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PAF49: An RNA Polymerase I subunit essential for rDNA transcription and stabilization of PAF53

The application of genetic and biochemical techniques in yeast has informed our knowledge of transcription in mammalian cells. Such systems have allowed investigators to determine whether a gene was essential and to determine its function in rDNA transcription. However, there are significant differe...

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Autores principales: McNamar, Rachel, Freeman, Emma, Baylor, Kairo N., Fakhouri, Aula M., Huang, Sui, Knutson, Bruce A., Rothblum, Lawrence I.
Formato: Online Artículo Texto
Lenguaje:English
Publicado: American Society for Biochemistry and Molecular Biology 2023
Materias:
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC10365956/
https://www.ncbi.nlm.nih.gov/pubmed/37356716
http://dx.doi.org/10.1016/j.jbc.2023.104951
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author McNamar, Rachel
Freeman, Emma
Baylor, Kairo N.
Fakhouri, Aula M.
Huang, Sui
Knutson, Bruce A.
Rothblum, Lawrence I.
author_facet McNamar, Rachel
Freeman, Emma
Baylor, Kairo N.
Fakhouri, Aula M.
Huang, Sui
Knutson, Bruce A.
Rothblum, Lawrence I.
author_sort McNamar, Rachel
collection PubMed
description The application of genetic and biochemical techniques in yeast has informed our knowledge of transcription in mammalian cells. Such systems have allowed investigators to determine whether a gene was essential and to determine its function in rDNA transcription. However, there are significant differences in the nature of the transcription factors essential for transcription by Pol I in yeast and mammalian cells, and yeast RNA polymerase I contains 14 subunits while mammalian polymerase contains 13 subunits. We previously reported the adaptation of the auxin-dependent degron that enabled a combination of a "genetics-like" approach and biochemistry to study mammalian rDNA transcription. Using this system, we studied the mammalian orthologue of yeast RPA34.5, PAF49, and found that it is essential for rDNA transcription and cell division. The auxin-induced degradation of PAF49 induced nucleolar stress and the accumulation of P53. Interestingly, the auxin-induced degradation of AID-tagged PAF49 led to the degradation of its binding partner, PAF53, but not vice versa. A similar pattern of co-dependent expression was also found when we studied the non-essential, yeast orthologues. An analysis of the domains of PAF49 that are essential for rDNA transcription demonstrated a requirement for both the dimerization domain and an “arm” of PAF49 that interacts with PolR1B. Further, we demonstrate this interaction can be disrupted to inhibit Pol I transcription in normal and cancer cells which leads to the arrest of normal cells and cancer cell death. In summary, we have shown that both PAF53 and PAF49 are necessary for rDNA transcription and cell growth.
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spelling pubmed-103659562023-07-26 PAF49: An RNA Polymerase I subunit essential for rDNA transcription and stabilization of PAF53 McNamar, Rachel Freeman, Emma Baylor, Kairo N. Fakhouri, Aula M. Huang, Sui Knutson, Bruce A. Rothblum, Lawrence I. J Biol Chem Research Article The application of genetic and biochemical techniques in yeast has informed our knowledge of transcription in mammalian cells. Such systems have allowed investigators to determine whether a gene was essential and to determine its function in rDNA transcription. However, there are significant differences in the nature of the transcription factors essential for transcription by Pol I in yeast and mammalian cells, and yeast RNA polymerase I contains 14 subunits while mammalian polymerase contains 13 subunits. We previously reported the adaptation of the auxin-dependent degron that enabled a combination of a "genetics-like" approach and biochemistry to study mammalian rDNA transcription. Using this system, we studied the mammalian orthologue of yeast RPA34.5, PAF49, and found that it is essential for rDNA transcription and cell division. The auxin-induced degradation of PAF49 induced nucleolar stress and the accumulation of P53. Interestingly, the auxin-induced degradation of AID-tagged PAF49 led to the degradation of its binding partner, PAF53, but not vice versa. A similar pattern of co-dependent expression was also found when we studied the non-essential, yeast orthologues. An analysis of the domains of PAF49 that are essential for rDNA transcription demonstrated a requirement for both the dimerization domain and an “arm” of PAF49 that interacts with PolR1B. Further, we demonstrate this interaction can be disrupted to inhibit Pol I transcription in normal and cancer cells which leads to the arrest of normal cells and cancer cell death. In summary, we have shown that both PAF53 and PAF49 are necessary for rDNA transcription and cell growth. American Society for Biochemistry and Molecular Biology 2023-06-24 /pmc/articles/PMC10365956/ /pubmed/37356716 http://dx.doi.org/10.1016/j.jbc.2023.104951 Text en © 2023 The Authors https://creativecommons.org/licenses/by/4.0/This is an open access article under the CC BY license (http://creativecommons.org/licenses/by/4.0/).
spellingShingle Research Article
McNamar, Rachel
Freeman, Emma
Baylor, Kairo N.
Fakhouri, Aula M.
Huang, Sui
Knutson, Bruce A.
Rothblum, Lawrence I.
PAF49: An RNA Polymerase I subunit essential for rDNA transcription and stabilization of PAF53
title PAF49: An RNA Polymerase I subunit essential for rDNA transcription and stabilization of PAF53
title_full PAF49: An RNA Polymerase I subunit essential for rDNA transcription and stabilization of PAF53
title_fullStr PAF49: An RNA Polymerase I subunit essential for rDNA transcription and stabilization of PAF53
title_full_unstemmed PAF49: An RNA Polymerase I subunit essential for rDNA transcription and stabilization of PAF53
title_short PAF49: An RNA Polymerase I subunit essential for rDNA transcription and stabilization of PAF53
title_sort paf49: an rna polymerase i subunit essential for rdna transcription and stabilization of paf53
topic Research Article
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC10365956/
https://www.ncbi.nlm.nih.gov/pubmed/37356716
http://dx.doi.org/10.1016/j.jbc.2023.104951
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