Centre for Cancer Research - Research Publications

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Author: Dawson, Sarah-Jane × Author: Dawson, Mark ×

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    Inhibition of the CtBP complex and FBXO11 enhances MHC class II expression and anti-cancer immune responses
    Chan, KL ; Gomez, J ; Cardinez, C ; Kumari, N ; Sparbier, CE ; Lam, EYN ; Yeung, MM ; Garciaz, S ; Kuzich, JA ; Ong, DM ; Brown, FC ; Chan, Y-C ; Vassiliadis, D ; Wainwright, EN ; Motazedian, A ; Gillespie, A ; Fennell, KA ; Lai, J ; House, IG ; Macpherson, L ; Ang, C-S ; Dawson, S-J ; Beavis, PA ; Wei, AH ; Burr, ML ; Dawson, MA (CELL PRESS, 2022-10-10)
    There is increasing recognition of the prognostic significance of tumor cell major histocompatibility complex (MHC) class II expression in anti-cancer immunity. Relapse of acute myeloid leukemia (AML) following allogeneic stem cell transplantation (alloSCT) has recently been linked to MHC class II silencing in leukemic blasts; however, the regulation of MHC class II expression remains incompletely understood. Utilizing unbiased CRISPR-Cas9 screens, we identify that the C-terminal binding protein (CtBP) complex transcriptionally represses MHC class II pathway genes, while the E3 ubiquitin ligase complex component FBXO11 mediates degradation of CIITA, the principal transcription factor regulating MHC class II expression. Targeting these repressive mechanisms selectively induces MHC class II upregulation across a range of AML cell lines. Functionally, MHC class II+ leukemic blasts stimulate antigen-dependent CD4+ T cell activation and potent anti-tumor immune responses, providing fundamental insights into the graft-versus-leukemia effect. These findings establish the rationale for therapeutic strategies aimed at restoring tumor-specific MHC class II expression to salvage AML relapse post-alloSCT and also potentially to enhance immunotherapy outcomes in non-myeloid malignancies.
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    Targeting Menin disrupts the KMT2A/B and polycomb balance to paradoxically activate bivalent genes
    Sparbier, CE ; Gillespie, A ; Gomez, J ; Kumari, N ; Motazedian, A ; Chan, KL ; Bell, CC ; Gilan, O ; Chan, Y-C ; Popp, S ; Gough, DJ ; Eckersley-Maslin, MA ; Dawson, S-J ; Lehner, PJ ; Sutherland, KD ; Ernst, P ; McGeehan, GM ; Lam, EYN ; Burr, ML ; Dawson, MA (NATURE PORTFOLIO, 2023-02)
    Precise control of activating H3K4me3 and repressive H3K27me3 histone modifications at bivalent promoters is essential for normal development and frequently corrupted in cancer. By coupling a cell surface readout of bivalent MHC class I gene expression with whole-genome CRISPR-Cas9 screens, we identify specific roles for MTF2-PRC2.1, PCGF1-PRC1.1 and Menin-KMT2A/B complexes in maintaining bivalency. Genetic loss or pharmacological inhibition of Menin unexpectedly phenocopies the effects of polycomb disruption, resulting in derepression of bivalent genes in both cancer cells and pluripotent stem cells. While Menin and KMT2A/B contribute to H3K4me3 at active genes, a separate Menin-independent function of KMT2A/B maintains H3K4me3 and opposes polycomb-mediated repression at bivalent genes. Release of KMT2A from active genes following Menin targeting alters the balance of polycomb and KMT2A at bivalent genes, facilitating gene activation. This functional partitioning of Menin-KMT2A/B complex components reveals therapeutic opportunities that can be leveraged through inhibition of Menin.
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    Pharmacologic Reduction of Mitochondrial Iron Triggers a Noncanonical BAX/BAK Dependent Cell Death
    Garciaz, S ; Guirguis, AA ; Muller, S ; Brown, FC ; Chan, Y-C ; Motazediani, A ; Rowe, CL ; Kuzich, JA ; Chan, KL ; Tran, K ; Smith, L ; MacPherson, L ; Liddicoat, B ; Lam, EYN ; Caneque, T ; Burr, ML ; Litalien, V ; Pomilio, G ; Poplineau, M ; Duprez, E ; Dawson, S-J ; Ramm, G ; Cox, AG ; Brown, KK ; Huang, DCS ; Wei, AH ; McArthur, K ; Rodriguez, R ; Dawson, MA (AMER ASSOC CANCER RESEARCH, 2022-03)
    UNLABELLED: Cancer cell metabolism is increasingly recognized as providing an exciting therapeutic opportunity. However, a drug that directly couples targeting of a metabolic dependency with the induction of cell death in cancer cells has largely remained elusive. Here we report that the drug-like small-molecule ironomycin reduces the mitochondrial iron load, resulting in the potent disruption of mitochondrial metabolism. Ironomycin promotes the recruitment and activation of BAX/BAK, but the resulting mitochondrial outer membrane permeabilization (MOMP) does not lead to potent activation of the apoptotic caspases, nor is the ensuing cell death prevented by inhibiting the previously established pathways of programmed cell death. Consistent with the fact that ironomycin and BH3 mimetics induce MOMP through independent nonredundant pathways, we find that ironomycin exhibits marked in vitro and in vivo synergy with venetoclax and overcomes venetoclax resistance in primary patient samples. SIGNIFICANCE: Ironomycin couples targeting of cellular metabolism with cell death by reducing mitochondrial iron, resulting in the alteration of mitochondrial metabolism and the activation of BAX/BAK. Ironomycin induces MOMP through a different mechanism to BH3 mimetics, and consequently combination therapy has marked synergy in cancers such as acute myeloid leukemia. This article is highlighted in the In This Issue feature, p. 587.
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    Targeting enhancer switching overcomes non-genetic drug resistance in acute myeloid leukaemia
    Bell, CC ; Fenne, KA ; Chan, Y-C ; Rambow, F ; Yeung, MM ; Vassiliadis, D ; Lara, L ; Yeh, P ; Martelotto, LG ; Rogiers, A ; Kremer, BE ; Barbash, O ; Mohammad, HP ; Johanson, TM ; Burr, ML ; Dhar, A ; Karpinich, N ; Tian, L ; Tyler, DS ; MacPherson, L ; Shi, J ; Pinnawala, N ; Fong, CY ; Papenfuss, AT ; Grimmond, SM ; Dawson, S-J ; Allan, RS ; Kruger, RG ; Vakoc, CR ; Goode, DL ; Naik, SH ; Gilan, O ; Lam, EYN ; Marine, J-C ; Prinjha, RK ; Dawson, MA (NATURE PORTFOLIO, 2019-06-20)
    Non-genetic drug resistance is increasingly recognised in various cancers. Molecular insights into this process are lacking and it is unknown whether stable non-genetic resistance can be overcome. Using single cell RNA-sequencing of paired drug naïve and resistant AML patient samples and cellular barcoding in a unique mouse model of non-genetic resistance, here we demonstrate that transcriptional plasticity drives stable epigenetic resistance. With a CRISPR-Cas9 screen we identify regulators of enhancer function as important modulators of the resistant cell state. We show that inhibition of Lsd1 (Kdm1a) is able to overcome stable epigenetic resistance by facilitating the binding of the pioneer factor, Pu.1 and cofactor, Irf8, to nucleate new enhancers that regulate the expression of key survival genes. This enhancer switching results in the re-distribution of transcriptional co-activators, including Brd4, and provides the opportunity to disable their activity and overcome epigenetic resistance. Together these findings highlight key principles to help counteract non-genetic drug resistance.