• 文献标题:   Differential genotoxic and epigenotoxic effects of graphene family nanomaterials (GFNs) in human bronchial epithelial cells
  • 文献类型:   Article
  • 作  者:   CHATTERJEE N, YANG J, CHOI J
  • 作者关键词:   graphene family nanomaterials gfns, dna damagerepair, global dna methylation, dna methyltransferases dnmts, dna demethylases tets
  • 出版物名称:   MUTATION RESEARCHGENETIC TOXICOLOGY ENVIRONMENTAL MUTAGENESIS
  • ISSN:   1383-5718 EI 1879-3592
  • 通讯作者地址:   Univ Seoul
  • 被引频次:   17
  • DOI:   10.1016/j.mrgentox.2016.01.006
  • 出版年:   2016

▎ 摘  要

The widespread applications of graphene family nanomaterials (GFNs) raised the considerable concern over human health and environment. The cyto-genotoxic potentiality of GFNs has attracted much more attention, albeit the potential effects on the cellular epigenome remain largely unknown. The effects of GFNs on cellular genome were evaluated with single and double stranded DNA damage and DNA repair gene expressions while the effects on epigenome was accomplished by addressing the global DNA methylation and expression of DNA methylation machineries at non-cytotoxic to moderately cytotoxic doses in in vitro system. We used five different representatives of GFNs-pristine (GNP-Prist), carboxylated (GNP-COOH) and aminated (GNP-NH2) graphene nanoplatelets as well as single layer (SLGO) and few layer (FLGO) graphene oxide. The order of single stranded DNA damage was observed as GNP-Prist >= GNP-COOH > GNP-NH2 >= FLGO > SLGO at 10 mg/L and marked dose dependency was found in SLGO. The GFNs possibly caused genotoxicity by affecting nucleotide excision repair and non-homologus end joining repair systems. Besides, dose dependent increase in global DNA methylation (hypermethylation) were observed in SLGO/FLGO exposure and conversely, GNPs.treatment caused hypomethylation following the order as GNP-COOH > GNP-NH2 >= GNP-Prist. The decrements of DNA methyltransferase (DNMT3B gene) and methyl-CpG binding domain protein (MBD1) genes were probably the cause of global hypomethylation induced by GNPs. Conversely, the de novo methylation through the up-regulation of DNMT3B and MBD1 genes gave rise to the global DNA hypermethylation in SLGO/FLGO treated cells. In general, the GFNs induced genotoxicity and alterations of global DNA methylation exhibited compounds type specificity with differential physico-chemical properties. Taken together, our study suggests that the GFNs could cause more subtle changes in gene expression programming by modulating DNA methylation status and this information would be helpful for their prospective use in biomedical field. (C) 2016 Elsevier B.V. All rights reserved.