MYC activity is negatively regulated by a C-terminal lysine cluster

A. R. Wasylishen; M. Kalkat; S. S. Kim; A. Pandyra; P. K. Chan; S. Oliveri; E. Sedivy; D. Konforte; C. Bros; B. Raught; L. Z. Penn

doi:10.1038/onc.2013.36

MYC activity is negatively regulated by a C-terminal lysine cluster

A. R. Wasylishen, M. Kalkat, S. S. Kim, A. Pandyra, P. K. Chan, S. Oliveri, E. Sedivy, D. Konforte, C. Bros, B. Raught, L. Z. Penn

Genetics

Research output: Contribution to journal › Article › peer-review

14 Scopus citations

Abstract

The MYC oncogene is not only deregulated in cancer through abnormally high levels of expression, but also through oncogenic lesions in upstream signalling cascades. Modelling MYC deregulation using signalling mutants is a productive research strategy. For example, the MYC threonine-58 to alanine substitution mutant (T58A) within MYC-homology box 1 is more transforming than wild-type (WT) MYC, because of decreased apoptosis and increased protein stability. Understanding the regulatory mechanisms controlling T58 phosphorylation has led to new approaches for the development of MYC inhibitors. In this manuscript, we have extensively characterized a MYC signalling mutant in which six lysine residues near the highly conserved MYC homology box IV and basic region have been substituted to arginines (6KR). Previous literature suggests these lysines can undergo both ubiquitylation and acetylation. We show MYC 6KR is able to fully rescue the slow growth phenotype of HO15.19 MYC-null fibroblasts, and promote cell cycle entry of serum-starved MCF10A cells. Remarkably, 6KR increased anchorage-independent colony growth compared with WT MYC in both SH-EP and MCF10A cells. Moreover, it was also more potent in promoting xenograft tumour growth of Rat1A and SH-EP cells. Combined, our data identify this region and these six lysines as important residues for the negative regulation of MYC-induced transformation. Mechanistically, we demonstrate that, unlike T58A, the increased transformation is not a result of increased protein stability or a reduced capacity for 6KR to induce apoptosis. Through expression analysis and luciferase reporter assays, we show that 6KR has increased transcriptional activity compared with WT MYC. Combined, through a comprehensive evaluation across multiple cell types, we identify an important regulatory region within MYC. A better understanding of the full scope of signalling through these residues will provide further insights into the mechanisms contributing to MYC-induced tumorigenesis and may unveil novel therapeutic strategies to target Myc in cancer.

Original language	English (US)
Pages (from-to)	1066-1072
Number of pages	7
Journal	Oncogene
Volume	33
Issue number	8
DOIs	https://doi.org/10.1038/onc.2013.36
State	Published - Feb 20 2014

Keywords

Apoptosis
Cellular transformation
Lysine
Myc
Transcription

ASJC Scopus subject areas

Molecular Biology
Genetics
Cancer Research

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10.1038/onc.2013.36

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title = "MYC activity is negatively regulated by a C-terminal lysine cluster",

abstract = "The MYC oncogene is not only deregulated in cancer through abnormally high levels of expression, but also through oncogenic lesions in upstream signalling cascades. Modelling MYC deregulation using signalling mutants is a productive research strategy. For example, the MYC threonine-58 to alanine substitution mutant (T58A) within MYC-homology box 1 is more transforming than wild-type (WT) MYC, because of decreased apoptosis and increased protein stability. Understanding the regulatory mechanisms controlling T58 phosphorylation has led to new approaches for the development of MYC inhibitors. In this manuscript, we have extensively characterized a MYC signalling mutant in which six lysine residues near the highly conserved MYC homology box IV and basic region have been substituted to arginines (6KR). Previous literature suggests these lysines can undergo both ubiquitylation and acetylation. We show MYC 6KR is able to fully rescue the slow growth phenotype of HO15.19 MYC-null fibroblasts, and promote cell cycle entry of serum-starved MCF10A cells. Remarkably, 6KR increased anchorage-independent colony growth compared with WT MYC in both SH-EP and MCF10A cells. Moreover, it was also more potent in promoting xenograft tumour growth of Rat1A and SH-EP cells. Combined, our data identify this region and these six lysines as important residues for the negative regulation of MYC-induced transformation. Mechanistically, we demonstrate that, unlike T58A, the increased transformation is not a result of increased protein stability or a reduced capacity for 6KR to induce apoptosis. Through expression analysis and luciferase reporter assays, we show that 6KR has increased transcriptional activity compared with WT MYC. Combined, through a comprehensive evaluation across multiple cell types, we identify an important regulatory region within MYC. A better understanding of the full scope of signalling through these residues will provide further insights into the mechanisms contributing to MYC-induced tumorigenesis and may unveil novel therapeutic strategies to target Myc in cancer.",

keywords = "Apoptosis, Cellular transformation, Lysine, Myc, Transcription",

author = "Wasylishen, {A. R.} and M. Kalkat and Kim, {S. S.} and A. Pandyra and Chan, {P. K.} and S. Oliveri and E. Sedivy and D. Konforte and C. Bros and B. Raught and Penn, {L. Z.}",

note = "Funding Information: We thank Dr Martin Eilers for kindly providing the Myc 6KR construct, Dr Garry Nolan for providing retroviral reagents and packaging cell lines. SH-EP Tet21/N-Myc, MCF10A, Rat-1A and HO15.19 cells were kindly provided by Dr Manfred Schwab, Dr Senthil Muthuswamy, Dr Edward Prochownick and Dr John Sedivy, respectively. Additionally we thank Drs Bruno Amati, Chi Dang and Stephen Hann for kindly providing luciferase reporter constructs. We also thank Andrew Rust and Drs Angelina Stojanova and Peter Mullen for technical assistance, and the members of the Penn Lab for helpful discussions and critical review of this manuscript. This research was funded by grants from the Canadian Cancer Society Research Institute and Canadian Institute for Health Research (LZP), Canadian Breast Cancer Foundation Ontario Region Doctoral Fellowships (ARW and AP) and an Ontario Graduate Student Fellowship (MK). BR and LZP hold the Canada Research Chairs in Proteomics & Molecular Medicine and Molecular Oncology, respectively. Additional support was provided by the Ontario Ministry of Health and Long Term Care. The views expressed do not necessarily reflect those of the OMOHLTC.",

year = "2014",

month = feb,

day = "20",

doi = "10.1038/onc.2013.36",

language = "English (US)",

volume = "33",

pages = "1066--1072",

journal = "Oncogene",

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TY - JOUR

T1 - MYC activity is negatively regulated by a C-terminal lysine cluster

AU - Wasylishen, A. R.

AU - Kalkat, M.

AU - Kim, S. S.

AU - Pandyra, A.

AU - Chan, P. K.

AU - Oliveri, S.

AU - Sedivy, E.

AU - Konforte, D.

AU - Bros, C.

AU - Raught, B.

AU - Penn, L. Z.

N1 - Funding Information: We thank Dr Martin Eilers for kindly providing the Myc 6KR construct, Dr Garry Nolan for providing retroviral reagents and packaging cell lines. SH-EP Tet21/N-Myc, MCF10A, Rat-1A and HO15.19 cells were kindly provided by Dr Manfred Schwab, Dr Senthil Muthuswamy, Dr Edward Prochownick and Dr John Sedivy, respectively. Additionally we thank Drs Bruno Amati, Chi Dang and Stephen Hann for kindly providing luciferase reporter constructs. We also thank Andrew Rust and Drs Angelina Stojanova and Peter Mullen for technical assistance, and the members of the Penn Lab for helpful discussions and critical review of this manuscript. This research was funded by grants from the Canadian Cancer Society Research Institute and Canadian Institute for Health Research (LZP), Canadian Breast Cancer Foundation Ontario Region Doctoral Fellowships (ARW and AP) and an Ontario Graduate Student Fellowship (MK). BR and LZP hold the Canada Research Chairs in Proteomics & Molecular Medicine and Molecular Oncology, respectively. Additional support was provided by the Ontario Ministry of Health and Long Term Care. The views expressed do not necessarily reflect those of the OMOHLTC.

PY - 2014/2/20

Y1 - 2014/2/20

N2 - The MYC oncogene is not only deregulated in cancer through abnormally high levels of expression, but also through oncogenic lesions in upstream signalling cascades. Modelling MYC deregulation using signalling mutants is a productive research strategy. For example, the MYC threonine-58 to alanine substitution mutant (T58A) within MYC-homology box 1 is more transforming than wild-type (WT) MYC, because of decreased apoptosis and increased protein stability. Understanding the regulatory mechanisms controlling T58 phosphorylation has led to new approaches for the development of MYC inhibitors. In this manuscript, we have extensively characterized a MYC signalling mutant in which six lysine residues near the highly conserved MYC homology box IV and basic region have been substituted to arginines (6KR). Previous literature suggests these lysines can undergo both ubiquitylation and acetylation. We show MYC 6KR is able to fully rescue the slow growth phenotype of HO15.19 MYC-null fibroblasts, and promote cell cycle entry of serum-starved MCF10A cells. Remarkably, 6KR increased anchorage-independent colony growth compared with WT MYC in both SH-EP and MCF10A cells. Moreover, it was also more potent in promoting xenograft tumour growth of Rat1A and SH-EP cells. Combined, our data identify this region and these six lysines as important residues for the negative regulation of MYC-induced transformation. Mechanistically, we demonstrate that, unlike T58A, the increased transformation is not a result of increased protein stability or a reduced capacity for 6KR to induce apoptosis. Through expression analysis and luciferase reporter assays, we show that 6KR has increased transcriptional activity compared with WT MYC. Combined, through a comprehensive evaluation across multiple cell types, we identify an important regulatory region within MYC. A better understanding of the full scope of signalling through these residues will provide further insights into the mechanisms contributing to MYC-induced tumorigenesis and may unveil novel therapeutic strategies to target Myc in cancer.

AB - The MYC oncogene is not only deregulated in cancer through abnormally high levels of expression, but also through oncogenic lesions in upstream signalling cascades. Modelling MYC deregulation using signalling mutants is a productive research strategy. For example, the MYC threonine-58 to alanine substitution mutant (T58A) within MYC-homology box 1 is more transforming than wild-type (WT) MYC, because of decreased apoptosis and increased protein stability. Understanding the regulatory mechanisms controlling T58 phosphorylation has led to new approaches for the development of MYC inhibitors. In this manuscript, we have extensively characterized a MYC signalling mutant in which six lysine residues near the highly conserved MYC homology box IV and basic region have been substituted to arginines (6KR). Previous literature suggests these lysines can undergo both ubiquitylation and acetylation. We show MYC 6KR is able to fully rescue the slow growth phenotype of HO15.19 MYC-null fibroblasts, and promote cell cycle entry of serum-starved MCF10A cells. Remarkably, 6KR increased anchorage-independent colony growth compared with WT MYC in both SH-EP and MCF10A cells. Moreover, it was also more potent in promoting xenograft tumour growth of Rat1A and SH-EP cells. Combined, our data identify this region and these six lysines as important residues for the negative regulation of MYC-induced transformation. Mechanistically, we demonstrate that, unlike T58A, the increased transformation is not a result of increased protein stability or a reduced capacity for 6KR to induce apoptosis. Through expression analysis and luciferase reporter assays, we show that 6KR has increased transcriptional activity compared with WT MYC. Combined, through a comprehensive evaluation across multiple cell types, we identify an important regulatory region within MYC. A better understanding of the full scope of signalling through these residues will provide further insights into the mechanisms contributing to MYC-induced tumorigenesis and may unveil novel therapeutic strategies to target Myc in cancer.

KW - Apoptosis

KW - Cellular transformation

KW - Lysine

KW - Myc

KW - Transcription

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ER -

MYC activity is negatively regulated by a C-terminal lysine cluster

Abstract

Keywords

ASJC Scopus subject areas

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