Methylation of SUV39H1 by SET7/9 results in heterochromatin relaxation and genome instability

Wang, Donglai; Zhou, Jingyi; Liu, Xiangyu; Lu, Danyu; Shen, Chen; Du, Yipeng; Wei, Fu-Zheng; Song, Bing; Lu, Xiaopeng; Yu, Yu; Wang, Lina; Zhao, Ying; Wang, Haiying; Yang, Ye; Akiyama, Yoshimitsu; Zhang, Hongquan; Zhu, Wei‐Guo

doi:10.1073/pnas.1216596110

Cited by 101 publications

(107 citation statements)

References 35 publications

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“…Moreover, the role of H3K4 methylation in nucleotide excision repair is interesting, and H3K4R mutation exerts different impacts on nucleotide excision repair on different genomic loci (Chaudhuri et al, 2009). In our previous studies, we also described the critical role of an H3K4 methyltransferase SET7/9 in DNA damage response and oxidative stress, but through methylating non-histone proteins Wang et al, 2013). At last, H3K23 trimethylation (H3K23me3), a novel characterized histone modification, is reported to blocks DNA damage in pericentric heterochromatin during meiosis in Tetrahymena (Papazyan et al, 2014).…”

Section: Methylationmentioning

confidence: 99%

“…At first, H3K9me3 is an essential histone marker of heterochromatin (Grewal and Jia, 2007). H3K9 methyltransferase SUV39H1 is required for the maintenance of heterochromatic state, and its methylation by SET7/9 impairs its enzymatic activity resulting in decreased H3K9me3 and heterochromatin instability (Peng and Karpen, 2009;Wang et al, 2013). Next, H3K9 methylation is important for the cellular response to DNA damage, but the role of H3K9 methylation is different at the early-stage and late-stage of DNA damage response.…”

Section: Methylationmentioning

confidence: 99%

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Histone modifications in DNA damage response

Cao

Shen

Zhu

2016

Sci. China Life Sci.

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DNA damage is a relatively common event in eukaryotic cell and may lead to genetic mutation and even cancer. DNA damage induces cellular responses that enable the cell either to repair the damaged DNA or cope with the damage in an appropriate way. Histone proteins are also the fundamental building blocks of eukaryotic chromatin besides DNA, and many types of post-translational modifications often occur on tails of histones. Although the function of these modifications has remained elusive, there is ever-growing studies suggest that histone modifications play vital roles in several chromatin-based processes, such as DNA damage response. In this review, we will discuss the main histone modifications, and their functions in DNA damage response.DNA damage response, histone modifications, chromatin, DNA repair Citation:

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Section: Methylationmentioning

confidence: 99%

Section: Methylationmentioning

confidence: 99%

Histone modifications in DNA damage response

Cao

Shen

Zhu

2016

Sci. China Life Sci.

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“…There have been several non-histone proteins reported as the substrates for Set7/9, including TAF10 (TATA box binding protein (TBP)-associated factor, 30 kDa), 9 oestrogen receptor a (ERa), 10 RelA, 11 PCAF (P300/CBP-associated factor), 12 Stat3, 13 Yap, 14 and Suv39h1. 15 However, in most cases the functional significance of this methylation is still not clear. The beststudied targets of Set7/9-mediated methylation are p53 16 and E2 promoter-binding factor 1 (E2F1), 17 transcription factors involved in regulation of DNA damage response (DDR).…”

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confidence: 99%

KMTase Set7/9 is a critical regulator of E2F1 activity upon genotoxic stress

et al. 2014

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During the recent years lysine methyltransferase Set7/9 ((Su(var)-3-9, Enhancer-of-Zeste, Trithorax) domain containing protein 7/9) has emerged as an important regulator of different transcription factors. In this study, we report a novel function for Set7/9 as a critical co-activator of E2 promoter-binding factor 1 (E2F1)-dependent transcription in response to DNA damage. By means of various biochemical, cell biology, and bioinformatics approaches, we uncovered that cell-cycle progression through the G1/S checkpoint of tumour cells upon DNA damage is defined by the threshold of expression of both E2F1 and Set7/9. The latter affects the activity of E2F1 by indirectly modulating histone modifications in the promoters of E2F1-dependent genes. Moreover, Set7/9 differentially affects E2F1 transcription targets: it promotes cell proliferation via expression of the CCNE1 gene and represses apoptosis by inhibiting the TP73 gene. Our biochemical screening of the panel of lung tumour cell lines suggests that these two factors are critically important for transcriptional upregulation of the CCNE1 gene product and hence successful progression through cell cycle. These findings identify Set7/9 as a potential biomarker in tumour cells with overexpressed E2F1 activity. Cell Death and Differentiation (2014) 21, 1889-1899; doi:10.1038/cdd.2014.108; published online 15 August 2014Lysine methylation of non-histone proteins has recently emerged as a novel regulatory mechanism to control protein functions. 1-4Set7/9 ((Su(var)-3-9, Enhancer-of-Zeste, Trithorax) domain containing protein 7/9) is a founding member of the family of non-chromatin lysine methyltransferases (KMTases). Set7/9 was initially identified as a monomethylase of histone H3 lysine 4 (H3K4) in vitro. 4,5However, we and others showed that the recombinant Set7/9 failed to target nucleosomes for methylation, [6][7][8] suggesting that Set7/9 functions as a factor-specific KMTase. There have been several non-histone proteins reported as the substrates for Set7/9, including TAF10 (TATA box binding protein (TBP)-associated factor, 30 kDa), 9 oestrogen receptor a (ERa), 10 RelA, 11 PCAF (P300/CBP-associated factor), 12 Stat3,13 Yap, 14 and Suv39h1. 15 However, in most cases the functional significance of this methylation is still not clear. The beststudied targets of Set7/9-mediated methylation are p53 16 and E2 promoter-binding factor 1 (E2F1), 17 transcription factors involved in regulation of DNA damage response (DDR).In response to genotoxic stress cancer cells undergo cell-cycle arrest either in G1/S or G2/M or in both checkpoints. The presence of intact p53 in cancer cells mediates transient G1/S checkpoint arrest, 18,19 which allows cells to repair the damaged DNA before replication or, if the amount of damage is insurmountable, drives cells into apoptosis. 20,21On the contrary, the activity of the E2F family transcription factors, especially E2F1, drives cells from the G1/S block to mitosis. 22,23 Transcriptional activity of E2F1, in turn, is repressed by the retin...

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“…On the other hand, more compact constitutive heterochromatin, observed in Sirt7 deficient cells, might prevent opening of chromatin regions that are in need for DNA repair causing accumulation of DNA damage and accelerated aging. In fact, recent evidence points to the importance of temporary chromatin relaxation even within highly compacted constitutive heterochromatin to allow DNA repair during stress responses [35]. The clear increase of constitutive heterochromatin in Sirt7 mutant cells seems to be in contrast to increased relaxation of facultative rDNA heterochromatin, which is also apparent in Sirt7 KO cells.…”

Section: Discussionmentioning

confidence: 99%

Sirt7 inhibits Sirt1-mediated activation of Suv39h1

et al. 2018

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Sirtuins regulate a variety of cellular processes through protein deacetylation. The best-known member of mammalian sirtuin family, Sirt1, plays important roles in the maintenance of cellular homeostasis by regulating cell metabolism, differentiation and stress responses, among others. Sirt1 activity requires tight regulation to meet specific cellular requirements, which is achieved at different levels and by specific mechanisms. Recently, a regulatory loop between Sirt1 and another sirtuin, Sirt7, was identified. Sirt7 inhibits Sirt1 autodeacetylation at K230 and activation thereby preventing Sirt1-mediated repression of adipocyte differentiation by inhibition of the PPARγ gene. Here, we extend the regulatory complexity of Sirt7-dependent restriction of Sirt1 activity by demonstrating that Sirt7 reduces activation of a previously described prominent Sirt1 target, the histone methyltransferase Suv39h1. We show that removal of the acetyl-group at K230 in Sirt1 due to the absence of Sirt7 leads to hyperactivation of Sirt1 and thereby to constantly increased activity of Suv39h1.

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Methylation of SUV39H1 by SET7/9 results in heterochromatin relaxation and genome instability

Cited by 101 publications

References 35 publications

Histone modifications in DNA damage response

Histone modifications in DNA damage response

KMTase Set7/9 is a critical regulator of E2F1 activity upon genotoxic stress

Sirt7 inhibits Sirt1-mediated activation of Suv39h1

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