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In Silicodiscovery of Histone-
lysine N-methyltransferaseSETD2
             inhibitors.
         Juan Carlos Torres Sánchez1
        Gretel SaraíMontañez Próspere1
                                             1
                       Adriana O. Díaz
                                          2
                  Dr. Hector M. Maldonado
         1RISE   Program, University of Puerto Rico at Cayey;
          2Universidad  Central del Caribe, Medical School.
In Silico discovery of Histone-lysine N-methyltransferase SETD2 inhibitors.


               Outline of the Presentation

 • Background and Significance
         A. Methyltransferases
         B. Histone-lysine N Methyltransferase

 • Hypothesis
 • Methodology
 • Results
 • Conclusions
 • Future Work
 • Acknowledgments/Questions
Background and Significance
Methyltranferases:

• A methyltransferase, also known as a methylase, is a type of
  tranferase enzyme that transfers a methyl group from a donor
  molecule (usually S-adenosyl methionine; SAM) to an acceptor.

• Methylation often occurs on nucleic bases in DNA or amino acids
  in protein structures.

•    Several methyltransferases have ben identified including DNA
    (cytosine-5)-methyltransferase 1
    (DNMT1), tRNAmethyltransferase (TRDMT1) and protein
    methyltransferase (SETD2)
Background and Significance
Histone Methyltranferases (HMT):
• HMT are histone-modifying enzymes, including histone-lysine N-
  methyltransferase and histone-arginine N-methyltransferase.

• These group of enzymes catalyze the transfer of up to three methyl
  groups to lysine and/or arginine residues of histone proteins.

• Histones are highly alkaline proteins found in eukaryotic cell nuclei
  that package and order the DNA into structural units called
  nucleosomes.

• Methylation of histones is important biologically because it is the
  principal epigenetic modification of chromatin that determines gene
  expression, genomic stability, etc.
Background and Significance
Histone Methyltranferases (HMT):
• Abnormal expression or activity of methylation-regulating enzymes
  has been noted in some types of human cancers, suggesting
  associations between histone methylation and malignant
  transformation of cells or formation of tumors
• It is now generally accepted that in addition to genetic
  aberrations, cancer can be initiated by epigenetic changes in which
  gene expression is altered without genomic abnormalities.
• The protein methyltransferases (PMTs) have emerged as a novel
  target class, especially for oncology indications where specific genetic
  alterations, affecting PMT activity, drive cancer tumorigenesis.
Hypothesis


“Selective, high-affinity inhibitors of Histone-
 lysine N-methyltransferaseSETD2 can be
 identified via an In Silico approach targeting this
 protein SAM binding site”.
Objectives:
1. Identify a new target for drug development in the
   Histone-lysine N-methyltransferaseSETD2 by analysis
   of benzene mapping and the interactions of previously
   identified compounds.

1. Using information from these interactions, create
   Pharmacophore Models (LigandScout) for the selected
   target and perform a virtual pre-screening of Drug
   Databases against our model.

1. Perform a secondary screening to identify “top-hits” or
   potential lead compounds (AutoDockVina)
Methodology
Software Used:
•   PyMOL Molecular Graphics System v1.3 http://www.pymol.org
•   AutoDock (protein-protein docking software) http://autodock.scripps.edu/
•   Auto Dock Tools: Graphical Interfase for
    AutoDockhttp://mgltools.scripps.edu/downloads
•   AutoDockVina: improving the speed and accuracy of docking with a new scoring
    function, efficient optimization and multithreading. http://vina.scripps.edu/
•   LigandScout: Advanced Pharmacophore Modeling and Screening of Drug
    Databases. http://www.inteligand.com/ligandscout/


Databases Used:
•   SwissProt/TrEMBL; (Protein knowledgebase and Computer-annotated supplement
    to Swiss-Prot) http://www.expasy.ch/sprot/
•   Research Collaboratory for Structural Bioinformatics (RCSB) www.pdb.org
•   ZINC: A free database for virtual screening: http://zinc.docking.org/
Results: Pharmacophore model generation.
            3H6L.pdb               3H6L.pdb                  3H6L.pdb




         ZINC00000000           ZINC00000000              ZINC00000000




       Pharmacophore Model 01             Pharmacophore Model 02
Conclusions
• Initial analysis of the Histone-lysine N-methyltransferase SETD2 suggests
  that the binding site for the methyl donor compound SAM can be used as
  potential targets for In Silico drug discovery and development.

• Two distinct pharmacophore models where generated and used to filter
  the original database of small chemical compounds to less than 20% of
  the total number of compounds.

•   A total of 31,669 compounds where docked In Silico to the target protein
    and the results ranked according to their predicted binding energies.

• A group of drugs-like-compounds with high binding energies (less than -
  9.0 kcal/mol) were identified in the secondary screening consistent with
  the possibility of high affinity interactions.
Future Work
• Complete the screening of the lead-like database (>1.7 million
  compounds) using both Pharmacophore models.

• Evaluate results of top-hits and if appropriate use this
  information to refine the Pharmacophore model and repeat the
  screening cycle.

• Obtain/purchase some of the predicted high affinity
  compounds and test their potential as inhibitors in a bioassay.
Acknowledgments

• Dr. Maldonado

• Adriana Díaz

• Dra. Díaz

• Dra. Gonzalez
Questions?...




  Thanks for your attention.

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In silico drug discovery 2

  • 1. In Silicodiscovery of Histone- lysine N-methyltransferaseSETD2 inhibitors. Juan Carlos Torres Sánchez1 Gretel SaraíMontañez Próspere1 1 Adriana O. Díaz 2 Dr. Hector M. Maldonado 1RISE Program, University of Puerto Rico at Cayey; 2Universidad Central del Caribe, Medical School.
  • 2. In Silico discovery of Histone-lysine N-methyltransferase SETD2 inhibitors. Outline of the Presentation • Background and Significance A. Methyltransferases B. Histone-lysine N Methyltransferase • Hypothesis • Methodology • Results • Conclusions • Future Work • Acknowledgments/Questions
  • 3. Background and Significance Methyltranferases: • A methyltransferase, also known as a methylase, is a type of tranferase enzyme that transfers a methyl group from a donor molecule (usually S-adenosyl methionine; SAM) to an acceptor. • Methylation often occurs on nucleic bases in DNA or amino acids in protein structures. • Several methyltransferases have ben identified including DNA (cytosine-5)-methyltransferase 1 (DNMT1), tRNAmethyltransferase (TRDMT1) and protein methyltransferase (SETD2)
  • 4. Background and Significance Histone Methyltranferases (HMT): • HMT are histone-modifying enzymes, including histone-lysine N- methyltransferase and histone-arginine N-methyltransferase. • These group of enzymes catalyze the transfer of up to three methyl groups to lysine and/or arginine residues of histone proteins. • Histones are highly alkaline proteins found in eukaryotic cell nuclei that package and order the DNA into structural units called nucleosomes. • Methylation of histones is important biologically because it is the principal epigenetic modification of chromatin that determines gene expression, genomic stability, etc.
  • 5. Background and Significance Histone Methyltranferases (HMT): • Abnormal expression or activity of methylation-regulating enzymes has been noted in some types of human cancers, suggesting associations between histone methylation and malignant transformation of cells or formation of tumors • It is now generally accepted that in addition to genetic aberrations, cancer can be initiated by epigenetic changes in which gene expression is altered without genomic abnormalities. • The protein methyltransferases (PMTs) have emerged as a novel target class, especially for oncology indications where specific genetic alterations, affecting PMT activity, drive cancer tumorigenesis.
  • 6. Hypothesis “Selective, high-affinity inhibitors of Histone- lysine N-methyltransferaseSETD2 can be identified via an In Silico approach targeting this protein SAM binding site”.
  • 7. Objectives: 1. Identify a new target for drug development in the Histone-lysine N-methyltransferaseSETD2 by analysis of benzene mapping and the interactions of previously identified compounds. 1. Using information from these interactions, create Pharmacophore Models (LigandScout) for the selected target and perform a virtual pre-screening of Drug Databases against our model. 1. Perform a secondary screening to identify “top-hits” or potential lead compounds (AutoDockVina)
  • 8. Methodology Software Used: • PyMOL Molecular Graphics System v1.3 http://www.pymol.org • AutoDock (protein-protein docking software) http://autodock.scripps.edu/ • Auto Dock Tools: Graphical Interfase for AutoDockhttp://mgltools.scripps.edu/downloads • AutoDockVina: improving the speed and accuracy of docking with a new scoring function, efficient optimization and multithreading. http://vina.scripps.edu/ • LigandScout: Advanced Pharmacophore Modeling and Screening of Drug Databases. http://www.inteligand.com/ligandscout/ Databases Used: • SwissProt/TrEMBL; (Protein knowledgebase and Computer-annotated supplement to Swiss-Prot) http://www.expasy.ch/sprot/ • Research Collaboratory for Structural Bioinformatics (RCSB) www.pdb.org • ZINC: A free database for virtual screening: http://zinc.docking.org/
  • 9.
  • 10.
  • 11. Results: Pharmacophore model generation. 3H6L.pdb 3H6L.pdb 3H6L.pdb ZINC00000000 ZINC00000000 ZINC00000000 Pharmacophore Model 01 Pharmacophore Model 02
  • 12.
  • 13. Conclusions • Initial analysis of the Histone-lysine N-methyltransferase SETD2 suggests that the binding site for the methyl donor compound SAM can be used as potential targets for In Silico drug discovery and development. • Two distinct pharmacophore models where generated and used to filter the original database of small chemical compounds to less than 20% of the total number of compounds. • A total of 31,669 compounds where docked In Silico to the target protein and the results ranked according to their predicted binding energies. • A group of drugs-like-compounds with high binding energies (less than - 9.0 kcal/mol) were identified in the secondary screening consistent with the possibility of high affinity interactions.
  • 14. Future Work • Complete the screening of the lead-like database (>1.7 million compounds) using both Pharmacophore models. • Evaluate results of top-hits and if appropriate use this information to refine the Pharmacophore model and repeat the screening cycle. • Obtain/purchase some of the predicted high affinity compounds and test their potential as inhibitors in a bioassay.
  • 15. Acknowledgments • Dr. Maldonado • Adriana Díaz • Dra. Díaz • Dra. Gonzalez
  • 16. Questions?... Thanks for your attention.

Notas do Editor

  1. Also known as a methylasa
  2. A la izquierda la foto de la proteina. Arriba derechafoto con los benzenos. Abajo derechafoto con la droga.