DNA methyltransferase

(Redirected from DNMT)

In biochemistry, the DNA methyltransferase (DNA MTase, DNMT) family of enzymes catalyze the transfer of a methyl group to DNA. DNA methylation serves a wide variety of biological functions. All the known DNA methyltransferases use S-adenosyl methionine (SAM) as the methyl donor.

N-6 DNA Methylase
crystal structure of type i restriction enzyme ecoki m protein (ec 2.1.1.72) (m.ecoki)
Identifiers
SymbolN6_Mtase
PfamPF02384
Pfam clanCL0063
InterProIPR003356
PROSITEPDOC00087
Available protein structures:
Pfam  structures / ECOD  
PDBRCSB PDB; PDBe; PDBj
PDBsumstructure summary
HsdM N-terminal domain
Identifiers
SymbolHsdM_N
PfamPF12161
Available protein structures:
Pfam  structures / ECOD  
PDBRCSB PDB; PDBe; PDBj
PDBsumstructure summary
C-5 cytosine-specific DNA methylase
structure of human dnmt2, an enigmatic dna methyltransferase homologue
Identifiers
SymbolDNA_methylase
PfamPF00145
Pfam clanCL0063
InterProIPR001525
PROSITEPDOC00089
SCOP21hmy / SCOPe / SUPFAM
CDDcd00315
Available protein structures:
Pfam  structures / ECOD  
PDBRCSB PDB; PDBe; PDBj
PDBsumstructure summary
DNA methylase
crystal structure of methyltransferase mboiia (moraxella bovis)
Identifiers
SymbolN6_N4_Mtase
PfamPF01555
Pfam clanCL0063
InterProIPR002941
PROSITEPDOC00088
SCOP21boo / SCOPe / SUPFAM
Available protein structures:
Pfam  structures / ECOD  
PDBRCSB PDB; PDBe; PDBj
PDBsumstructure summary

Classification

edit

Substrate

edit

MTases can be divided into three different groups on the basis of the chemical reactions they catalyze:

m6A and m4C methyltransferases are found primarily in prokaryotes (although recent evidence has suggested that m6A is abundant in eukaryotes[1]). m5C methyltransferases are found in some lower eukaryotes, in most higher plants, and in animals beginning with the echinoderms.

The m6A methyltransferases (N-6 adenine-specific DNA methylase) (A-Mtase) are enzymes that specifically methylate the amino group at the C-6 position of adenines in DNA. They are found in the three existing types of bacterial restriction-modification systems (in type I system the A-Mtase is the product of the hsdM gene, and in type III it is the product of the mod gene). These enzymes are responsible for the methylation of specific DNA sequences in order to prevent the host from digesting its own genome via its restriction enzymes. These methylases have the same sequence specificity as their corresponding restriction enzymes. These enzymes contain a conserved motif Asp/Asn-Pro-Pro-Tyr/Phe in their N-terminal section, this conserved region could be involved in substrate binding or in the catalytic activity.[2][3][4][5] The structure of N6-MTase TaqI (M.TaqI) has been resolved to 2.4 A. The molecule folds into 2 domains, an N-terminal catalytic domain, which contains the catalytic and cofactor binding sites, and comprises a central 9-stranded beta-sheet, surrounded by 5 helices; and a C-terminal DNA recognition domain, which is formed by 4 small beta-sheets and 8 alpha-helices. The N- and C-terminal domains form a cleft that accommodates the DNA substrate.[6] A classification of N-MTases has been proposed, based on conserved motif (CM) arrangements.[5] According to this classification, N6-MTases that have a DPPY motif (CM II) occurring after the FxGxG motif (CM I) are designated D12 class N6-adenine MTases. The type I restriction and modification system is composed of three polypeptides R, M and S. The M (hsdM) and S subunits together form a methyltransferase that methylates two adenine residues in complementary strands of a bipartite DNA recognition sequence. In the presence of the R subunit, the complex can also act as an endonuclease, binding to the same _target sequence but cutting the DNA some distance from this site. Whether the DNA is cut or modified depends on the methylation state of the _target sequence. When the _target site is unmodified, the DNA is cut. When the _target site is hemimethylated, the complex acts as a maintenance methyltransferase, modifying the DNA so that both strands become methylated. hsdM contains an alpha-helical domain at the N-terminus, the HsdM N-terminal domain.[7]

Among the m6A methyltransferases (N-6 adenine-specific DNA methylase) there is a group of orphan MTases that do not participate in the bacterial restriction/methylation system.[8] These enzymes have a regulatory role in gene expression and cell cycle regulation. EcoDam from E. coli [9] and CcrM from Caulobacter crescentus [10] are well characterized members of these family. More recently, CamA from Clostridioides difficile, was shown to play key functional roles in sporulation, biofilm formations and host-adaptation.[11]

m4C methyltransferases (N-4 cytosine-specific DNA methylases) are enzymes that specifically methylate the amino group at the C-4 position of cytosines in DNA.[5] Such enzymes are found as components of type II restriction-modification systems in prokaryotes. Such enzymes recognise a specific sequence in DNA and methylate a cytosine in that sequence. By this action they protect DNA from cleavage by type II restriction enzymes that recognise the same sequence[citation needed]

m5C methyltransferases (C-5 cytosine-specific DNA methylase) (C5 Mtase) are enzymes that specifically methylate the C-5 carbon of cytosines in DNA to produce C5-methylcytosine.[12][13][14] In mammalian cells, cytosine-specific methyltransferases methylate certain CpG sequences, which are believed to modulate gene expression and cell differentiation. In bacteria, these enzymes are a component of restriction-modification systems and serve as valuable tools for the manipulation of DNA.[13][15] The structure of HhaI methyltransferase (M.HhaI) has been resolved to 2.5 A: the molecule folds into 2 domains - a larger catalytic domain containing catalytic and cofactor binding sites, and a smaller DNA recognition domain.[16]

Highly conserved DNA methyltransferases of the m4C, m5C, and m6A types have been reported,[17] which appear as promising _targets for the development of novel epigenetic inhibitors to fight bacterial virulence, antibiotic resistance, among other biomedical applications.

De novo vs. maintenance

edit

De novo methyltransferases recognize something in the DNA that allows them to newly methylate cytosines. These are expressed mainly in early embryo development and they set up the pattern of methylation. De novo methyltransferases are also active when a signal-responsive cell, such as a neuron, needs to alter protein expression.[18] As an example, when fear conditioning creates a new memory in a rat, 9.17% of the genes in the rat hippocampus neuron genome are differentially methylated.[19]

Maintenance methyltransferases add methylation to DNA when one strand is already methylated. These work throughout the life of the organism to maintain the methylation pattern that had been established by the de novo methyltransferases.[citation needed]

Mammalian

edit

At least four differently active DNA methyltransferases have been identified in mammals. They are named DNMT1,[20] two isoforms transcribed from the DNMT3a gene: DNMT3a1 and DNMT3a2,[21] and DNMT3b.[22] Recently, another enzyme DNMT3c has been discovered specifically expressed in the male germline in the mouse.[23]

 
Some activation signals on a nucleosome.Nucleosomes consist of four pairs of histone proteins in a tightly assembled core region plus up to 30% of each histone remaining in a loosely organized tail (only one tail of each pair is shown). DNA is wrapped around the histone core proteins in chromosomes. The lysines (K) are designated with a number showing their position as, for instance (K4), indicating lysine as the 4th amino acid from the amino (N) end of the tail in the histone protein. Methylations {Me}, and acetylations [Ac] are common post-translational modifications on the lysines of the histone tails.

[citation needed]

 
Some repression signals on a nucleosome.

Manzo et al.[24] observed differences in genomic binding of DNMT3a1, DNMT3a2 and DNMT3b. They found 3,970 regions exclusively enriched for DNMT3a1, 3,838 exclusively enriched for DNMT3a2 and 3,432 exclusively enriched for DNMT3b.

The DNMT enzymes are not only regulated in their methylating locations on the genome by where they bind to DNA,[24] but they are also regulated by the post-translational modifications on the histone proteins of the nucleosomes around which the genomic DNA is wrapped (see Figures). Rose and Klose[25] reviewed the relationship between DNA methylation and histone lysine methylation. For example, they indicated that H3K4me3 appears to block DNA methylation while H3K9me3 plays a role in promoting DNA methylation.

DNMT3L[26] is a protein closely related to DNMT3a and DNMT3b in structure and critical for DNA methylation, but appears to be inactive on its own.

DNMT1

edit

DNMT1 is the most abundant DNA methyltransferase in mammalian cells, and considered to be the key maintenance methyltransferase in mammals. It predominantly methylates hemimethylated CpG di-nucleotides in the mammalian genome. The recognition motif for the human enzyme involves only three of the bases in the CpG dinucleotide pair: a C on one strand and CpG on the other. This relaxed substrate specificity requirement allows it to methylate unusual structures like DNA slippage intermediates at de novo rates that equal its maintenance rate.[27] Like other DNA cytosine-5 methyltransferases the human enzyme recognizes flipped out cytosines in double stranded DNA and operates by the nucleophilic attack mechanism.[28] In human cancer cells DNMT1 is responsible for both de novo and maintenance methylation of tumor suppressor genes.[29][30] The enzyme is about 1,620 amino acids long. The first 1,100 amino acids constitute the regulatory domain of the enzyme, and the remaining residues constitute the catalytic domain. These are joined by Gly-Lys repeats. Both domains are required for the catalytic function of DNMT1.[citation needed]

DNMT1 has several isoforms, the somatic DNMT1, a splice variant (DNMT1b) and an oocyte-specific isoform (DNMT1o). DNMT1o is synthesized and stored in the cytoplasm of the oocyte and translocated to the cell nucleus during early embryonic development, while the somatic DNMT1 is always found in the nucleus of somatic tissue.[citation needed]

DNMT1 null mutant embryonic stem cells were viable and contained a small percentage of methylated DNA and methyltransferase activity. Mouse embryos homozygous for a deletion in Dnmt1 die at 10–11 days gestation.[31]

TRDMT1

edit

Although this enzyme has strong sequence similarities with 5-methylcytosine methyltransferases of both prokaryotes and eukaryotes, in 2006, the enzyme was shown to methylate position 38 in aspartic acid transfer RNA and does not methylate DNA.[32] The name for this methyltransferase has been changed from DNMT2 to TRDMT1 (tRNA aspartic acid methyltransferase 1) to better reflect its biological function.[33] TRDMT1 is the first RNA cytosine methyltransferase to be identified in human cells.

DNMT3

edit

DNMT3 is a family of DNA methyltransferases that could methylate hemimethylated and unmethylated CpG at the same rate. The architecture of DNMT3 enzymes is similar to that of DNMT1, with a regulatory region attached to a catalytic domain. There are at least five members of the DNMT3 family: DNMT3a1, DNMT3a2, 3b, 3c and 3L.[citation needed]

DNMT3a1, DNMT3a2 and DNMT3b can mediate methylation of CpG sites in gene promoters, resulting in gene repression. These DNA methyltransferases can also methylate CpG sites within the coding regions of genes, where such methylation can increase gene transcription.[34] Work with DNMT3a1 showed it preferentially localized to CpG islands bivalently marked by H3K4me3 (a transcription promoting mark) and H3K27me3 (a transcription repressive mark), coinciding with the promoters of many transcription factors. Work with DNMT3a2, in neurons, found that the DNA methylation changes caused by DNMT3a2 predominantly occur in intergenic and intronic regions. These intergenic and intronic DNA methylations were thought to likely regulate enhancer activity, alternative splicing or the expression of non-coding RNAs.[35]

DNMT3a1 can co-localize with heterochromatin protein (HP1) and methyl-CpG-binding protein (MeCBP), among a number of other factors.[36] They can also interact with DNMT1, which might be a co-operative event during DNA methylation. DNMT3a prefers CpG methylation to CpA, CpT, and CpC methylation, though there appears to be some sequence preference of methylation for DNMT3a and DNMT3b. DNMT3a methylates CpG sites at a rate much slower than DNMT1, but greater than DNMT3b.

The expression of DNMT3a2 differs from DNMT3a1 and DNMT3b because DNMT3a2 expression occurs in the pattern of an immediate early gene. DNMT3a2 is induced to express in neurons, for instance, by new neuronal activity.[37][35] This may be of importance in establishing long-term memory.[38] In a rat, high levels of new DNA methylations in neurons of the hippocampus occur after a memorable event is imposed on a rat, such as contextual fear conditioning.[19] Bayraktar and Kreutz[39] found that DNMT inhibitors, applied in the brain, prevented long-term memories from forming.

DNMT3L contains DNA methyltransferase motifs and is required for establishing maternal genomic imprints, despite being catalytically inactive. DNMT3L is expressed during gametogenesis when genomic imprinting takes place. The loss of DNMT3L leads to bi-allelic expression of genes normally not expressed by the maternal allele. DNMT3L interacts with DNMT3a and DNMT3b and co-localized in the nucleus. Though DNMT3L appears incapable of methylation, it may participate in transcriptional repression.

Clinical significance

edit

DNMT inhibitors

edit

Because of the epigenetic effects of the DNMT family, some DNMT inhibitors are under investigation for treatment of some cancers:[40]

See also

edit

References

edit
  1. ^ Iyer LM, Zhang D, Aravind L (January 2016). "Adenine methylation in eukaryotes: Apprehending the complex evolutionary history and functional potential of an epigenetic modification". BioEssays. 38 (1): 27–40. doi:10.1002/bies.201500104. PMC 4738411. PMID 26660621.
  2. ^ Loenen WA, Daniel AS, Braymer HD, Murray NE (November 1987). "Organization and sequence of the hsd genes of Escherichia coli K-12". Journal of Molecular Biology. 198 (2): 159–70. doi:10.1016/0022-2836(87)90303-2. PMID 3323532.
  3. ^ Narva KE, Van Etten JL, Slatko BE, Benner JS (December 1988). "The amino acid sequence of the eukaryotic DNA [N6-adenine]methyltransferase, M.CviBIII, has regions of similarity with the prokaryotic isoschizomer M.TaqI and other DNA [N6-adenine] methyltransferases". Gene. 74 (1): 253–9. doi:10.1016/0378-1119(88)90298-3. PMID 3248728.
  4. ^ Lauster R (March 1989). "Evolution of type II DNA methyltransferases. A gene duplication model". Journal of Molecular Biology. 206 (2): 313–21. doi:10.1016/0022-2836(89)90481-6. PMID 2541254.
  5. ^ a b c Timinskas A, Butkus V, Janulaitis A (May 1995). "Sequence motifs characteristic for DNA [cytosine-N4] and DNA [adenine-N6] methyltransferases. Classification of all DNA methyltransferases". Gene. 157 (1–2): 3–11. doi:10.1016/0378-1119(94)00783-O. PMID 7607512.
  6. ^ Labahn J, Granzin J, Schluckebier G, Robinson DP, Jack WE, Schildkraut I, Saenger W (November 1994). "Three-dimensional structure of the adenine-specific DNA methyltransferase M.Taq I in complex with the cofactor S-adenosylmethionine". Proceedings of the National Academy of Sciences of the United States of America. 91 (23): 10957–61. doi:10.1073/pnas.91.23.10957. PMC 45145. PMID 7971991.
  7. ^ Kelleher JE, Daniel AS, Murray NE (September 1991). "Mutations that confer de novo activity upon a maintenance methyltransferase". Journal of Molecular Biology. 221 (2): 431–40. doi:10.1016/0022-2836(91)80064-2. PMID 1833555.
  8. ^ Adhikari S, Curtis PD (September 2016). "DNA methyltransferases and epigenetic regulation in bacteria". FEMS Microbiology Reviews. 40 (5): 575–91. doi:10.1093/femsre/fuw023. PMID 27476077.
  9. ^ Chahar S, Elsawy H, Ragozin S, Jeltsch A (January 2010). "Changing the DNA recognition specificity of the EcoDam DNA-(adenine-N6)-methyltransferase by directed evolution". Journal of Molecular Biology. 395 (1): 79–88. doi:10.1016/j.jmb.2009.09.027. PMID 19766657.
  10. ^ Maier JA, Albu RF, Jurkowski TP, Jeltsch A (December 2015). "Investigation of the C-terminal domain of the bacterial DNA-(adenine N6)-methyltransferase CcrM". Biochimie. 119: 60–7. doi:10.1016/j.biochi.2015.10.011. PMID 26475175.
  11. ^ Oliveira PH, Ribis JW, Garrett EM, Trzilova D, Kim A, Sekulovic O, et al. (January 2020). "Epigenomic characterization of Clostridioides difficile finds a conserved DNA methyltransferase that mediates sporulation and pathogenesis". Nature Microbiology. 5 (1): 166–180. doi:10.1038/s41564-019-0613-4. PMC 6925328. PMID 31768029.
  12. ^ Pósfai J, Bhagwat AS, Roberts RJ (December 1988). "Sequence motifs specific for cytosine methyltransferases". Gene. 74 (1): 261–5. doi:10.1016/0378-1119(88)90299-5. PMID 3248729.
  13. ^ a b Kumar S, Cheng X, Klimasauskas S, Mi S, Posfai J, Roberts RJ, Wilson GG (January 1994). "The DNA (cytosine-5) methyltransferases". Nucleic Acids Research. 22 (1): 1–10. doi:10.1093/nar/22.1.1. PMC 307737. PMID 8127644.
  14. ^ Lauster R, Trautner TA, Noyer-Weidner M (March 1989). "Cytosine-specific type II DNA methyltransferases. A conserved enzyme core with variable _target-recognizing domains". Journal of Molecular Biology. 206 (2): 305–12. doi:10.1016/0022-2836(89)90480-4. PMID 2716049.
  15. ^ Cheng X (February 1995). "DNA modification by methyltransferases". Current Opinion in Structural Biology. 5 (1): 4–10. doi:10.1016/0959-440X(95)80003-J. PMID 7773746.
  16. ^ Cheng X, Kumar S, Posfai J, Pflugrath JW, Roberts RJ (July 1993). "Crystal structure of the HhaI DNA methyltransferase complexed with S-adenosyl-L-methionine". Cell. 74 (2): 299–307. doi:10.1016/0092-8674(93)90421-L. PMID 8343957. S2CID 54238106.
  17. ^ Oliveira PH, Fang G (May 2020). "Conserved DNA Methyltransferases: A Window into Fundamental Mechanisms of Epigenetic Regulation in Bacteria". Trends in Microbiology. 29 (1): 28–40. doi:10.1016/j.tim.2020.04.007. PMC 7666040. PMID 32417228.
  18. ^ McClung CA, Nestler EJ (January 2008). "Neuroplasticity mediated by altered gene expression". Neuropsychopharmacology. 33 (1): 3–17. doi:10.1038/sj.npp.1301544. PMID 17728700. S2CID 18241370.
  19. ^ a b Duke CG, Kennedy AJ, Gavin CF, Day JJ, Sweatt JD (July 2017). "Experience-dependent epigenomic reorganization in the hippocampus". Learn Mem. 24 (7): 278–288. doi:10.1101/lm.045112.117. PMC 5473107. PMID 28620075.
  20. ^ "DNMT1". Gene Symbol Report. HUGO Gene Nomenclature Committee. Archived from the original on 2012-10-06. Retrieved 2012-09-27.
  21. ^ Chen T, Ueda Y, Xie S, Li E (October 2002). "A novel Dnmt3a isoform produced from an alternative promoter localizes to euchromatin and its expression correlates with active de novo methylation". J Biol Chem. 277 (41): 38746–54. doi:10.1074/jbc.M205312200. PMID 12138111.
  22. ^ "DNMT3B". Gene Symbol Report. HUGO Gene Nomenclature Committee. Archived from the original on 2012-11-20. Retrieved 2012-09-27.
  23. ^ Barau J, Teissandier A, Zamudio N, Roy S, Nalesso V, Hérault Y, et al. (November 2016). "The DNA methyltransferase DNMT3C protects male germ cells from transposon activity". Science. 354 (6314): 909–912. Bibcode:2016Sci...354..909B. doi:10.1126/science.aah5143. PMID 27856912. S2CID 30907442.
  24. ^ a b Manzo M, Wirz J, Ambrosi C, Villaseñor R, Roschitzki B, Baubec T (December 2017). "Isoform-specific localization of DNMT3A regulates DNA methylation fidelity at bivalent CpG islands". EMBO J. 36 (23): 3421–3434. doi:10.15252/embj.201797038. PMC 5709737. PMID 29074627.
  25. ^ Rose NR, Klose RJ (December 2014). "Understanding the relationship between DNA methylation and histone lysine methylation". Biochim Biophys Acta. 1839 (12): 1362–72. doi:10.1016/j.bbagrm.2014.02.007. PMC 4316174. PMID 24560929.
  26. ^ "DNMT3L". Gene Symbol Report. HUGO Gene Nomenclature Committee. Retrieved 2012-09-27.
  27. ^ Kho MR, Baker DJ, Laayoun A, Smith SS (January 1998). "Stalling of human DNA (cytosine-5) methyltransferase at single-strand conformers from a site of dynamic mutation". Journal of Molecular Biology. 275 (1): 67–79. doi:10.1006/jmbi.1997.1430. PMID 9451440.
  28. ^ Smith SS, Kaplan BE, Sowers LC, Newman EM (May 1992). "Mechanism of human methyl-directed DNA methyltransferase and the fidelity of cytosine methylation". Proceedings of the National Academy of Sciences of the United States of America. 89 (10): 4744–8. Bibcode:1992PNAS...89.4744S. doi:10.1073/pnas.89.10.4744. PMC 49160. PMID 1584813.
  29. ^ Jair KW, Bachman KE, Suzuki H, Ting AH, Rhee I, Yen RW, et al. (January 2006). "De novo CpG island methylation in human cancer cells". Cancer Research. 66 (2): 682–92. doi:10.1158/0008-5472.CAN-05-1980. PMID 16423997.
  30. ^ Ting AH, Jair KW, Schuebel KE, Baylin SB (January 2006). "Differential requirement for DNA methyltransferase 1 in maintaining human cancer cell gene promoter hypermethylation". Cancer Research. 66 (2): 729–35. doi:10.1158/0008-5472.CAN-05-1537. PMID 16424002.
  31. ^ Li E, Bestor TH, Jaenisch R (June 1992). "_targeted mutation of the DNA methyltransferase gene results in embryonic lethality". Cell. 69 (6): 915–26. doi:10.1016/0092-8674(92)90611-F. PMID 1606615. S2CID 19879601.
  32. ^ Goll MG, Kirpekar F, Maggert KA, Yoder JA, Hsieh CL, Zhang X, et al. (January 2006). "Methylation of tRNAAsp by the DNA methyltransferase homolog Dnmt2". Science. 311 (5759): 395–8. Bibcode:2006Sci...311..395G. doi:10.1126/science.1120976. PMID 16424344. S2CID 39089541.
  33. ^ "TRDMT1 tRNA aspartic acid methyltransferase 1 (Homo sapiens)". Entrez Gene. NCBI. 2010-11-01. Retrieved 2010-11-07.
  34. ^ Yang X, Han H, De Carvalho DD, Lay FD, Jones PA, Liang G (October 2014). "Gene body methylation can alter gene expression and is a therapeutic _target in cancer". Cancer Cell. 26 (4): 577–90. doi:10.1016/j.ccr.2014.07.028. PMC 4224113. PMID 25263941.
  35. ^ a b Karaca KG, Kupke J, Brito DV, Zeuch B, Thome C, Weichenhan D, Lutsik P, Plass C, Oliveira AM (January 2020). "Neuronal ensemble-specific DNA methylation strengthens engram stability". Nat Commun. 11 (1): 639. Bibcode:2020NatCo..11..639G. doi:10.1038/s41467-020-14498-4. PMC 6994722. PMID 32005851.
  36. ^ Hegde M, Joshi MB (April 2021). "Comprehensive analysis of regulation of DNA methyltransferase isoforms in human breast tumors". J Cancer Res Clin Oncol. 147 (4): 937–971. doi:10.1007/s00432-021-03519-4. PMC 7954751. PMID 33604794.
  37. ^ Oliveira AM, Hemstedt TJ, Bading H (July 2012). "Rescue of aging-associated decline in Dnmt3a2 expression restores cognitive abilities". Nat Neurosci. 15 (8): 1111–3. doi:10.1038/nn.3151. PMID 22751036. S2CID 10590208.
  38. ^ Bernstein C (2022). "DNA Methylation and Establishing Memory". Epigenet Insights. 15: 25168657211072499. doi:10.1177/25168657211072499. PMC 8793415. PMID 35098021.
  39. ^ Bayraktar G, Kreutz MR (2018). "The Role of Activity-Dependent DNA Demethylation in the Adult Brain and in Neurological Disorders". Front Mol Neurosci. 11: 169. doi:10.3389/fnmol.2018.00169. PMC 5975432. PMID 29875631.
  40. ^ Mack GS (December 2010). "To selectivity and beyond". Nature Biotechnology. 28 (12): 1259–66. doi:10.1038/nbt.1724. PMID 21139608. S2CID 11480326.
  41. ^ "EC Approves Marketing Authorization Of DACOGEN For Acute Myeloid Leukemia". 2012-09-28. Retrieved 28 September 2012.

Further reading

edit
edit
This article incorporates text from the public domain Pfam and InterPro: IPR001525
This article incorporates text from the public domain Pfam and InterPro: IPR003356
This article incorporates text from the public domain Pfam and InterPro: IPR012327
This article incorporates text from the public domain Pfam and InterPro: IPR002941
  NODES
Note 1