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Kelliher, Michelle

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overview	Michelle Kelliher received her B.A. in Biology from Smith College and a M.S. degree in Biology from Yale University. She received her Ph.D. in Immunology from Tufts University Sackler School of Biomedical Sciences and completed her post-doctoral training in the Department of Genetics at Harvard Medical School. In 1998, Dr. Kelliher joined the UMMS Faculty and is currently a Professor in the Molecular, Cellular and Cancer Biology Department. Dr. Kelliher is a Scholar and Stohlman Scholar of the Leukemia and Lymphoma Society of America and a Sidney Kimmel Cancer Scholar. Her research is supported by the NIH (NCI and NIAID), a Hyundai Hope Grant for Pediatric Cancers and an Alex’s Lemonade Stand Innovator Award. Visit the Kelliher Lab website: http://labs.umassmed.edu/kelliherlab/ Mechanisms of Leukemogenesis Genetically engineered mouse model (GEMM) of pediatric T-ALL T cell acute lymphoblastic leukemia (T-ALL) is largely caused by the activation of TAL1, LMO1/2 and the NOTCH1 oncogenes. To model the disease in mice, we ectopically expressed the basic-helix-loop-helix (bHLH) transcription factor TAL1 and its binding partner LMO2 in developing mouse thymocytes. These transgenic mice develop T-ALL that resembles the human disease. We have shown that the DNA binding activity of TAL1 is not required to induce leukemia in mice and demonstrated that E2A or HEB heterozygosity accelerates TAL1-mediated disease (O’Neil et al., 2001; 2004). These studies revealed that TAL1 transforms in part, by interfering with the E47/HEB bHLH heterodimer required for the expression of T cell differentiation genes (Figure?). In collaboration with the Look lab, we performed ChIP-seq analyses that demonstrated that TAL1 also participates in a TAL1-GATA3-RUNX1 autoregulatory loop that induces the expression of stem cell genes such as MYB in leukemia (Sanda et al., 2012). Identifying cooperating oncogenes We have used our GEMM and retroviral insertional mutagenesis (RIM) to identify genes that cooperate with TAL1 to cause leukemia in mice. The RIM screens revealed recurrent retroviral insertions in the Notch1, Myc and Ikaros loci (Sharma et al., 2006). Consistent with these data, NOTCH1 mutations were discovered in 54% of T-ALL patients and shown to develop spontaneously in our TAL1 transgenic mice (O’Neil et al., 2006). These mouse T-ALLs also express dominant-negative forms of Ikaros, indicating that Ikaros acts as a tumor suppressor in the disease. We then discovered that NOTCH1 contributes to leukemogenesis by directly regulating the expression of MYC (Sharma et al., 2006). NOTCH1-MYC axis mediates L-IC activity Leukemia-initiating cells (L-IC) are hypothesized to exhibit extensive proliferative and self-renewal capabilities and thereby mediate relapse. Using our GEMM of T-ALL, we identified the DN3 progenitor population as enriched in L-IC activity. Since NOTCH1 is important in thymic progenitor expansion, we hypothesized that the L-IC may depend on the NOTCH1-MYC pathway for their activity. We found that treatment with a gamma-secretase inhibitor (GSI) which prevents NOTCH1 activation or the bromodomain 4 (BRD4) inhibitor JQ1, which targets MYC, significantly reduces or eliminates the L-IC population and prevents disease initiation (Tatarek et al., 2011; Roderick et al., 2014). These studies suggested that NOTCH and BRD4 inhibition may target the L-IC and prevent relapse. Establishing patient-derived xenografts from relapsed pediatric T-ALL and ETP-ALL patients To translate our findings to the human disease, we generated patient-derived xenografts (PDX) from pediatric T-ALL patients at the time of diagnosis and upon induction failure or relapse. We are using these models to study disease heterogeneity and to test the efficacy of combination targeted therapies. We found that GSI-JQ1 combination therapy was effective in vivo, significantly prolonging survival in PDX models of relapsed pediatric T-ALL (Knoechel et al., 2014). We are one of a few labs world wide that have also successfully generated PDX models from patients with early thymic progenitor (ETP)-ALL, a particularly treatment resistant ALL subtype. In collaboration with the Letai laboratory, we demonstrated that ETP-ALL is uniquely BCL2-dependent and highly sensitive to treatment in vivo with the BCL2 inhibitor ABT-199 (Chongaile et al., 2014). Our current goals are to examine human L-IC activity in these models and to optimize lentiviral-mediated transduction and CRISPR/Cas9 screening in primary human leukemic cells. RIP Kinases in Cell Death and Inflammation My laboratory has had a long-standing interest in RIP Kinases and their role in TNF- and TRIF-dependent signaling. We demonstrated that a RIPK1 deficiency in the mouse results in neonatal lethality due to extensive TNF-induced cell death and inflammation (Kelliher et al., 1998; Cusson et al 2002). We showed that RIPK1 is recruited to the TNF receptor 1 (Tnfr1) and the Toll-like receptors (TLR) 3 and 4 via the adapter TRIF and is stably ubiquitin-modified with K63-linked polyubiquitin chains (Meylan et al., 2004; Lee et al., 2004). We have since established that in addition to TNF-induced apoptosis, RIPK1 regulates a form of programmed necrosis called necroptosis. Necroptosis is thought to require the kinase activities of RIPK1, RIPK3 and MLKL (Figure?) and induces an inflammatory form of cell death. We provide genetic evidence that in the absence of RIPK1, tissues undergo apoptosis and RIPK3-mediated necroptosis. Unlike Ripk1^-/- or Ripk1^-/-Tnfr1^-/- mice, which die during the postnatal period, Ripk1/Tnfr1/Ripk3 triple knock out mice survive to adulthood (Dillon et al., 2014). These in vivo studies demonstrate that RIPK1 is a master regulator of cell death and inflammation. To identify the cell types and tissues that depend on RIPK1 for survival, we developed Ripk1 conditional mice and RIPK1 kinase inactive (D138N) mice. These mouse models allow us to examine the role of RIPK1 in tissue homeostasis and inflammation. Our published work demonstrates critical survival roles for RIPK1 in the intestinal epithelium, keratinocytes and cells of the hematopoietic lineage (Dannappel, et al., 2014;Roderick et al., 2014). We also demonstrated that RIPK1D138N mice are completely protected from TNF-induced hypothermia and shock in vivo (Polykratis et al., 2014). These studies indicate that RIP kinase-dependent necroptotic death mediates shock and may contribute to sepsis, raising the possibility that RIPK inhibitors may have clinical utility in these patients and in chronic inflammatory disease.

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overview

Michelle Kelliher received her B.A. in Biology from Smith College and a M.S. degree in Biology from Yale University. She received her Ph.D. in Immunology from Tufts University Sackler School of Biomedical Sciences and completed her post-doctoral training in the Department of Genetics at Harvard Medical School. In 1998, Dr. Kelliher joined the UMMS Faculty and is currently a Professor in the Molecular, Cellular and Cancer Biology Department. Dr. Kelliher is a Scholar and Stohlman Scholar of the Leukemia and Lymphoma Society of America and a Sidney Kimmel Cancer Scholar. Her research is supported by the NIH (NCI and NIAID), a Hyundai Hope Grant for Pediatric Cancers and an Alex’s Lemonade Stand Innovator Award.

Visit the Kelliher Lab website: http://labs.umassmed.edu/kelliherlab/

Mechanisms of Leukemogenesis

Genetically engineered mouse model (GEMM) of pediatric T-ALL

T cell acute lymphoblastic leukemia (T-ALL) is largely caused by the activation of TAL1, LMO1/2 and the NOTCH1 oncogenes. To model the disease in mice, we ectopically expressed the basic-helix-loop-helix (bHLH) transcription factor TAL1 and its binding partner LMO2 in developing mouse thymocytes. These transgenic mice develop T-ALL that resembles the human disease. We have shown that the DNA binding activity of TAL1 is not required to induce leukemia in mice and demonstrated that E2A or HEB heterozygosity accelerates TAL1-mediated disease (O’Neil et al., 2001; 2004). These studies revealed that TAL1 transforms in part, by interfering with the E47/HEB bHLH heterodimer required for the expression of T cell differentiation genes (Figure?). In collaboration with the Look lab, we performed ChIP-seq analyses that demonstrated that TAL1 also participates in a TAL1-GATA3-RUNX1 autoregulatory loop that induces the expression of stem cell genes such as MYB in leukemia (Sanda et al., 2012).

Identifying cooperating oncogenes

We have used our GEMM and retroviral insertional mutagenesis (RIM) to identify genes that cooperate with TAL1 to cause leukemia in mice. The RIM screens revealed recurrent retroviral insertions in the Notch1, Myc and Ikaros loci (Sharma et al., 2006). Consistent with these data, NOTCH1 mutations were discovered in 54% of T-ALL patients and shown to develop spontaneously in our TAL1 transgenic mice (O’Neil et al., 2006). These mouse T-ALLs also express dominant-negative forms of Ikaros, indicating that Ikaros acts as a tumor suppressor in the disease. We then discovered that NOTCH1 contributes to leukemogenesis by directly regulating the expression of MYC (Sharma et al., 2006).

NOTCH1-MYC axis mediates L-IC activity

Leukemia-initiating cells (L-IC) are hypothesized to exhibit extensive proliferative and self-renewal capabilities and thereby mediate relapse. Using our GEMM of T-ALL, we identified the DN3 progenitor population as enriched in L-IC activity. Since NOTCH1 is important in thymic progenitor expansion, we hypothesized that the L-IC may depend on the NOTCH1-MYC pathway for their activity. We found that treatment with a gamma-secretase inhibitor (GSI) which prevents NOTCH1 activation or the bromodomain 4 (BRD4) inhibitor JQ1, which targets MYC, significantly reduces or eliminates the L-IC population and prevents disease initiation (Tatarek et al., 2011; Roderick et al., 2014). These studies suggested that NOTCH and BRD4 inhibition may target the L-IC and prevent relapse.

Establishing patient-derived xenografts from relapsed pediatric T-ALL and ETP-ALL patients

To translate our findings to the human disease, we generated patient-derived xenografts (PDX) from pediatric T-ALL patients at the time of diagnosis and upon induction failure or relapse. We are using these models to study disease heterogeneity and to test the efficacy of combination targeted therapies. We found that GSI-JQ1 combination therapy was effective in vivo, significantly prolonging survival in PDX models of relapsed pediatric T-ALL (Knoechel et al., 2014).

We are one of a few labs world wide that have also successfully generated PDX models from patients with early thymic progenitor (ETP)-ALL, a particularly treatment resistant ALL subtype. In collaboration with the Letai laboratory, we demonstrated that ETP-ALL is uniquely BCL2-dependent and highly sensitive to treatment in vivo with the BCL2 inhibitor ABT-199 (Chongaile et al., 2014). Our current goals are to examine human L-IC activity in these models and to optimize lentiviral-mediated transduction and CRISPR/Cas9 screening in primary human leukemic cells.

RIP Kinases in Cell Death and Inflammation

My laboratory has had a long-standing interest in RIP Kinases and their role in TNF- and TRIF-dependent signaling. We demonstrated that a RIPK1 deficiency in the mouse results in neonatal lethality due to extensive TNF-induced cell death and inflammation (Kelliher et al., 1998; Cusson et al 2002). We showed that RIPK1 is recruited to the TNF receptor 1 (Tnfr1) and the Toll-like receptors (TLR) 3 and 4 via the adapter TRIF and is stably ubiquitin-modified with K63-linked polyubiquitin chains (Meylan et al., 2004; Lee et al., 2004). We have since established that in addition to TNF-induced apoptosis, RIPK1 regulates a form of programmed necrosis called necroptosis. Necroptosis is thought to require the kinase activities of RIPK1, RIPK3 and MLKL (Figure?) and induces an inflammatory form of cell death. We provide genetic evidence that in the absence of RIPK1, tissues undergo apoptosis and RIPK3-mediated necroptosis. Unlike Ripk1^-/- or Ripk1^-/-Tnfr1^-/- mice, which die during the postnatal period, Ripk1/Tnfr1/Ripk3 triple knock out mice survive to adulthood (Dillon et al., 2014). These in vivo studies demonstrate that RIPK1 is a master regulator of cell death and inflammation.

To identify the cell types and tissues that depend on RIPK1 for survival, we developed Ripk1 conditional mice and RIPK1 kinase inactive (D138N) mice. These mouse models allow us to examine the role of RIPK1 in tissue homeostasis and inflammation. Our published work demonstrates critical survival roles for RIPK1 in the intestinal epithelium, keratinocytes and cells of the hematopoietic lineage (Dannappel, et al., 2014;Roderick et al., 2014). We also demonstrated that RIPK1D138N mice are completely protected from TNF-induced hypothermia and shock in vivo (Polykratis et al., 2014). These studies indicate that RIP kinase-dependent necroptotic death mediates shock and may contribute to sepsis, raising the possibility that RIPK inhibitors may have clinical utility in these patients and in chronic inflammatory disease.

One or more keywords matched the following items that are connected to Kelliher, Michelle

Item Type	Name
Academic Article	Tal-1 induces T cell acute lymphoblastic leukemia accelerated by casein kinase IIalpha.
Academic Article	The death domain kinase RIP mediates the TNF-induced NF-kappaB signal.
Academic Article	The distinct roles of TRAF2 and RIP in IKK activation by TNF-R1: TRAF2 recruits IKK to TNF-R1 while RIP mediates IKK activation.
Academic Article	RIP1 is an essential mediator of Toll-like receptor 3-induced NF-kappa B activation.
Academic Article	TAL1/SCL induces leukemia by inhibiting the transcriptional activity of E47/HEB.
Academic Article	RIP links TLR4 to Akt and is essential for cell survival in response to LPS stimulation.
Academic Article	p16Ink4a or p19Arf loss contributes to Tal1-induced leukemogenesis in mice.
Academic Article	Induction of a chronic myelogenous leukemia-like syndrome in mice with v-abl and BCR/ABL.
Academic Article	Coordinated regulation of Toll-like receptor and NOD2 signaling by K63-linked polyubiquitin chains.
Academic Article	A DNA-binding mutant of TAL1 cooperates with LMO2 to cause T cell leukemia in mice.
Academic Article	Rip1 mediates the Trif-dependent toll-like receptor 3- and 4-induced NF-{kappa}B activation but does not contribute to interferon regulatory factor 3 activation.
Academic Article	NOD2 pathway activation by MDP or Mycobacterium tuberculosis infection involves the stable polyubiquitination of Rip2.
Academic Article	Targeting the Notch1 and mTOR pathways in a mouse T-ALL model.
Academic Article	Increased NOD2-mediated recognition of N-glycolyl muramyl dipeptide.
Academic Article	Notch1 inhibition targets the leukemia-initiating cells in a Tal1/Lmo2 mouse model of T-ALL.
Concept	Immunotherapy
Concept	Enzyme-Linked Immunosorbent Assay
Concept	Immunity, Cellular
Concept	Immunity
Concept	Chromatin Immunoprecipitation
Concept	Models, Immunological
Concept	Immunophenotyping
Concept	Immunoprecipitation
Concept	Immunoenzyme Techniques
Concept	Immunomodulation
Concept	Immunity, Innate
Concept	Adjuvants, Immunologic
Concept	Immunologic Deficiency Syndromes
Concept	Immunotherapy, Adoptive
Concept	Immunoglobulin Class Switching
Concept	Receptors, Immunologic
Concept	Systemic Inflammatory Response Syndrome
Concept	Immunohistochemistry
Concept	Immunoblotting
Academic Article	Activation of NOD receptors by Neisseria gonorrhoeae modulates the innate immune response.
Academic Article	An epigenetic mechanism of resistance to targeted therapy in T cell acute lymphoblastic leukemia.
Academic Article	Caspase-8 and RIP kinases regulate bacteria-induced innate immune responses and cell death.
Academic Article	Cutting edge: RIPK1 Kinase inactive mice are viable and protected from TNF-induced necroptosis in vivo.
Academic Article	NEMO Prevents Steatohepatitis and Hepatocellular Carcinoma by Inhibiting RIPK1 Kinase Activity-Mediated Hepatocyte Apoptosis.
Academic Article	NEMO Prevents RIP Kinase 1-Mediated Epithelial Cell Death and Chronic Intestinal Inflammation by NF-?B-Dependent and -Independent Functions.
Academic Article	RIPK1 and RIPK3 Kinases Promote Cell-Death-Independent Inflammation by Toll-like Receptor 4.
Academic Article	Kinase Activities of RIPK1 and RIPK3 Can Direct IFN-? Synthesis Induced by Lipopolysaccharide.
Academic Article	RIP kinase 1-dependent endothelial necroptosis underlies systemic inflammatory response syndrome.
Academic Article	Dendritic Cell RIPK1 Maintains Immune Homeostasis by Preventing Inflammation and Autoimmunity.
Academic Article	Correction: Dendritic Cell RIPK1 Maintains Immune Homeostasis by Preventing Inflammation and Autoimmunity.
Academic Article	Connecting immune deficiency and inflammation.
Academic Article	NOTCH Signaling in T-Cell-Mediated Anti-Tumor Immunity and T-Cell-Based Immunotherapies.
Academic Article	Ptpn6 inhibits caspase-8- and Ripk3/Mlkl-dependent inflammation.
Academic Article	TBK1 inhibition unleashes RIPK1, resensitizing tumors to immunotherapy.

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