The transcriptional repressor JHDM3A demethylates trimethyl histone H3 lysine 9 and lysine 36 (original) (raw)

• Letter
• Published: 28 May 2006
• Kenichi Yamane1,2,
• Yangjin Bae3,
• Dianzheng Zhang3,
• Hediye Erdjument-Bromage4,
• Paul Tempst4,
• Jiemin Wong3 &
• …
• Yi Zhang1,2

Nature volume 442, pages 312–316 (2006)Cite this article

• 5533 Accesses
• 509 Citations
• 9 Altmetric
• Metrics details

Abstract

Post-translational modification of chromatin has profound effects on many biological processes including transcriptional regulation, heterochromatin organization, and X-chromosome inactivation1,2. Recent studies indicate that methylation on specific histone lysine (K) residues participates in many of these processes3. Lysine methylation occurs in three distinct states, having either one (me1), two (me2) or three (me3) methyl groups attached to the amine group of the lysine side chain. These differences in modification state have an important role in defining how methylated chromatin is recognized and interpreted4,5,6. Until recently, histone lysine methylation was considered a stable modification7,8, but the identification of histone demethylase enzymes has demonstrated the reversibility of this epigenetic mark9,10,11. So far, all characterized histone demethylases show enzymatic activity towards lysine residues modified in the me1 or me2 state9,10,11, leaving open the possibility that me3 constitutes an irreversible modification. Here we demonstrate that JHDM3A (jumonji C (JmjC)-domain-containing histone demethylase 3A; also known as JMJD2A) is capable of removing the me3 group from modified H3 lysine 9 (H3K9) and H3 lysine 36 (H3K36). Overexpression of JHDM3A abrogates recruitment of HP1 (heterochromatin protein 1) to heterochromatin, indicating a role for JHDM3A in antagonizing methylated H3K9 nucleated events. siRNA-mediated knockdown of JHDM3A leads to increased levels of H3K9 methylation and upregulation of a JHDM3A target gene, ASCL2, indicating that JHDM3A may function in euchromatin to remove histone methylation marks that are associated with active transcription12.

This is a preview of subscription content, access via your institution

Access options

Subscribe to this journal

Receive 51 print issues and online access

$199.00 per year

only $3.90 per issue

Buy this article

• Purchase on SpringerLink
• Instant access to full article PDF

Prices may be subject to local taxes which are calculated during checkout

Additional access options:

• Log in
• Learn about institutional subscriptions
• Read our FAQs
• Contact customer support

Similar content being viewed by others

References

1. Bird, A. DNA methylation patterns and epigenetic memory. Genes Dev. 16, 6–21 (2002)
   Article CAS PubMed Google Scholar
2. Jenuwein, T. & Allis, C. D. Translating the histone code. Science 293, 1074–1080 (2001)
   Article CAS PubMed Google Scholar
3. Martin, C. & Zhang, Y. The diverse functions of histone lysine methylation. Nature Rev. Mol. Cell Biol. 6, 838–849 (2005)
   Article CAS Google Scholar
4. Flanagan, J. F. et al. Double chromodomains cooperate to recognize the methylated histone H3 tail. Nature 438, 1181–1185 (2005)
   Article ADS CAS PubMed Google Scholar
5. Jacobs, S. A. & Khorasanizadeh, S. Structure of HP1 chromodomain bound to a lysine 9-methylated histone H3 tail. Science 295, 2080–2083 (2002)
   Article ADS CAS PubMed Google Scholar
6. Min, J., Zhang, Y. & Xu, R. M. Structural basis for specific binding of Polycomb chromodomain to histone H3 methylated at Lys 27. Genes Dev. 17, 1823–1828 (2003)
   Article CAS PubMed PubMed Central Google Scholar
7. Bannister, A. J., Schneider, R. & Kouzarides, T. Histone methylation: dynamic or static? Cell 109, 801–806 (2002)
   Article CAS PubMed Google Scholar
8. Duerre, J. A. & Lee, C. T. In vivo methylation and turnover of rat brain histones. J. Neurochem. 23, 541–547 (1974)
   Article CAS PubMed Google Scholar
9. Shi, Y. et al. Histone demethylation mediated by the nuclear amine oxidase homolog LSD1. Cell 119, 941–953 (2004)
   Article CAS PubMed Google Scholar
10. Tsukada, Y. et al. Histone demethylation by a family of JmjC domain-containing proteins. Nature 439, 811–816 (2006)
    Article ADS CAS PubMed Google Scholar
11. Yamane, K. et al. JHDM2A, a JmjC-containing H3K9 demethylase, facilitates transcription activation by androgen receptor. Cell 125, 483–495 (2006)
    Article CAS PubMed Google Scholar
12. Vakoc, C. R., Mandat, S. A., Olenchock, B. A. & Blobel, G. A. Histone H3 lysine 9 methylation and HP1γ are associated with transcription elongation through mammalian chromatin. Mol. Cell 19, 381–391 (2005)
    Article CAS PubMed Google Scholar
13. Clissold, P. M. & Ponting, C. P. JmjC: cupin metalloenzyme-like domains in jumonji, hairless and phospholipase A2β. Trends Biochem. Sci. 26, 7–9 (2001)
    Article CAS PubMed Google Scholar
14. Trewick, S. C., McLaughlin, P. J. & Allshire, R. C. Methylation: lost in hydroxylation? EMBO Rep. 6, 315–320 (2005)
    Article CAS PubMed PubMed Central Google Scholar
15. Katoh, M. & Katoh, M. Identification and characterization of JMJD2 family genes in silico. Int. J. Oncol. 24, 1623–1628 (2004)
    CAS PubMed Google Scholar
16. Gray, S. G. et al. Functional characterization of JMJD2A, a histone deacetylase- and retinoblastoma-binding protein. J. Biol. Chem. 280, 28507–28518 (2005)
    Article CAS PubMed Google Scholar
17. Zhang, D., Yoon, H. G. & Wong, J. JMJD2A is a novel N-CoR-interacting protein and is involved in repression of the human transcription factor achaete scute-like homologue 2 (ASCL2/Hash2). Mol. Cell. Biol. 25, 6404–6414 (2005)
    Article CAS PubMed PubMed Central Google Scholar
18. Bannister, A. J. et al. Spatial distribution of di- and tri-methyl lysine 36 of histone H3 at active genes. J. Biol. Chem. 280, 17732–17736 (2005)
    Article CAS PubMed Google Scholar
19. Bannister, A. J. et al. Selective recognition of methylated lysine 9 on histone H3 by the HP1 chromo domain. Nature 410, 120–124 (2001)
    Article ADS CAS PubMed Google Scholar
20. Lachner, M., O'Carroll, D., Rea, S., Mechtler, K. & Jenuwein, T. Methylation of histone H3 lysine 9 creates a binding site for HP1 proteins. Nature 410, 116–120 (2001)
    Article ADS CAS PubMed Google Scholar
21. Peters, A. H. et al. Partitioning and plasticity of repressive histone methylation states in mammalian chromatin. Mol. Cell 12, 1577–1589 (2003)
    Article CAS PubMed Google Scholar
22. Rice, J. C. et al. Histone methyltransferases direct different degrees of methylation to define distinct chromatin domains. Mol. Cell 12, 1591–1598 (2003)
    Article CAS PubMed Google Scholar
23. Whetstine, J. R. et al. Reversal of histone lysine trimethylation by the JMJD2 family of histone demethylases. Cell 125, 467–481 (2006)
    Article CAS PubMed Google Scholar
24. Sarraf, S. A. & Stancheva, I. Methyl-CpG binding protein MBD1 couples histone H3 methylation at lysine 9 by SETDB1 to DNA replication and chromatin assembly. Mol. Cell 15, 595–605 (2004)
    Article CAS PubMed Google Scholar
25. Schultz, D., Ayyanathan, K., Negorev, D., Maul, G. & Rauscher, F. SETDB1: a novel KAP-1-associated histone H3, lysine 9-specific methyltransferase that contributes to HP1-mediated silencing of euchromatic genes by KRAB zinc-finger proteins. Genes Dev. 16, 919–932 (2002)
    Article CAS PubMed PubMed Central Google Scholar
26. Kim, J. et al. Tudor, MBT and chromo domains gauge the degree of lysine methylation. EMBO Rep. 7, 397–403 (2006)
    CAS PubMed PubMed Central Google Scholar
27. Huang, Y., Fang, J., Bedford, M. T., Zhang, Y. & Xu, R. M. Recognition of histone H3 lysine-4 methylation by the double Tudor domain of JMJD2A. Science 312, 748–751 (2006)
    Article ADS CAS PubMed Google Scholar
28. Zhang, X. et al. Structure of the Neurospora SET domain protein DIM-5, a histone H3 lysine methyltransferase. Cell 111, 117–127 (2002)
    Article CAS PubMed PubMed Central Google Scholar

Download references

Acknowledgements

We thank J. Fang, B. Strahl, T. Jenuwein, L. Schmiedeberg, A. Verreault and Y. Shinkai for plasmids; X. Cheng and R. Cao for Dim5 protein and EZH2 complex, respectively; L. Lacomis for help with mass spectrometry; and technical assistance from C. Toumazou. This work was supported by NIH grants to Y.Z., P.T. and J.W. Y.Z. is an Investigator of the Howard Hughes Medical Institute. Author Contributions R.J.K. carried out most of the experiments in Figs 1–3and the Supplementary Figures; K.Y. generated recombinant protein; H.E.-B. and P.T. performed mass spectrometric analysis; Y.B., D.Z. and J.W. carried out the experiments in Fig. 4; R.J.K. and Y.Z. wrote the paper.

Author information

Authors and Affiliations

1. Howard Hughes Medical Institute,
   Robert J. Klose, Kenichi Yamane & Yi Zhang
2. Department of Biochemistry and Biophysics, Lineberger Comprehensive Cancer Center, University of North Carolina at Chapel Hill, Chapel Hill, North Carolina, 27599-7295, USA
   Robert J. Klose, Kenichi Yamane & Yi Zhang
3. Department of Molecular and Cellular Biology, Baylor College of Medicine, One Baylor Plaza, Texas, 77030, Houston, USA
   Yangjin Bae, Dianzheng Zhang & Jiemin Wong
4. Molecular Biology Program, Memorial Sloan Kettering Cancer Center, 1275 York Avenue, New York, 10021, New York, USA
   Hediye Erdjument-Bromage & Paul Tempst

Authors

1. Robert J. Klose
   You can also search for this author inPubMed Google Scholar
2. Kenichi Yamane
   You can also search for this author inPubMed Google Scholar
3. Yangjin Bae
   You can also search for this author inPubMed Google Scholar
4. Dianzheng Zhang
   You can also search for this author inPubMed Google Scholar
5. Hediye Erdjument-Bromage
   You can also search for this author inPubMed Google Scholar
6. Paul Tempst
   You can also search for this author inPubMed Google Scholar
7. Jiemin Wong
   You can also search for this author inPubMed Google Scholar
8. Yi Zhang
   You can also search for this author inPubMed Google Scholar

Corresponding author

Correspondence toYi Zhang.

Ethics declarations

Competing interests

Reprints and permissions information is available at npg.nature.com/reprintsandpermissions. The authors declare no competing financial interests.

Supplementary information

Rights and permissions

About this article

Cite this article

Klose, R., Yamane, K., Bae, Y. et al. The transcriptional repressor JHDM3A demethylates trimethyl histone H3 lysine 9 and lysine 36.Nature 442, 312–316 (2006). https://doi.org/10.1038/nature04853

Download citation

• Received: 16 January 2006
• Accepted: 04 May 2006
• Published: 28 May 2006
• Issue Date: 20 July 2006
• DOI: https://doi.org/10.1038/nature04853

This article is cited by

Editorial Summary

Up to the mark

Two papers in this issue identify enzymes capable of demethylating a trimethyl group from the Lys 9 residue of histone H3 — a 'mark' required for the establishment of heterochromatin and previously considered stable. Cloos et al. show that GASC1, a member of the JMJD2 enzyme family, can disrupt heterochromatin structure when overexpressed and may contribute to tumour development. Klose et al. show that overexpression of JHDM3A, also a JMJD2-type enzyme, disrupts heterochromatin structure. It may function in euchromatin to regulate transcription.