Literature DB >> 29308322

Impaired NK cell recognition of vemurafenib-treated melanoma cells is overcome by simultaneous application of histone deacetylase inhibitors.

Sheila López-Cobo1, Natalia Pieper2, Carmen Campos-Silva1, Eva M García-Cuesta1, Hugh T Reyburn1, Annette Paschen2, Mar Valés-Gómez1.   

Abstract

Therapy of metastatic melanoma advanced recently with the clinical implementation of signalling pathway inhibitors, such as vemurafenib, specifically targeting mutant BRAFV600E. In general, patients experience remarkable clinical responses under BRAF inhibitor (BRAFi) treatment but eventually progress within 6-8 months due to resistance development. Responding metastases show an increased immune cell infiltrate, including also NK cells, that, however, is no longer detectable in BRAFi-resistant lesions, suggesting NK cell activity should be exploited to prevent disease progression. Here, we examined the effects of BRAFi on the expression of ligands targeting activating NK cells receptors immediately after treatment onset, prior to resistance development. We demonstrate that BRAFV600E mutant melanoma cells cultured in the presence of vemurafenib, strongly decreased surface expression of ligands for NK activating receptors including the NKG2D-ligand, MICA, and the DNAM-1 ligand, CD155, and became significantly less susceptible to NK cell attack. NKG2D-ligand protein downregulation was due to a significant decrease in mRNA levels, already detectable 24 h after drug treatment. Interestingly, vemurafenib-induced MICA downregulation could be counteracted by treatment of melanoma cells with the histone deacetylase (HDAC) inhibitor (HDACi) sodium butyrate, that also upregulated the DNAM1-ligand, Nectin-2. HDACi treatment enhanced surface expression of NKG2D-ligands in the presence of BRAFi, accompanied by recovery of NK cell recognition, but only upon simultaneous drug application. These results suggest that co-administration of BRAFi and HDAC inhibitors as well as having direct effects on melanoma cell survival, could also synergise to improve NK cell recognition and avoid tumour immune evasion.

Entities:  

Keywords:  BRAF inhibitors; DNAM1; HDAC inhibitor; NK cell; NKG2D; combination therapy; melanoma

Year:  2017        PMID: 29308322      PMCID: PMC5749663          DOI: 10.1080/2162402X.2017.1392426

Source DB:  PubMed          Journal:  Oncoimmunology        ISSN: 2162-4011            Impact factor:   8.110


  55 in total

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Review 5.  HLA and melanoma: multiple alterations in HLA class I and II expression in human melanoma cell lines from ESTDAB cell bank.

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10.  NKG2D is a Key Receptor for Recognition of Bladder Cancer Cells by IL-2-Activated NK Cells and BCG Promotes NK Cell Activation.

Authors:  Eva María García-Cuesta; Sheila López-Cobo; Mario Álvarez-Maestro; Gloria Esteso; Gema Romera-Cárdenas; Mercedes Rey; Robin L Cassady-Cain; Ana Linares; Alejandro Valés-Gómez; Hugh Thomson Reyburn; Luis Martínez-Piñeiro; Mar Valés-Gómez
Journal:  Front Immunol       Date:  2015-06-08       Impact factor: 7.561

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1.  Astragaloside IV suppresses post-ischemic natural killer cell infiltration and activation in the brain: involvement of histone deacetylase inhibition.

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2.  HO-1 Limits the Efficacy of Vemurafenib/PLX4032 in BRAFV600E Mutated Melanoma Cells Adapted to Physiological Normoxia or Hypoxia.

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6.  A TLR7 agonist strengthens T and NK cell function during BRAF-targeted therapy in a preclinical melanoma model.

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7.  Immunoassays for scarce tumour-antigens in exosomes: detection of the human NKG2D-Ligand, MICA, in tetraspanin-containing nanovesicles from melanoma.

Authors:  Sheila López-Cobo; Carmen Campos-Silva; Amanda Moyano; Myriam Oliveira-Rodríguez; Annette Paschen; María Yáñez-Mó; María Carmen Blanco-López; Mar Valés-Gómez
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