP) as an ideal target antigen for glioblastoma immunotherapy, with expression on both tumor cells and tumor blood vessels. However, CAR‐T cells targeting FAP have never been investigated as a therapy for glioblastoma. Methods: We generated a novel FAP targeting CAR with CD3ζ and CD28 signalling domains and tested the resulting CAR‐T cells for their lytic activity and cytokine secretion function in vitro (using real‐time impedance, flow cytometry, imaging and bead‐based cytokine assays), and in vivo (using a xenograft mimicking the natural heterogeneity of human glioblastoma). Results: FAP‐CAR‐T cells exhibited target specificity against model cell lines and potent cytotoxicity against patient‐derived glioma neural stem cells, even when only a subpopulation expressed FAP, indicating a bystander killing mechanism. Using co‐culture assays, we confirmed FAP‐CAR‐T cells mediate bystander killing of antigen‐negative tumor cells, but only after activation by FAP‐positive target cells. This bystander killing was at least partially mediated by soluble factors and amplified by IL‐2 which activated the non‐transduced fraction of the CAR‐T product. Finally, a low dose of intravenously administered FAP‐CAR‐T cells controlled, without overt toxicity, the growth of subcutaneous tumors created using a mixture of antigen‐negative and antigen‐positive glioblastoma cells. Conclusions: Our findings advance FAP as a leading candidate for clinical CAR‐T therapy of glioblastoma and highlight under‐recognised antigen nonspecific mechanisms that may contribute meaningfully to the antitumor activity of CAR‐T cells. [ABSTRACT FROM AUTHOR]

Published
2024
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7. An orthotopic syngeneic mouse model of bortezomib‐resistant multiple myeloma.

Author

Li, Manjun, Bennett, Melissa K., Toubia, John, Pope, Victoria S., Tea, Melinda N., Tamang, Sarah, Samuel, Michael S., Anderson, Paul H., Gliddon, Briony L., Powell, Jason A., and Pitson, Stuart M.

Subjects
LABORATORY mice, MULTIPLE myeloma, ANIMAL disease models, ANIMAL models in research, INCURABLE diseases
Abstract

Summary: While bortezomib has significant benefits in multiple myeloma (MM) therapy, the disease remains incurable due to the invariable development of bortezomib resistance. This emphasises the need for advanced models for preclinical evaluation of new therapeutic approaches for bortezomib‐resistant MM. Here, we describe the development of an orthotopic syngeneic bortezomib‐resistant MM mouse model based on the most well‐characterised syngeneic MM mouse model derived from spontaneous MM‐forming C57BL/KaLwRij mice. Using bortezomib‐resistant 5TGM1 cells, we report and characterise a robust syngeneic mouse model of bortezomib‐resistant MM that is well suited to the evaluation of new therapeutic approaches for proteasome inhibitor‐resistant MM. [ABSTRACT FROM AUTHOR]

Published
2024
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8. GD2-targeting CAR-T cells enhanced by transgenic IL-15 expression are an effective and clinically feasible therapy for glioblastoma

Author

Gargett, Tessa, primary, Ebert, Lisa M, additional, Truong, Nga T H, additional, Kollis, Paris M, additional, Sedivakova, Kristyna, additional, Yu, Wenbo, additional, Yeo, Erica C F, additional, Wittwer, Nicole L, additional, Gliddon, Briony L, additional, Tea, Melinda N, additional, Ormsby, Rebecca, additional, Poonnoose, Santosh, additional, Nowicki, Jake, additional, Vittorio, Orazio, additional, Ziegler, David S, additional, Pitson, Stuart M, additional, and Brown, Michael P, additional

Published
2022
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9. Characterising Distinct Migratory Profiles of Infiltrating T-Cell Subsets in Human Glioblastoma

Author

Kollis, Paris M., primary, Ebert, Lisa M., additional, Toubia, John, additional, Bastow, Cameron R., additional, Ormsby, Rebecca J., additional, Poonnoose, Santosh I., additional, Lenin, Sakthi, additional, Tea, Melinda N., additional, Pitson, Stuart M., additional, Gomez, Guillermo A., additional, Brown, Michael P., additional, and Gargett, Tessa, additional

Published
2022
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10. Additional file 7 of 3D-printed microplate inserts for long term high-resolution imaging of live brain organoids

Author

Mansilla, Mariana Oksdath, Salazar-Hernandez, Camilo, Perrin, Sally L., Scheer, Kaitlin G., Cildir, Gökhan, Toubia, John, Kristyna Sedivakova, Tea, Melinda N., Sakthi Lenin, Ponthier, Elise, Yeo, Erica C. F., Tergaonkar, Vinay, Poonnoose, Santosh, Ormsby, Rebecca J., Pitson, Stuart M., Brown, Michael P., Ebert, Lisa M., and Gomez, Guillermo A.

Abstract

Additional file 7: Supplementary Information. This contains information related to 1) Image J script for image segmentation and quantification of different organoid parameters and 2) Matlab script for Spearman correlation coefficient analysis between RNA expression profiles.

Published
2021
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11. Additional file 5 of 3D-printed microplate inserts for long term high-resolution imaging of live brain organoids

Author

Mansilla, Mariana Oksdath, Salazar-Hernandez, Camilo, Perrin, Sally L., Scheer, Kaitlin G., Cildir, Gökhan, Toubia, John, Kristyna Sedivakova, Tea, Melinda N., Sakthi Lenin, Ponthier, Elise, Yeo, Erica C. F., Tergaonkar, Vinay, Poonnoose, Santosh, Ormsby, Rebecca J., Pitson, Stuart M., Brown, Michael P., Ebert, Lisa M., and Gomez, Guillermo A.

Abstract

Additional file 5: Supplementary Table 1 (Related to Fig. 2). Linear regression results for measurements of organoid growth rates from brain organoids grown using different microplate inserts.

Published
2021
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12. Additional file 1 of 3D-printed microplate inserts for long term high-resolution imaging of live brain organoids

Author

Mansilla, Mariana Oksdath, Salazar-Hernandez, Camilo, Perrin, Sally L., Scheer, Kaitlin G., Cildir, Gökhan, Toubia, John, Kristyna Sedivakova, Tea, Melinda N., Sakthi Lenin, Ponthier, Elise, Yeo, Erica C. F., Tergaonkar, Vinay, Poonnoose, Santosh, Ormsby, Rebecca J., Pitson, Stuart M., Brown, Michael P., Ebert, Lisa M., and Gomez, Guillermo A.

Abstract

Additional file 1: Supplementary Figure 1 (related to Fig. 2). Representative sections of cerebral organoids grown on the micro-well inserts and stained with Hoechst 33342 and against cleaved caspase 3. Cleaved caspase 3 is observed in the periphery of cortical structures within organoids, without significant differences across the different experimental conditions (i.e. with or without microplate inserts). Panels were made with cropped images (same size for all time points and conditions). Image’s intensity levels were contracted (same extent for each of the channels across all conditions) from their original 16-bit range to 8-bit RGB for Figure preparation in Adobe Illustrator. Scale Bar = 100 μm.

Published
2021
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13. A drug screening pipeline using 2D and 3D patient-derived in vitro models for pre-clinical analysis of therapy response in glioblastoma

Author

Lenin, Sakthi, Ponthier, Elise, Scheer, Kaitlin G., Yeo, Erica C.F., Tea, Melinda N., Ebert, Lisa M., Mansilla, Mariana Oksdath, Poonnoose, Santosh, Baumgartner, Ulrich, Day, Bryan W., Ormsby, Rebecca J., Pitson, Stuart M., Gomez, Guillermo A., Lenin, Sakthi, Ponthier, Elise, Scheer, Kaitlin G., Yeo, Erica C.F., Tea, Melinda N., Ebert, Lisa M., Mansilla, Mariana Oksdath, Poonnoose, Santosh, Baumgartner, Ulrich, Day, Bryan W., Ormsby, Rebecca J., Pitson, Stuart M., and Gomez, Guillermo A.

Abstract

Glioblastoma is one of the most common and lethal types of primary brain tumor. Despite aggressive treatment with chemotherapy and radiotherapy, tumor recurrence within 6–9 months is common. To overcome this, more effective therapies targeting cancer cell stemness, invasion, metabolism, cell death resistance and the interactions of tumor cells with their surrounding microen-vironment are required. In this study, we performed a systematic review of the molecular mechanisms that drive glioblastoma progression, which led to the identification of 65 drugs/inhibitors that we screened for their efficacy to kill patient-derived glioma stem cells in two dimensional (2D) cul-tures and patient-derived three dimensional (3D) glioblastoma explant organoids (GBOs). From the screening, we found a group of drugs that presented different selectivity on different patient-derived in vitro models. Moreover, we found that Costunolide, a TERT inhibitor, was effective in reducing the cell viability in vitro of both primary tumor models as well as tumor models pre-treated with chemotherapy and radiotherapy. These results present a novel workflow for screening a relatively large groups of drugs, whose results could lead to the identification of more personalized and effective treatment for recurrent glioblastoma.

Published
2021

14. A Drug Screening Pipeline Using 2D and 3D Patient-Derived In Vitro Models for Pre-Clinical Analysis of Therapy Response in Glioblastoma

Author

Lenin, Sakthi, primary, Ponthier, Elise, additional, Scheer, Kaitlin G., additional, Yeo, Erica C. F., additional, Tea, Melinda N., additional, Ebert, Lisa M., additional, Oksdath Mansilla, Mariana, additional, Poonnoose, Santosh, additional, Baumgartner, Ulrich, additional, Day, Bryan W., additional, Ormsby, Rebecca J., additional, Pitson, Stuart M., additional, and Gomez, Guillermo A., additional

Published
2021
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15. Endothelial, pericyte and tumor cell expression in glioblastoma identifies fibroblast activation protein (FAP) as an excellent target for immunotherapy

Author

Ebert, Lisa M., Yu, Wenbo, Gargett, Tessa, Toubia, John, Kollis, Paris M., Tea, Melinda N., Ebert, Brenton W., Bardy, Cedric, van den Hurk, Mark, Bonder, Claudine S., Manavis, Jim, Ensbey, Kathleen S., Oksdath Mansilla, Mariana, Scheer, Kaitlin G., Perrin, Sally L., Ormsby, Rebecca J., Poonnoose, Santosh, Koszyca, Barbara, Pitson, Stuart M., Day, Bryan W., Gomez, Guillermo A., Brown, Michael P., Ebert, Lisa M., Yu, Wenbo, Gargett, Tessa, Toubia, John, Kollis, Paris M., Tea, Melinda N., Ebert, Brenton W., Bardy, Cedric, van den Hurk, Mark, Bonder, Claudine S., Manavis, Jim, Ensbey, Kathleen S., Oksdath Mansilla, Mariana, Scheer, Kaitlin G., Perrin, Sally L., Ormsby, Rebecca J., Poonnoose, Santosh, Koszyca, Barbara, Pitson, Stuart M., Day, Bryan W., Gomez, Guillermo A., and Brown, Michael P.

Abstract

Objectives: Targeted immunotherapies such as chimeric antigen receptor (CAR)-T cells are emerging as attractive treatment options for glioblastoma, but rely on identification of a suitable tumor antigen. We validated a new target antigen for glioblastoma, fibroblast activation protein (FAP), by undertaking a detailed expression study of human samples. Methods: Glioblastoma and normal tissues were assessed using immunostaining, supported by analyses of published transcriptomic datasets. Short-term cultures of glioma neural stem (GNS) cells were compared to cultures of healthy astrocytes and neurons using flow cytometry. Glioblastoma tissues were dissociated and analysed by high-parameter flow cytometry and single-cell transcriptomics (scRNAseq). Results: Compared to normal brain, FAP was overexpressed at the gene and protein level in a large percentage of glioblastoma tissues, with highest levels of expression associated with poorer prognosis. FAP was also overexpressed in several paediatric brain cancers. FAP was commonly expressed by cultured GNS cells but absent from normal neurons and astrocytes. Within glioblastoma tissues, the strongest expression of FAP was around blood vessels. In fact, almost every tumor vessel was highlighted by FAP expression, whereas normal tissue vessels and cultured endothelial cells (ECs) lacked expression. Single-cell analyses of dissociated tumors facilitated a detailed characterisation of the main cellular components of the glioblastoma microenvironment and revealed that vessel-localised FAP is because of expression on both ECs and pericytes. Conclusion: Fibroblast activation protein is expressed by multiple cell types within glioblastoma, highlighting it as an ideal immunotherapy antigen to target destruction of both tumor cells and their supporting vascular network.

Published
2020

16. Endothelial, pericyte and tumor cell expression in glioblastoma identifies fibroblast activation protein (FAP) as an excellent target for immunotherapy

Author

Ebert, Lisa M, primary, Yu, Wenbo, additional, Gargett, Tessa, additional, Toubia, John, additional, Kollis, Paris M, additional, Tea, Melinda N, additional, Ebert, Brenton W, additional, Bardy, Cedric, additional, van den Hurk, Mark, additional, Bonder, Claudine S, additional, Manavis, Jim, additional, Ensbey, Kathleen S, additional, Oksdath Mansilla, Mariana, additional, Scheer, Kaitlin G, additional, Perrin, Sally L, additional, Ormsby, Rebecca J, additional, Poonnoose, Santosh, additional, Koszyca, Barbara, additional, Pitson, Stuart M, additional, Day, Bryan W, additional, Gomez, Guillermo A, additional, and Brown, Michael P, additional

Published
2020
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18. Cytoplasmic dynein regulates the subcellular localization of sphingosine kinase 2 to elicit tumor-suppressive functions in glioblastoma

Author

Neubauer, Heidi A., primary, Tea, Melinda N., additional, Zebol, Julia R., additional, Gliddon, Briony L., additional, Stefanidis, Cassandra, additional, Moretti, Paul A. B., additional, Pitman, Melissa R., additional, Costabile, Maurizio, additional, Kular, Jasreen, additional, Stringer, Brett W., additional, Day, Bryan W., additional, Samuel, Michael S., additional, Bonder, Claudine S., additional, Powell, Jason A., additional, and Pitson, Stuart M., additional

Published
2018
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20. Ceramide-induced integrated stress response overcomes Bcl-2 inhibitor resistance in acute myeloid leukemia

Author

Lewis, Alexander C., Pope, Victoria S., Tea, Melinda N., Li, Manjun, Nwosu, Gus O., Nguyen, Thao M., Wallington-Beddoe, Craig T., Moretti, Paul A.B., Anderson, Dovile, Creek, Darren J., Costabile, Maurizio, Ali, Saira R., Thompson-Peach, Chloe A.L., Dredge, B. Kate, Bert, Andrew G., Goodall, Gregory J., Ekert, Paul G., Brown, Anna L., D'Andrea, Richard, Robinson, Nirmal, Pitman, Melissa R., Thomas, Daniel, Ross, David M., Gliddon, Briony L., Powell, Jason A., and Pitson, Stuart M.

Abstract

Inducing cell death by the sphingolipid ceramide is a potential anti-cancer strategy, but the underlying mechanisms remain poorly defined. Here, we show that triggering accumulation of ceramide in acute myeloid leukaemia (AML) cells by inhibition of sphingosine kinase induces an apoptotic integrated stress response (ISR) through protein kinase R-mediated activation of the master transcription factor ATF4. This leads to transcription of the BH3-only protein, Noxa, and degradation of the pro-survival Mcl-1 protein on which AML cells are highly dependent on for survival. Targeting this novel ISR pathway in combination with the Bcl-2 inhibitor venetoclax synergistically killed primary AML blasts, including those with venetoclax-resistant mutations, as well as immunophenotypic leukemic stem cells, and reduced leukemic engraftment in patient-derived AML xenografts. Collectively, these findings provide mechanistic insight into the anti-cancer effects of ceramide and pre-clinical evidence for new approaches to augment Bcl-2 inhibition in the therapy of AML and other cancers with high Mcl-1 dependency.

Published
2024
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21. Resensitising proteasome inhibitor-resistant myeloma with sphingosine kinase 2 inhibition

Author

Briony L. Gliddon, Craig T. Wallington-Beddoe, Manjun Li, Darren J. Creek, Melissa R. Pitman, Melinda N. Tea, Paul Wang, Dovile Anderson, John Toubia, Melissa K. Bennett, Robert Z. Orlowski, Stuart M. Pitson, Jason A. Powell, Bennett, Melissa K, Li, Manjun, Tea, Melinda N, Pitman, Melissa R, Toubia, John, Wang, Paul PS, Anderson, Dovile, Creek, Darren J, Orlowski, Robert Z, Gliddon, Briony L, Powell, Jason A, Wallington-Beddoe, Craig T, and Pitson, Stuart M

Subjects
Cancer Research, ATF4, activating transcription factor 4, Resistance, Myeloma, medicine.disease_cause, Sphingolipid, Bortezomib, Unfolded protein response, Gene Knockout Techniques, Mice, chemistry.chemical_compound, UPR, unfolded protein response, GSEA, gene set enrichment analysis, immune system diseases, hemic and lymphatic diseases, Enzyme Inhibitors, RC254-282, Mutation, bortezomib, Sphingosine Kinase 2, Neoplasms. Tumors. Oncology. Including cancer and carcinogens, unfolded protein response, BR, bortezomib resistant, Phosphotransferases (Alcohol Group Acceptor), myeloma, S1P, sphingosine 1-phosphate, Multiple Myeloma, Proteasome Inhibitors, medicine.drug, wt, wild-type, Original article, ATF6, activating transcription factor 6, Cell Survival, IRE1, inositol-requiring enzyme 1, Antineoplastic Agents, resistance, ER, endoplasmic reticulum, Structure-Activity Relationship, Cell Line, Tumor, medicine, Animals, Humans, cardiovascular diseases, neoplasms, SK2, sphingosine kinase 2, Dose-Response Relationship, Drug, business.industry, PERK, protein kinase R-like ER kinase, XBP1s, X-box binding protein 1s, Xenograft Model Antitumor Assays, Carfilzomib, CR, carfilzomib resistant, Disease Models, Animal, Proteasome, chemistry, Drug Resistance, Neoplasm, Proteasome inhibitor, Cancer research, sphingolipid, business
Abstract

Refereed/Peer-reviewed The introduction of the proteasome inhibitor bortezomib into treatment regimens for myeloma has led to substantial improvement in patient survival. However, whilst bortezomib elicits initial responses in many myeloma patients, this haematological malignancy remains incurable due to the development of acquired bortezomib resistance. With other patients presenting with disease that is intrinsically bortezomib resistant, it is clear that new therapeutic approaches are desperately required to target bortezomib-resistant myeloma. We have previously shown that targeting sphingolipid metabolism with the sphingosine kinase 2 (SK2) inhibitor K145 in combination with bortezomib induces synergistic death of bortezomib-naive myeloma. In the current study, we have demonstrated that targeting sphingolipid metabolism with K145 synergises with bortezomib and effectively resensitises bortezomib-resistant myeloma to this proteasome inhibitor Notably, these effects were dependent on enhanced activation of the unfolded protein response, and were observed in numerous separate myeloma models that appear to have different mechanisms of bortezomib resistance, including a new bortezomib-resistant myeloma model we describe which possesses a clinically relevant proteasome mutation. Furthermore, K145 also displayed synergy with the next-generation proteasome inhibitor carfilzomib in bortezomib-resistant and carfilzomib-resistant myeloma cells. Together, these findings indicate that targeting sphingolipid metabolism via SK2 inhibition may be effective in combination with a broad spectrum of proteasome inhibitors in the proteasome inhibitor resistant setting, and is an approach worth clinical exploration.

Published
2022

22. Characterising Distinct Migratory Profiles of Infiltrating T-Cell Subsets in Human Glioblastoma

Author

Paris M. Kollis, Lisa M. Ebert, John Toubia, Cameron R. Bastow, Rebecca J. Ormsby, Santosh I. Poonnoose, Sakthi Lenin, Melinda N. Tea, Stuart M. Pitson, Guillermo A. Gomez, Michael P. Brown, Tessa Gargett, Kollis, Paris M, Ebert, Lisa M, Toubia, John, Bastow, Cameron R, Ormsby, Rebecca J, Poonnoose, Santosh I, Lenin, Sakthi, Tea, Melinda N, Pitson, Stuart M, Gomez, Guillermo A, Brown, Michael P, and Gargett, Tessa

Subjects
Integrins, Immunology, T cells, glioblastoma, chemokine receptors, chemokines, migration, Ligands, T-Lymphocyte Subsets, scRNA-seq, integrins, Humans, Immunology and Allergy, Chemokines, Glioblastoma
Abstract

Refereed/Peer-reviewed Glioblastoma is the most common and aggressive form of primary brain cancer, with no improvements in the 5-year survival rate of 4.6% over the past three decades. T-cell-based immunotherapies such as immune-checkpoint inhibitors and chimeric antigen receptor T-cell therapy have prolonged the survival of patients with other cancers and have undergone early-phase clinical evaluation in glioblastoma patients. However, a major challenge for T-cell-based immunotherapy of glioblastoma and other solid cancers is T-cell infiltration into tumours. This process is mediated by chemokine-chemokine receptor and integrin-adhesion molecule interactions, yet the specific nature of the molecules that may facilitate T-cell homing into glioblastoma are unknown. Here, we have characterised chemokine receptor and integrin expression profiles of endogenous glioblastoma-infiltrating T cells, and the chemokine expression profile of glioblastoma-associated cells, by single-cell RNA-sequencing. Subsequently, chemokine receptors and integrins were validated at the protein level to reveal enrichment of receptors CCR2, CCR5, CXCR3, CXCR4, CXCR6, CD49a, and CD49d in glioblastoma-infiltrating T-cell populations relative to T cells in matched patient peripheral blood. Complementary chemokine ligand expression was then validated in glioblastoma biopsies and glioblastoma-derived primary cell cultures. Together, enriched expression of homing receptor-ligand pairs identified in this study implicate a potential role in mediating T-cell infiltration into glioblastoma. Importantly, our data characterising the migratory receptors on endogenous tumour-infiltrating T cells could be exploited to enhance the tumour-homing properties of future T-cell immunotherapies for glioblastoma.

Published
2022
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23. Ceramide-induced integrated stress response overcomes Bcl-2 inhibitor resistance in acute myeloid leukemia

Author

Alexander C. Lewis, Victoria S. Pope, Melinda N. Tea, Manjun Li, Gus O. Nwosu, Thao M. Nguyen, Craig T. Wallington-Beddoe, Paul A. B. Moretti, Dovile Anderson, Darren J. Creek, Maurizio Costabile, Saira R. Ali, Chloe A. L. Thompson-Peach, B. Kate Dredge, Andrew G. Bert, Gregory J. Goodall, Paul G. Ekert, Anna L. Brown, Richard D’Andrea, Nirmal Robinson, Melissa R. Pitman, Daniel Thomas, David M. Ross, Briony L. Gliddon, Jason A. Powell, Stuart M. Pitson, Lewis, Alexander C, Pope, Victoria S, Tea, Melinda N, Li, Manjun, Nwosu, Gus O, Nguyen, Thao M, Wallington-Beddoe, Craig T, Moretti, Paul AB, Costabile, Maurizio, Ali, Saira R, Dredge, B Kate, Bert, Andrew G, Goodall, Gregory J, Brown, Anna L, D'Andrea, Richard, Robinson, Nirmal, Pitman, Melissa R, Ross, David M, Gliddon, Briony L, Powell, Jason A, and Pitson, Stuart M

Subjects
AML, hemic and lymphatic diseases, Immunology, protein kinase R, Cell Biology, Hematology, ceramide, acute myeloid leukemia, integrated stress response, ISR, Biochemistry
Abstract

Inducing cell death by the sphingolipid ceramide is a potential anticancer strategy, but the underlying mechanisms remain poorly defined. In this study, triggering an accumulation of ceramide in acute myeloid leukemia (AML) cells by inhibition of sphingosine kinase induced an apoptotic integrated stress response (ISR) through protein kinase R–mediated activation of the master transcription factor ATF4. This effect led to transcription of the BH3-only protein Noxa and degradation of the prosurvival Mcl-1 protein on which AML cells are highly dependent for survival. Targeting this novel ISR pathway, in combination with the Bcl-2 inhibitor venetoclax, synergistically killed primary AML blasts, including those with venetoclax-resistant mutations, as well as immunophenotypic leukemic stem cells, and reduced leukemic engraftment in patient-derived AML xenografts. Collectively, these findings provide mechanistic insight into the anticancer effects of ceramide and preclinical evidence for new approaches to augment Bcl-2 inhibition in the therapy of AML and other cancers with high Mcl-1 dependency.

Published
2022

24. GD2-targeting CAR-T cells enhanced by transgenic IL-15 expression are an effective and clinically feasible therapy for glioblastoma

Author

Tessa Gargett, Lisa M Ebert, Nga T H Truong, Paris M Kollis, Kristyna Sedivakova, Wenbo Yu, Erica C F Yeo, Nicole L Wittwer, Briony L Gliddon, Melinda N Tea, Rebecca Ormsby, Santosh Poonnoose, Jake Nowicki, Orazio Vittorio, David S Ziegler, Stuart M Pitson, Michael P Brown, Gargett, Tessa, Ebert, Lisa M, Truong, Nga TH, Kollis, Paris M, Sedivakova, Kristyna, Yu, Wenbo, Yeo, Erica CF, Wittwer, Nicole L, Gliddon, Briony L, Tea, Melinda N, Ormsby, Rebecca, Poonnoose, Santosh, Nowicki, Jake, Vittorio, Orazio, Ziegler, David S, Pitson, Stuart M, and Brown, Michael P

Subjects
Interleukin-15, Pharmacology, brain neoplasms, Cancer Research, Receptors, Chimeric Antigen, Brain Neoplasms, T-Lymphocytes, Immunology, receptors, Glioma, adoptive, Xenograft Model Antitumor Assays, Oncology, chimeric antigen, Gangliosides, Humans, Molecular Medicine, Immunology and Allergy, immunotherapy, Glioblastoma, Immune Checkpoint Inhibitors
Abstract

BackgroundAggressive primary brain tumors such as glioblastoma are uniquely challenging to treat. The intracranial location poses barriers to therapy, and the potential for severe toxicity. Effective treatments for primary brain tumors are limited, and 5-year survival rates remain poor. Immune checkpoint inhibitor therapy has transformed treatment of some other cancers but has yet to significantly benefit patients with glioblastoma. Early phase trials of CAR-T cell therapy have demonstrated that this approach is safe and feasible, but with limited evidence of its effectiveness. The choices of appropriate target antigens for CAR-T cell therapy also remain limited.MethodsWe profiled an extensive biobank of patients’ biopsy tissues and patient-derived early passage glioma neural stem cell lines for GD2 expression using immunomicroscopy and flow cytometry. We then employed an approved clinical manufacturing process to make CAR-T cells from peripheral blood of glioblastoma and diffuse midline glioma patients and characterized their phenotype and function in vitro. Finally, we tested intravenously administered CAR-T cells in an aggressive intracranial xenograft model of glioblastoma and used multicolor flow cytometry, multicolor whole-tissue immunofluorescence and next-generation RNA sequencing to uncover markers associated with effective tumor control.ResultsHere we show that the tumor-associated antigen GD2 is highly and consistently expressed in primary glioblastoma tissue removed at surgery. Moreover, despite glioblastoma patients having perturbations in their immune system, highly functional GD2-specific CAR-T cells can be produced from their peripheral T cells using an approved clinical manufacturing process. Finally, after intravenous administration, GD2-CAR-T cells effectively infiltrated the brain and controlled tumor growth in an aggressive orthotopic xenograft model of glioblastoma. Tumor control was further improved using CAR-T cells manufactured with a clinical retroviral vector encoding an IL-15 transgene alongside the GD2-specific CAR. These CAR-T cells achieved a striking 50% complete response rate by bioluminescence imaging in established intracranial tumors. Markers associated with tumor control included those related to T-cell homing, infiltration, and cytotoxicity.ConclusionsTargeting GD2 using a clinically deployed CAR-T therapy has a sound scientific and clinical rationale as a treatment for glioblastoma and other aggressive primary brain tumors.What is already known on this topicGD2 is a tumor antigen of significant interest for targeting immunotherapy. A single preclinical study has shown the effectiveness of GD2-CAR-T cell therapy in an orthotopic xenograft model of diffuse midline glioma. Similarly, there is one previous preclinical study of GD2-CAR-T therapy in a orthotopic glioblastoma xenograft model but tumor control was achieved only following intracranial injection of CAR-T cells. Given that GD2-CAR-T therapy is already being evaluated clinically for other tumor indications, it is important to establish whether there is an acceptable rationale for its use in brain tumors.What this study addsThis is the first description of a GD2-targeted CAR-T cell therapy that shows antitumor effectiveness in a preclinical model of human glioblastoma following intravenous administration. It is also the first study to investigate the potential effects that the immune profile of glioblastoma patients may have on the feasibility of CAR-T cell manufacturing.How this study might affect research, practice, or policyThe results of this study have led to the initiation of an Australian phase 1 clinical trial program aiming to test GD2-specific CAR-T cells for the treatment of childhood and adult primary brain tumors. The study provides valuable insights into the microenvironmental factors that influence the effectiveness of CAR-T cell therapy for this type of tumor, paving the way for further optimization of CAR-T cell technology for treatment of aggressive primary brain tumors such as glioblastoma.

Published
2022
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25. A Drug Screening Pipeline Using 2D and 3D Patient-Derived In Vitro Models for Pre-Clinical Analysis of Therapy Response in Glioblastoma

Author

Lisa M. Ebert, Sakthi Lenin, Santosh Poonnoose, Ulrich Baumgartner, Stuart M. Pitson, Melinda N Tea, Erica C. F. Yeo, Kaitlin G. Scheer, Guillermo A. Gomez, Elise Ponthier, Rebecca J. Ormsby, Bryan W. Day, Mariana Oksdath Mansilla, Lenin, Sakthi, Ponthier, Elise, Scheer, Kaitlin G., Yeo, Erica C.F., Tea, Melinda N., Ebert, Lisa M., Mansilla, Mariana Oksdath, Poonnoose, Santosh, Baumgartner, Ulrich, Day, Bryan W., Ormsby, Rebecca J., Pitson, Stuart M., and Gomez, Guillermo A.

Subjects
therapy resistance, QH301-705.5, medicine.medical_treatment, Brain tumor, Drug Evaluation, Preclinical, Antineoplastic Agents, Catalysis, Article, Inorganic Chemistry, Glioma, medicine, Humans, tumor microenvironment, drug screening, Physical and Theoretical Chemistry, Precision Medicine, Biology (General), Molecular Biology, QD1-999, Spectroscopy, Cells, Cultured, organoids, Chemotherapy, Tumor microenvironment, business.industry, Brain Neoplasms, Organic Chemistry, glioblastoma, General Medicine, personalized medicine, medicine.disease, Primary tumor, Computer Science Applications, Radiation therapy, Chemistry, Cancer cell, Cancer research, Stem cell, business
Abstract

Glioblastoma is one of the most common and lethal types of primary brain tumor. Despite aggressive treatment with chemotherapy and radiotherapy, tumor recurrence within 6–9 months is common. To overcome this, more effective therapies targeting cancer cell stemness, invasion, metabolism, cell death resistance and the interactions of tumor cells with their surrounding microen-vironment are required. In this study, we performed a systematic review of the molecular mechanisms that drive glioblastoma progression, which led to the identification of 65 drugs/inhibitors that we screened for their efficacy to kill patient-derived glioma stem cells in two dimensional (2D) cul-tures and patient-derived three dimensional (3D) glioblastoma explant organoids (GBOs). From the screening, we found a group of drugs that presented different selectivity on different patient-derived in vitro models. Moreover, we found that Costunolide, a TERT inhibitor, was effective in reducing the cell viability in vitro of both primary tumor models as well as tumor models pre-treated with chemotherapy and radiotherapy. These results present a novel workflow for screening a relatively large groups of drugs, whose results could lead to the identification of more personalized and effective treatment for recurrent glioblastoma Refereed/Peer-reviewed

Published
2021

26. Targeting the Sphingolipid System as a Therapeutic Direction for Glioblastoma

Author

Melinda N. Tea, Stuart M. Pitson, Santosh Poonnoose, Tea, Melinda N, Poonnoose, Santosh I, and Pitson, Stuart M

Subjects
0301 basic medicine, Cancer Research, Ceramide, Malignant brain tumor, Cell, Review, lcsh:RC254-282, 03 medical and health sciences, chemistry.chemical_compound, 0302 clinical medicine, Medicine, Sphingosine-1-phosphate, ceramide, sphingosine 1-phosphate, business.industry, urogenital system, Myelin sheaths, glioblastoma, medicine.disease, lcsh:Neoplasms. Tumors. Oncology. Including cancer and carcinogens, Sphingolipid, nervous system diseases, 030104 developmental biology, medicine.anatomical_structure, Oncology, chemistry, 030220 oncology & carcinogenesis, Sphingolipid metabolism, Cancer research, lipids (amino acids, peptides, and proteins), sphingolipid, business, Glioblastoma
Abstract

Glioblastoma (GBM) is the most commonly diagnosed malignant brain tumor in adults. The prognosis for patients with GBM remains poor and largely unchanged over the last 30 years, due to the limitations of existing therapies. Thus, new therapeutic approaches are desperately required. Sphingolipids are highly enriched in the brain, forming the structural components of cell membranes, and are major lipid constituents of the myelin sheaths of nerve axons, as well as playing critical roles in cell signaling. Indeed, a number of sphingolipids elicit a variety of cellular responses involved in the development and progression of GBM. Here, we discuss the role of sphingolipids in the pathobiology of GBM, and how targeting sphingolipid metabolism has emerged as a promising approach for the treatment of GBM. Refereed/Peer-reviewed

Published
2020

27. Cytoplasmic dynein regulates the subcellular localization of sphingosine kinase 2 to elicit tumor-suppressive functions in glioblastoma

Author

Cassandra Stefanidis, Claudine S. Bonder, Briony L. Gliddon, Maurizio Costabile, Melinda N. Tea, Melissa R. Pitman, Julia R. Zebol, Paul A.B. Moretti, Heidi A. Neubauer, Brett W. Stringer, Bryan W. Day, Stuart M. Pitson, Jason A. Powell, Jasreen Kular, Michael S. Samuel, Neubauer, Heidi A, Tea, Melinda N, Zebol, Julia R, Gliddon, Briony L, Stefanidis, Cassandra, Moretti, Paul AB, Pitman, Melissa R, Costabile, Maurizio, Kular, Jasreen, Stringer, Brett W, Day, Bryan W, Samuel, Michael S, Bonder, Claudine S, Powell, Jason A, and Pitson, Stuart M

Subjects
0301 basic medicine, Cytoplasmic Dyneins, Cancer Research, Carcinogenesis, Apoptosis, Biology, Article, Cell membrane, 03 medical and health sciences, chemistry.chemical_compound, Mice, 0302 clinical medicine, Sphingosine, Cell Line, Tumor, Genetics, medicine, Animals, Humans, Genes, Tumor Suppressor, Molecular Biology, Cell Proliferation, Kinase, Cell growth, Endoplasmic reticulum, Cell Membrane, Sphingosine Kinase 2, cell signalling, Subcellular localization, Xenograft Model Antitumor Assays, Cell biology, Gene Expression Regulation, Neoplastic, CNS cancer, Phosphotransferases (Alcohol Group Acceptor), 030104 developmental biology, medicine.anatomical_structure, HEK293 Cells, chemistry, Cytoplasm, 030220 oncology & carcinogenesis, Lysophospholipids, Glioblastoma
Abstract

While the two mammalian sphingosine kinases, SK1 and SK2, both catalyze the generation of pro-survival sphingosine 1-phosphate (S1P), their roles vary dependent on their different subcellular localization. SK1 is generally found in the cytoplasm or at the plasma membrane where it can promote cell proliferation and survival. SK2 can be present at the plasma membrane where it appears to have a similar function to SK1, but can also be localized to the nucleus, endoplasmic reticulum or mitochondria where it mediates cell death. Although SK2 has been implicated in cancer initiation and progression, the mechanisms regulating SK2 subcellular localization are undefined. Here, we report that SK2 interacts with the intermediate chain subunits of the retrograde-directed transport motor complex, cytoplasmic dynein 1 (DYNC1I1 and -2), and we show that this interaction, particularly with DYNC1I1, facilitates the transport of SK2 away from the plasma membrane. DYNC1I1 is dramatically downregulated in patient samples of glioblastoma (GBM), where lower expression of DYNC1I1 correlates with poorer patient survival. Notably, low DYNC1I1 expression in GBM cells coincided with more SK2 localized to the plasma membrane, where it has been recently implicated in oncogenesis. Re-expression of DYNC1I1 reduced plasma membrane-localized SK2 and extracellular S1P formation, and decreased GBM tumor growth and tumor-associated angiogenesis in vivo. Consistent with this, chemical inhibition of SK2 reduced the viability of patient-derived GBM cells in vitro and decreased GBM tumor growth in vivo. Thus, these findings demonstrate a tumor-suppressive function of DYNC1I1, and uncover new mechanistic insights into SK2 regulation which may have implications in targeting this enzyme as a therapeutic strategy in GBM. Refereed/Peer-reviewed

Published
2019

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