Medical Biology - Research Publications

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Author: Herold, Marco × Author: Kueh, Andrew × End date: 2019 × Start date: 2010 ×

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Now showing 1 - 7 of 7
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    A non-canonical function of Ezh2 preserves immune homeostasis
    Vasanthakumar, A ; Xu, D ; Lun, ATL ; Kueh, AJ ; van Gisbergen, KPJM ; Iannarella, N ; Li, X ; Yu, L ; Wang, D ; Williams, BRG ; Lee, SCW ; Majewski, IJ ; Godfrey, DI ; Smyth, GK ; Alexander, WS ; Herold, MJ ; Kallies, A ; Nutt, SL ; Allan, RS (WILEY, 2017-04)
    Enhancer of zeste 2 (Ezh2) mainly methylates lysine 27 of histone-H3 (H3K27me3) as part of the polycomb repressive complex 2 (PRC2) together with Suz12 and Eed. However, Ezh2 can also modify non-histone substrates, although it is unclear whether this mechanism has a role during development. Here, we present evidence for a chromatin-independent role of Ezh2 during T-cell development and immune homeostasis. T-cell-specific depletion of Ezh2 induces a pronounced expansion of natural killer T (NKT) cells, although Ezh2-deficient T cells maintain normal levels of H3K27me3. In contrast, removal of Suz12 or Eed destabilizes canonical PRC2 function and ablates NKT cell development completely. We further show that Ezh2 directly methylates the NKT cell lineage defining transcription factor PLZF, leading to its ubiquitination and subsequent degradation. Sustained PLZF expression in Ezh2-deficient mice is associated with the expansion of a subset of NKT cells that cause immune perturbation. Taken together, we have identified a chromatin-independent function of Ezh2 that impacts on the development of the immune system.
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    CRISPR/Cas9: A tool for immunological research
    Hochheiser, K ; Kueh, AJ ; Gebhardt, T ; Herold, MJ (WILEY, 2018-04)
    The CRISPR/Cas9-system was originally identified as part of the adaptive immune system in bacteria and has since been adapted for the genetic manipulation of eukaryotic cells. The technique is of particular value for biomedical sciences, as it enables the genetic manipulation of cell lines and primary cells as well as whole organisms with unprecedented ease and efficiency. Furthermore, the CRISPR/Cas9-technology has the potential for future therapeutic applications in the clinic. Here, we discuss the use of CRISPR/Cas9 for the genetic modification of haematopoietic cells and the generation of mouse models for immunological research. Additionally, we explain how the technique can be applied as a screening-tool to identify genes involved in different immunological processes. Moreover, we will talk about recent extensions of using the CRISPR/Cas9 technology, such as a transcriptional activator or repressor. Finally, we discuss the first clinical trials that use CRISPR/Cas9 and discuss potential future applications.
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    A point mutation in the Ncr1 signal peptide impairs the development of innate lymphoid cell subsets
    Almeida, FF ; Tognarelli, S ; Marcais, A ; Kueh, AJ ; Friede, ME ; Liao, Y ; Willis, SN ; Luong, K ; Faure, F ; Mercier, FE ; Galluso, J ; Firth, M ; Narni-Mancinelli, E ; Rais, B ; Scadden, DT ; Spallotta, F ; Weil, S ; Giannattasio, A ; Kalensee, F ; Zoeller, T ; Huntington, ND ; Schleicher, U ; Chiocchetti, AG ; Ugolini, S ; Herold, MJ ; Shi, W ; Koch, J ; Steinle, A ; Vivier, E ; Walzer, T ; Belz, GT ; Ullrich, E (TAYLOR & FRANCIS INC, 2018)
    NKp46 (CD335) is a surface receptor shared by both human and mouse natural killer (NK) cells and innate lymphoid cells (ILCs) that transduces activating signals necessary to eliminate virus-infected cells and tumors. Here, we describe a spontaneous point mutation of cysteine to arginine (C14R) in the signal peptide of the NKp46 protein in congenic Ly5.1 mice and the newly generated NCRB6C14R strain. Ly5.1C14R NK cells expressed similar levels of Ncr1 mRNA as C57BL/6, but showed impaired surface NKp46 and reduced ability to control melanoma tumors in vivo. Expression of the mutant NKp46C14R in 293T cells showed that NKp46 protein trafficking to the cell surface was compromised. Although Ly5.1C14R mice had normal number of NK cells, they showed an increased number of early maturation stage NK cells. CD49a+ILC1s were also increased but these cells lacked the expression of TRAIL. ILC3s that expressed NKp46 were not detectable and were not apparent when examined by T-bet expression. Thus, the C14R mutation reveals that NKp46 is important for NK cell and ILC differentiation, maturation and function. Significance Innate lymphoid cells (ILCs) play important roles in immune protection. Various subsets of ILCs express the activating receptor NKp46 which is capable of recognizing pathogen derived and tumor ligands and is necessary for immune protection. Here, we describe a spontaneous point mutation in the signal peptide of the NKp46 protein in congenic Ly5.1 mice which are widely used for tracking cells in vivo. This Ncr1 C14R mutation impairs NKp46 surface expression resulting in destabilization of Ncr1 and accumulation of NKp46 in the endoplasmic reticulum. Loss of stable NKp46 expression impaired the maturation of NKp46+ ILCs and altered the expression of TRAIL and T-bet in ILC1 and ILC3, respectively.
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    Mining the Plasma Cell Transcriptome for Novel Cell Surface Proteins
    Trezise, S ; Karnowski, A ; Fedele, PL ; Mithraprabhu, S ; Liao, Y ; D'Costa, K ; Kueh, AJ ; Hardy, MP ; Owczarek, CM ; Herold, MJ ; Spencer, A ; Shi, W ; Willis, SN ; Nutt, SL ; Corcoran, LM (MDPI AG, 2018-08-01)
    Antibody Secreting Cells (ASCs) are a fundamental component of humoral immunity, however, deregulated or excessive antibody production contributes to the pathology of autoimmune diseases, while transformation of ASCs results in the malignancy Multiple Myeloma (MM). Despite substantial recent improvements in treating these conditions, there is as yet no widely used ASC-specific therapeutic approach, highlighting a critical need to identify novel methods of targeting normal and malignant ASCs. Surface molecules specifically expressed by the target cell population represent ideal candidates for a monoclonal antibody-based therapy. By interrogating the ASC gene signature that we previously defined we identified three surface proteins, Plpp5, Clptm1l and Itm2c, which represent potential targets for novel MM treatments. Plpp5, Clptm1l and Itm2c are highly and selectively expressed by mouse and human ASCs as well as MM cells. To investigate the function of these proteins within the humoral immune system we have generated three novel mouse strains, each carrying a loss-of-function mutation in either Plpp5, Clptm1l or Itm2c. Through analysis of these novel strains, we have shown that Plpp5, Clptm1l and Itm2c are dispensable for the development, maturation and differentiation of B-lymphocytes, and for the production of antibodies by ASCs. As adult mice lacking either protein showed no apparent disease phenotypes, it is likely that targeting these molecules on ASCs will have minimal on-target adverse effects.
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    Male sterility in Mcl-1-flox mice is not due to enhanced Mcl1 protein stability
    Ah-Cann, C ; Tailler, M ; Kueh, AJ ; Herold, MJ ; Opferman, JT ; Asselin-Labat, M-L ; Bouillet, P (NATURE PUBLISHING GROUP, 2016-12)
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    VDAC2 enables BAX to mediate apoptosis and limit tumor development
    Chin, HS ; Li, MX ; Tan, IKL ; Ninnis, RL ; Reljic, B ; Scicluna, K ; Dagley, LF ; Sandow, JJ ; Kelly, GL ; Samson, AL ; Chappaz, S ; Khaw, SL ; Chang, C ; Morokoff, A ; Brinkmann, K ; Webb, A ; Hockings, C ; Hall, CM ; Kueh, AJ ; Ryan, MT ; Kluck, RM ; Bouillet, P ; Herold, MJ ; Gray, DHD ; Huang, DCS ; van Delft, MF ; Dewson, G (NATURE PUBLISHING GROUP, 2018-11-26)
    Intrinsic apoptosis is critical to prevent tumor formation and is engaged by many anti-cancer agents to eliminate tumor cells. BAX and BAK, the two essential mediators of apoptosis, are thought to be regulated through similar mechanisms and act redundantly to drive apoptotic cell death. From an unbiased genome-wide CRISPR/Cas9 screen, we identified VDAC2 (voltage-dependent anion channel 2) as important for BAX, but not BAK, to function. Genetic deletion of VDAC2 abrogated the association of BAX and BAK with mitochondrial complexes containing VDAC1, VDAC2, and VDAC3, but only inhibited BAX apoptotic function. Deleting VDAC2 phenocopied the loss of BAX in impairing both the killing of tumor cells by anti-cancer agents and the ability to suppress tumor formation. Together, our studies show that efficient BAX-mediated apoptosis depends on VDAC2, and reveal a striking difference in how BAX and BAK are functionally impacted by their interactions with VDAC2.