Targeting of acute myeloid leukemia in vitro and in vivo with an anti-CD123 mAb engineered for optimal ADCC

Busfield, Samantha J.; Biondo, Mark; Wong, Margaret G.; Ramshaw, Hayley S.; Lee, E M; Ghosh, Souravi; Braley, Hal; Panousis, Con; Roberts, Andrew W.; He, Simon; Thomas, Daniel; Fabri, Louis; Vairo, Gino; Lock, Richard B.; Lopez, Angel F.; Nash, Andrew D.

doi:10.1038/leu.2014.128

Cited by 123 publications

(101 citation statements)

References 48 publications

(43 reference statements)

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“…A loose correlation between these two properties was observed for bulk AML cells (Figure 3), and similar correlations have been reported for the CD33-specific BiTE AMG330, 9 the CD123 antibody Talacotuzumab (CSL 362), 48,49 and the CD3 x CD123 DART agent MGD006. 56 While the target antigen density likely dictates the strength of binding of these agents to the target cells and the subsequent engagement of killer cells, it is unlikely that binding strength alone will translate 1:1 into an enhanced lytic activity.…”

Section: Discussionsupporting

confidence: 81%

Dual-targeting triplebody 33-16-123 (SPM-2) mediates effective redirected lysis of primary blasts from patients with a broad range of AML subtypes in combination with natural killer cells

et al. 2018

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A number of agents designed for immunotherapy of Acute Myeloid Leukemia (AML) are in preclinical and early clinical development. Most of them target a single antigen on the surface of AML cells. Here we describe the development and key biological properties of a tri-specific agent, the dual-targeting triplebody SPM-2, with binding sites for target antigens CD33 and CD123, and for CD16 to engage NK cells as cytolytic effectors. Primary blasts of nearly all AML patients carry at least one of these target antigens and the pair is particularly promising for the elimination of blasts and leukemia stem cells (LSCs) from a majority of AML patients by dual-targeting agents. The cytolytic activity of NK cells mediated by SPM-2 was analyzed in vitro for primary leukemic cells from 29 patients with a broad range of AML-subtypes. Blasts from all 29 patients, including patients with genomic alterations associated with an unfavorable genetic subtype, were lysed at nanomolar concentrations of SPM-2. Maximum susceptibility was observed for cells with a combined density of CD33 and CD123 above 10,000 copies/cell. Cell populations enriched for AML-LSCs (CD34pos and CD34pos CD38neg cells) from 2 AML patients carried an increased combined antigen density and were lysed at correspondingly lower concentrations of SPM-2 than unsorted blasts. These initial findings raise the expectation that SPM-2 may also be capable of eliminating AML-LSCs and thus of prolonging survival. In the future, patients with a broad range of AML subtypes may benefit from treatment with SPM-2.

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Section: Discussionsupporting

confidence: 81%

Dual-targeting triplebody 33-16-123 (SPM-2) mediates effective redirected lysis of primary blasts from patients with a broad range of AML subtypes in combination with natural killer cells

et al. 2018

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“…Recently, there have been increasing efforts to identify molecular aberrations that could serve as pharmacologic targets within AML and MDS stem cell compartments. [10][11][12][13][14][15][16] Resulting therapies have shown promising effects in preclinical studies, 17,18 but further work will be necessary to identify therapeutic targets against preleukemic stem cells that would lead to long-term remission and prevention of relapse in AML and MDS.…”

Section: Introductionmentioning

confidence: 99%

IL8-CXCR2 pathway inhibition as a therapeutic strategy against MDS and AML stem cells

Schinke

Giricz

et al. 2015

Blood

146

125

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“…IFN␥-mediated CD38 Up-regulation Requires p38, NF-B, and JAK/STAT-Previous studies have shown increased expression of CD38 by IFN␥ in chronic lymphocytic leukemia to be JAK/STAT and T-bet-dependent (20). To determine which downstream signaling pathways were required for the up-regulation of CD38 seen with IFN␥ treatment, primary AML apheresis samples were pretreated with inhibitors for ERK, PI3K, p38 MAPK, JAK/STAT, and NF-B.…”

Section: Ifn␥ Increases Fc␥ri Expression and Phagocytic Ability Inmentioning

confidence: 99%

“…The targeting of Fc␥RI has similarly been proposed, especially after the finding that IFN␥ could increase the expression of the high affinity Fc␥ receptor, Fc␥RI (16 -19). Recently, a study was completed using a monoclonal antibody to CD123 that has been humanized, affinity-matured, and Fc-engineered for increased affinity toward CD16 (Fc␥RIIIa), which showed an effect against AML both in vitro and in vivo in an environment with adequate NK cell function (20).…”

mentioning

confidence: 99%

Interferon-γ Promotes Antibody-mediated Fratricide of Acute Myeloid Leukemia Cells

Fatehchand¹,

McMichael²,

Reader³

et al. 2016

Journal of Biological Chemistry

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Edited by Peter CresswellAcute myeloid leukemia (AML) is characterized by the proliferation of immature myeloid lineage blasts. Due to its heterogeneity and to the high rate of acquired drug resistance and relapse, new treatment strategies are needed. Here, we demonstrate that IFN␥ promotes AML blasts to act as effector cells within the context of antibody therapy. Treatment with IFN␥ drove AML blasts toward a more differentiated state, wherein they showed increased expression of the M1-related markers HLA-DR and CD86, as well as of Fc␥RI, which mediates effector responses to therapeutic antibodies. Importantly, IFN␥ was able to up-regulate CD38, the target of the therapeutic antibody daratumumab. Because the antigen (CD38) and effector receptor (Fc␥RI) were both simultaneously up-regulated on the AML blasts, we tested whether IFN␥ treatment of the AML cell lines THP-1 and MV4-11 could stimulate them to target one another after the addition of daratumumab. Results showed that IFN␥ significantly increased daratumumab-mediated cytotoxicity, as measured both by 51 Cr release and lactate dehydrogenase release assays. We also found that the combination of IFN␥ and activation of Fc␥R led to the release of granzyme B by AML cells. Finally, using a murine NSG model of subcutaneous AML, we found that treatment with IFN␥ plus daratumumab significantly attenuated tumor growth. Taken together, these studies show a novel mechanism of daratumumab-mediated killing and a possible new therapeutic strategy for AML.

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Targeting of acute myeloid leukemia in vitro and in vivo with an anti-CD123 mAb engineered for optimal ADCC

Cited by 123 publications

References 48 publications

Dual-targeting triplebody 33-16-123 (SPM-2) mediates effective redirected lysis of primary blasts from patients with a broad range of AML subtypes in combination with natural killer cells

Dual-targeting triplebody 33-16-123 (SPM-2) mediates effective redirected lysis of primary blasts from patients with a broad range of AML subtypes in combination with natural killer cells

IL8-CXCR2 pathway inhibition as a therapeutic strategy against MDS and AML stem cells

Interferon-γ Promotes Antibody-mediated Fratricide of Acute Myeloid Leukemia Cells

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