期刊
TOXICOLOGICAL SCIENCES
卷 127, 期 1, 页码 246-255出版社
OXFORD UNIV PRESS
DOI: 10.1093/toxsci/kfs070
关键词
Nrf2; protein translation; ribosomes; subcellular relocalization
类别
资金
- National Institute of Health [T32 ES007091, R01 HL 076530, R01 HL089958, R21ES017473]
- Arizona Biomedical Research Commission
Histone deacetylase 6 (HDAC6) is known as a cytoplasmic enzyme that regulates cell migration, cell adhesion, and degradation of misfolded proteins by deacetylating substrates such as a-tubulin and Hsp90. When HaCaT keratinocytes were exposed to 1-200 mu M sodium arsenite, we observed perinuclear localization of HDAC6 within 30 min. Although the overall level of HDAC6 protein did not change, sodium arsenite caused an increase of HDAC6 in ribosomal fractions. Separation of ribosomal subunits versus intact ribosomes or polysomes indicated that HDAC6 was mainly detected in 40/43S fractions containing the small ribosomal subunit in untreated cells but was associated with 40/43S and 60/80S ribosomal fractions in arsenite-treated cells. Immunocytochemistry studies revealed that arsenite caused colocalization of HDAC6 with the ribosomal large and small subunit protein L36a and S6. Both L36a and S6 were detected in the immunocomplex of HDAC6 isolated from arsenite-treated cells. The observed physical interaction of HDAC6 with ribosomes pointed to a role of HDAC6 in stress-induced protein translation. Among arsenite stress-induced proteins, de novo Nrf2 protein translation was inhibited by Tubastatin A. These data demonstrate that HDAC6 was recruited to ribosomes, physically interacted with ribosomal proteins, and regulated de nova protein translation in keratinocytes responding to arsenite stress.
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