Int6 regulates both proteasomal degradation and translation initiation and is critical for proper formation of acini by human mammary epithelium: Dual regulation of protein synthesis and degradation by Int6

INT6/EIF3E has been implicated in breast tumorigenesis, but its functional activities remain poorly defined. We found that repressing INT6 expression induced transformed properties in normal human mammary epithelium (MCF10A); in contrast, Int6 silencing induced apoptosis in HeLa cells. As in yeast,...

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Autores principales: Suo, Jinfeng, Snider, Sarah J., Mills, Gordon B., Creighton, Chad J., Chen, Albert, Schiff, Rachel, Lloyd, Richard E., Chang, Eric C.
Formato: Texto
Lenguaje:English
Publicado: 2010
Materias:
Article
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC3017639/
https://www.ncbi.nlm.nih.gov/pubmed/20890303
http://dx.doi.org/10.1038/onc.2010.445
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author Suo, Jinfeng
Snider, Sarah J.
Mills, Gordon B.
Creighton, Chad J.
Chen, Albert
Schiff, Rachel
Lloyd, Richard E.
Chang, Eric C.
author_facet Suo, Jinfeng
Snider, Sarah J.
Mills, Gordon B.
Creighton, Chad J.
Chen, Albert
Schiff, Rachel
Lloyd, Richard E.
Chang, Eric C.
author_sort Suo, Jinfeng
collection PubMed
description INT6/EIF3E has been implicated in breast tumorigenesis, but its functional activities remain poorly defined. We found that repressing INT6 expression induced transformed properties in normal human mammary epithelium (MCF10A); in contrast, Int6 silencing induced apoptosis in HeLa cells. As in yeast, Int6 in human cells was required for assembly of active proteasomes. A reverse phase protein array screen identified SRC3/AIB1 as one oncoprotein whose level and stability increased when Int6 was silenced in MCF10A cells. Our data further show that Int6 binds SRC3 and its ubiquitin ligase Fbw7, thus perhaps mediating the interaction between SRC3-Fbw7 and proteasomes. Consistent with this, Int6 silencing did not increase SRC3 levels in HeLa cells, which have low Fbw7 levels. Surprisingly, however, polyubiquitylated proteins do not accumulate or may even decrease in Int6-silenced cells that contain defective proteasomes. Considering that decreased ubiquitin might explain this observation and that Int6 might control ubiquitin levels in its role as a subunit of eIF3 (eukaryote translation initiation factor), we found that silencing Int6 reduced monoubiquitin protein levels, which correlated with a shift of ubiquitin mRNAs from larger polysomes to non-translating ribosomes. In contrast, levels of many housekeeping proteins did not change. This apparent reduction in the translation of ubiquitin genes correlated with a modest reduction in protein synthesis rate and formation of large polysomes. To further determine whether Int6 can selectively control translation, we analyzed translation of different 5′-UTR reporters and found that indeed, loss of Int6 had differential effects on these reporters. Together the data suggest that Int6 depletion blocks ubiquitin-dependent proteolysis by decreasing both ubiquitin levels and the assembly of functional proteasome machinery, leading to accumulation of oncoproteins such as SRC3 that can transform mammary epithelium. Our data also raise the possibility that Int6 can further fine-tune protein levels by selectively controlling translation of specific mRNAs.
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spelling pubmed-30176392011-08-10 Int6 regulates both proteasomal degradation and translation initiation and is critical for proper formation of acini by human mammary epithelium: Dual regulation of protein synthesis and degradation by Int6 Suo, Jinfeng Snider, Sarah J. Mills, Gordon B. Creighton, Chad J. Chen, Albert Schiff, Rachel Lloyd, Richard E. Chang, Eric C. Oncogene Article INT6/EIF3E has been implicated in breast tumorigenesis, but its functional activities remain poorly defined. We found that repressing INT6 expression induced transformed properties in normal human mammary epithelium (MCF10A); in contrast, Int6 silencing induced apoptosis in HeLa cells. As in yeast, Int6 in human cells was required for assembly of active proteasomes. A reverse phase protein array screen identified SRC3/AIB1 as one oncoprotein whose level and stability increased when Int6 was silenced in MCF10A cells. Our data further show that Int6 binds SRC3 and its ubiquitin ligase Fbw7, thus perhaps mediating the interaction between SRC3-Fbw7 and proteasomes. Consistent with this, Int6 silencing did not increase SRC3 levels in HeLa cells, which have low Fbw7 levels. Surprisingly, however, polyubiquitylated proteins do not accumulate or may even decrease in Int6-silenced cells that contain defective proteasomes. Considering that decreased ubiquitin might explain this observation and that Int6 might control ubiquitin levels in its role as a subunit of eIF3 (eukaryote translation initiation factor), we found that silencing Int6 reduced monoubiquitin protein levels, which correlated with a shift of ubiquitin mRNAs from larger polysomes to non-translating ribosomes. In contrast, levels of many housekeeping proteins did not change. This apparent reduction in the translation of ubiquitin genes correlated with a modest reduction in protein synthesis rate and formation of large polysomes. To further determine whether Int6 can selectively control translation, we analyzed translation of different 5′-UTR reporters and found that indeed, loss of Int6 had differential effects on these reporters. Together the data suggest that Int6 depletion blocks ubiquitin-dependent proteolysis by decreasing both ubiquitin levels and the assembly of functional proteasome machinery, leading to accumulation of oncoproteins such as SRC3 that can transform mammary epithelium. Our data also raise the possibility that Int6 can further fine-tune protein levels by selectively controlling translation of specific mRNAs. 2010-10-04 2011-02-10 /pmc/articles/PMC3017639/ /pubmed/20890303 http://dx.doi.org/10.1038/onc.2010.445 Text en Users may view, print, copy, download and text and data- mine the content in such documents, for the purposes of academic research, subject always to the full Conditions of use: http://www.nature.com/authors/editorial_policies/license.html#terms
spellingShingle Article
Suo, Jinfeng
Snider, Sarah J.
Mills, Gordon B.
Creighton, Chad J.
Chen, Albert
Schiff, Rachel
Lloyd, Richard E.
Chang, Eric C.
Int6 regulates both proteasomal degradation and translation initiation and is critical for proper formation of acini by human mammary epithelium: Dual regulation of protein synthesis and degradation by Int6
title Int6 regulates both proteasomal degradation and translation initiation and is critical for proper formation of acini by human mammary epithelium: Dual regulation of protein synthesis and degradation by Int6
title_full Int6 regulates both proteasomal degradation and translation initiation and is critical for proper formation of acini by human mammary epithelium: Dual regulation of protein synthesis and degradation by Int6
title_fullStr Int6 regulates both proteasomal degradation and translation initiation and is critical for proper formation of acini by human mammary epithelium: Dual regulation of protein synthesis and degradation by Int6
title_full_unstemmed Int6 regulates both proteasomal degradation and translation initiation and is critical for proper formation of acini by human mammary epithelium: Dual regulation of protein synthesis and degradation by Int6
title_short Int6 regulates both proteasomal degradation and translation initiation and is critical for proper formation of acini by human mammary epithelium: Dual regulation of protein synthesis and degradation by Int6
title_sort int6 regulates both proteasomal degradation and translation initiation and is critical for proper formation of acini by human mammary epithelium: dual regulation of protein synthesis and degradation by int6
topic Article
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC3017639/
https://www.ncbi.nlm.nih.gov/pubmed/20890303
http://dx.doi.org/10.1038/onc.2010.445
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