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FRAGMENT-BASED DRUG
DISCOVERY
MO.SHAHANAWAZ
2200102926
M.PHARM (PHARMACEUTICAL CHEMISTRY)
FRAGMENT-BASED DRUG DISCOVERY
 The fragment based drug design starts with the identification of fragments or low
molecular weight compounds that generally bind with weak affinity to the target of
interest.
 The fragments that form high quality interactions are then optimized to lead
compounds with high affinity and selectivity.
 Fragment based screening and optimization methods have achieved credible success
in many drug discovery projects with one approved drug and many more compounds
in clinical trials.
 Fragment based drug design has emerged as an effective alternative to high
throughput screening for the identification of lead compounds in drug discovery.
LIPINSKI RULE OF
FIVE
Not more than 10
Hydrogen bond
acceptors
Not more than 5
Hydrogen bond
donor
Molecular
weight less
than 500-D
C-Log P not
greater than 5
STEP INVOLVED IN FBDD
FRAGMENT LIBRARY
 The term of fragment indicates that the molecular weight of compounds is relatively
small, which gives rise to high ligand efficiency and provides more opportunities for
growing the hits.
 Fragments should follow the rules-of-three.
I. Compounds have a molecular weight less than 300 Da.
II. ClogP value less than three.
III. Compounds have less than three hydrogen donors and acceptors .
Researchers usually have their own customized libraries in FBDD and molecular weight of
a fragment can be above 300 Da.
SCREENING METHODS
For screening of fragment following methods are used
1-Differential Scanning Fluorimetry (DSF)-Differential scanning fluorimetry is to
measure thermally induced protein denature in the presence of a fluorescence dye
such as Synpro Orange that binds to hydrophobic regions of a protein.
 The method is based on a phenomenon that stability of most proteins decreases
when the environmental temperature (Tm) is increased.
 The Tm at which the amounts of folded and unfolded proteins are equal is termed
as melting Tm.
 The compound binding to a protein enhances the Tm of a protein and such a
compound is then considered as a positive hit.
2-Isothermal Titration Calorimetry (ITC)-Isothermal titration calorimetry is a
powerful technique to measure binding affinity, binding and enthalpy changes of
molecular interactions between a protein and a protein/ligand in solution.
3-Surface Plasmon Resonance (SPR)-Surface plasmon resonance has been widely
applied in probing protein–protein, protein–ligand, protein–DNA/RNA, and DNA–DNA
interactions.
4-NMR Spectroscopy-. This technique is sensitive enough to identify fragments with
different binding affinities (from nanomolar to millimolar). Compared with other
methods, NMR screening gives rise to less false positive hits and a mixture of
fragments can be screened.
5-X-Ray Crystallography-X-ray crystallography is a powerful tool to obtain structures
of proteins and complexes at high resolutions. It plays essential roles in structure-
based drug discovery
COMPOUND OPTIMIZATION
 As fragments usually bind weakly to targets and exhibit no potent inhibitory effect
on the activity of the targets, further chemical modification of the hits is required
in hit-to-lead step.
 In this procedure, hits will be developed into leads which bind to the target with
higher affinities and exhibit potent activities against the target.
 Three strategies namely fragment growing, fragment hopping, and fragment
linking are frequently utilized.
Growing of Fragment Hits
 Fragment growing is the most commonly used strategy to grow fragments into
compounds with higher molecular weights and higher potencies.
 Various chemical groups can be added to the building block (hit) to improve its
potency.
 Fragment merging or scaffold hopping- is another strategy to grow fragments
into potent compounds.
 This strategy is based on condition that the identified fragments have an
overlapped binding site. Potent compounds can be developed by
combining/merging chemical features of two or more fragments.
 Fragment linking- is considered as the most powerful way to develop potent
inhibitors from fragments.
 A lead compound can be developed by linking two or more fragments together.
 The challenge in this strategy is to identify fragments that are in close proximity
and the introduced linker has no negative effect on the activity of the fragment.
TARGETS FOR FBDD
 Fragment-based drug discovery is mainly applicable to target based drug
discovery.
 Druggability of a target is always analyzed in target-based drug discovery
projects and is utilized to predict possibility of developing drugs by identifying a
pocket favoring binding to small-molecule compounds
EXAMPLES OF SUCCESSFUL DRUGS THAT WERE DISCOVERED USING
FBDD
 Venetoclax: Venetoclax is a drug used to treat chronic lymphocytic leukemia (CLL). It was
discovered using FBDD and works by inhibiting the B-cell lymphoma-2 (BCL-2) protein,
which is overexpressed in CLL.
 Rucaparib: Rucaparib is a drug used to treat ovarian cancer. It was discovered using FBDD
and works by inhibiting the poly (ADP-ribose) polymerase (PARP) enzyme, which is
overexpressed in some types of cancer.
 Alectinib: Alectinib is a drug used to treat non-small cell lung cancer (NSCLC). It was
discovered using FBDD and works by inhibiting the anaplastic lymphoma kinase (ALK)
protein, which is overexpressed in some types of NSCLC.
REFERENCES
 Abdulmalek, A. B., Sufyan, M. A., Abdulrahman, K. A., and Mohammed, A. K. (2020).
Fragment-based discovery of potential anticancer lead: computational and in vitro
studies. Curr. Comput. Aid. Drug Design 16, 1–9. doi: 10.2174/
1573409916666200620195025
 Akter, M., Drinkwater, N., Devine, S. M., Drew, S. C., Krishnarjuna, B., Debono, C. O., et al.
(2019). Identification of the binding site of apical membrane antigen 1 (AMA1) inhibitors
using a paramagnetic probe. ChemMedChem 14, 603–612. doi:
10.1002/cmdc.201800802
 Alvarado, C., Stahl, E., Koessel, K., Rivera, A., Cherry, B. R., Pulavarti, S. V. S. R. K., et al.
(2019). Development of a fragment-based screening assay for the focal adhesion
targeting domain using SPR and NMR. Molecules 24, 3352. doi:
10.3390/molecules24183352
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FRAGMENT-BASED DRUG DISCOVERY.pptx

  • 2. FRAGMENT-BASED DRUG DISCOVERY  The fragment based drug design starts with the identification of fragments or low molecular weight compounds that generally bind with weak affinity to the target of interest.  The fragments that form high quality interactions are then optimized to lead compounds with high affinity and selectivity.  Fragment based screening and optimization methods have achieved credible success in many drug discovery projects with one approved drug and many more compounds in clinical trials.  Fragment based drug design has emerged as an effective alternative to high throughput screening for the identification of lead compounds in drug discovery.
  • 3.
  • 4. LIPINSKI RULE OF FIVE Not more than 10 Hydrogen bond acceptors Not more than 5 Hydrogen bond donor Molecular weight less than 500-D C-Log P not greater than 5
  • 6. FRAGMENT LIBRARY  The term of fragment indicates that the molecular weight of compounds is relatively small, which gives rise to high ligand efficiency and provides more opportunities for growing the hits.  Fragments should follow the rules-of-three. I. Compounds have a molecular weight less than 300 Da. II. ClogP value less than three. III. Compounds have less than three hydrogen donors and acceptors . Researchers usually have their own customized libraries in FBDD and molecular weight of a fragment can be above 300 Da.
  • 7. SCREENING METHODS For screening of fragment following methods are used 1-Differential Scanning Fluorimetry (DSF)-Differential scanning fluorimetry is to measure thermally induced protein denature in the presence of a fluorescence dye such as Synpro Orange that binds to hydrophobic regions of a protein.  The method is based on a phenomenon that stability of most proteins decreases when the environmental temperature (Tm) is increased.  The Tm at which the amounts of folded and unfolded proteins are equal is termed as melting Tm.  The compound binding to a protein enhances the Tm of a protein and such a compound is then considered as a positive hit.
  • 8. 2-Isothermal Titration Calorimetry (ITC)-Isothermal titration calorimetry is a powerful technique to measure binding affinity, binding and enthalpy changes of molecular interactions between a protein and a protein/ligand in solution. 3-Surface Plasmon Resonance (SPR)-Surface plasmon resonance has been widely applied in probing protein–protein, protein–ligand, protein–DNA/RNA, and DNA–DNA interactions. 4-NMR Spectroscopy-. This technique is sensitive enough to identify fragments with different binding affinities (from nanomolar to millimolar). Compared with other methods, NMR screening gives rise to less false positive hits and a mixture of fragments can be screened. 5-X-Ray Crystallography-X-ray crystallography is a powerful tool to obtain structures of proteins and complexes at high resolutions. It plays essential roles in structure- based drug discovery
  • 9. COMPOUND OPTIMIZATION  As fragments usually bind weakly to targets and exhibit no potent inhibitory effect on the activity of the targets, further chemical modification of the hits is required in hit-to-lead step.  In this procedure, hits will be developed into leads which bind to the target with higher affinities and exhibit potent activities against the target.  Three strategies namely fragment growing, fragment hopping, and fragment linking are frequently utilized.
  • 10. Growing of Fragment Hits  Fragment growing is the most commonly used strategy to grow fragments into compounds with higher molecular weights and higher potencies.  Various chemical groups can be added to the building block (hit) to improve its potency.  Fragment merging or scaffold hopping- is another strategy to grow fragments into potent compounds.  This strategy is based on condition that the identified fragments have an overlapped binding site. Potent compounds can be developed by combining/merging chemical features of two or more fragments.
  • 11.  Fragment linking- is considered as the most powerful way to develop potent inhibitors from fragments.  A lead compound can be developed by linking two or more fragments together.  The challenge in this strategy is to identify fragments that are in close proximity and the introduced linker has no negative effect on the activity of the fragment. TARGETS FOR FBDD  Fragment-based drug discovery is mainly applicable to target based drug discovery.  Druggability of a target is always analyzed in target-based drug discovery projects and is utilized to predict possibility of developing drugs by identifying a pocket favoring binding to small-molecule compounds
  • 12. EXAMPLES OF SUCCESSFUL DRUGS THAT WERE DISCOVERED USING FBDD  Venetoclax: Venetoclax is a drug used to treat chronic lymphocytic leukemia (CLL). It was discovered using FBDD and works by inhibiting the B-cell lymphoma-2 (BCL-2) protein, which is overexpressed in CLL.  Rucaparib: Rucaparib is a drug used to treat ovarian cancer. It was discovered using FBDD and works by inhibiting the poly (ADP-ribose) polymerase (PARP) enzyme, which is overexpressed in some types of cancer.  Alectinib: Alectinib is a drug used to treat non-small cell lung cancer (NSCLC). It was discovered using FBDD and works by inhibiting the anaplastic lymphoma kinase (ALK) protein, which is overexpressed in some types of NSCLC.
  • 13. REFERENCES  Abdulmalek, A. B., Sufyan, M. A., Abdulrahman, K. A., and Mohammed, A. K. (2020). Fragment-based discovery of potential anticancer lead: computational and in vitro studies. Curr. Comput. Aid. Drug Design 16, 1–9. doi: 10.2174/ 1573409916666200620195025  Akter, M., Drinkwater, N., Devine, S. M., Drew, S. C., Krishnarjuna, B., Debono, C. O., et al. (2019). Identification of the binding site of apical membrane antigen 1 (AMA1) inhibitors using a paramagnetic probe. ChemMedChem 14, 603–612. doi: 10.1002/cmdc.201800802  Alvarado, C., Stahl, E., Koessel, K., Rivera, A., Cherry, B. R., Pulavarti, S. V. S. R. K., et al. (2019). Development of a fragment-based screening assay for the focal adhesion targeting domain using SPR and NMR. Molecules 24, 3352. doi: 10.3390/molecules24183352