Post on 09-Jan-2017
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Novel, Improved Cell-Based Assays to Enable Immunotherapy Drug
Development for Checkpoint Receptors
Jane E. Lamerdin, PhD
Director of R&D, DiscoverX
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Target & Phenotypic Platforms
Enabling Cancer Immunotherapy Drugs – From Screening to Clinics
Target-Based Platform Phenotypic Platform
PathHunter Cellular Assays BioMAP Human Primary Cell Assays
APPLICATIONS
• Screening & lead optimization
• Bioassays for potency & stability testing
• NAb assays for immunogenicity testing
APPLICATIONS
• Efficacy & biomarker selection
• Pre-clinical safety studies
• Combination studies
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Target & Phenotypic Platforms
Enabling Cancer Immunotherapy Drugs – From Screening to Clinics
Target ID and Validation
Screening & Hit
Identification
Lead Optimization & Selection
Efficacy and Biomarker Selection
Safety & Pre-clinical Studies
Clinical Combination
Studies
PathHunter® Checkpoint Assays PathHunter® Bioassays for QC Lot Release Testing
BioMAP® Oncology Systems
BioMAP® Diversity PLUS™
BioMAP® Combo ELECT
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• Harnesses the immune system to battle tumors
• Selectively activate or inhibit T cells
• Based on clinical success of molecules targeting two inhibitory receptors, CTLA4 and PD-1
• Combination therapy, personalized medicine
• Customize treatment depending on patient’s tumor type
Cancer Immunotherapy
“Scientific Breakthrough of the Year” – 2013, Science Magazine
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Targeting T Cell Activation and Inhibitory Checkpoints
Tools Are Needed to Screen for and Develop New Therapeutics
Figure from: Nature 480 480–489 (22 December 2011) doi:10.1038/nature10673
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Challenges with Checkpoint Receptors
• Difficult to create cell-based assays for checkpoint receptors
• Often needs human blood tissue
• Difficult to handle human samples
• Donor variability
• Long, complicated protocols
• Assay not specific for target receptor
Pembrolizumab
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PathHunter® Assay Technology
Enzyme Fragment Complementation (EFC)
Split β-galactosidase Enzyme
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ProLink™ (PK) Enzyme Acceptor (EA)
Inactive Fragments Active Enzyme
~40 aa peptide Large fragment Complemented Enzyme
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• PD-1 contains inhibitory motifs
• Phosphorylation by Src kinases
• SHP proteins recruited to phosphorylated motifs
• SHP-2 attenuates TCR activation
PD-1 Signaling BiologyAssay based on native receptor biology
PathHunter PD-1 assay quantifies this early activation event
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PathHunter® PD-1 Signaling Assay
Target early step in PD-1 receptor activation
Plate Jurkat PD-1 cells;
add anti-PD-1 antibodyAdd U2OS PD-L1 or
PD-L2-presenting cells
Incubate 1hr
Add Detection Reagents
Incubate 1hr
Read on Benchtop
Luminometer
Incubate 1-2hr
Simple Add and Read Protocol
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PathHunter® PD-1 Signaling Assay
Responds to Cell-presented Ligand (Co-culture with PD-L1 or PD-L2)
Co-culture with PD-L2
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PathHunter® PD-1 Signaling Assay
Rapid and Robust Response to Anti-ligand or Anti-PD-1 Antibodies
Robust inhibition in < 2hr
Inhibition with anti-PD-1 or
anti-PD-L1 antibodies
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PathHunter® PD-1 Signaling Assay PerformanceHighly Specific and Reproducible Response
RSD <4%
Highly Specific Response Excellent Reproducibility
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PathHunter® Assay Applications
Supports development of biologics and small molecules
SMALL MOLECULES• Screening & lead optimization
BIOLOGICS• Screening & lead optimization• Characterization Assays• Development of QC Lot Release Assays
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PathHunter® vs. Reporter Gene Assay
15X More Sensitive and 4X Faster
PathHunter Assay Competitor Assay
Data generated with same commercial anti-PD-1 antibody (BioLegend Cat # 329709)
Total Assay Time <5 hrs >22 hrs
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PathHunter® Checkpoint Assay Advantages
• Biologically relevant response
• Without handling difficult and donor-variable human tissue
• Easy Protocol With Fast Results
• Simple add and read protocol and results in less than 5 hours
• Multiple Applications
• Supports development of biologics and small molecules
• Highly Sensitive Response
• 15X more sensitive than other assays
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Targeting T-cell Activation and Inhibitory Checkpoints
Modulate immune response to destroy cancer cells
Activating
Receptors =
TNFR superfamily
membersSignal through
canonical and non-
canonical NF-kB
pathways
Nature 480 480–489 (22 December 2011) doi:10.1038/nature10673
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• A number of co-stimulatory receptors have been reported to signal through both canonical and non-canonical NF-kB pathways:
• BAFF
• 4-1BB
• OX40
• GITR
• Interrogate non-canonical signaling by quantifying NIK stabilization
TNFR Superfamily Receptor SignalingSignaling Through the Non-canonical NF-κB Pathway
Immunol Rev. 2012 Mar; 246(1): 125–140
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NIK is Stabilized in Response to Ligand Engagement of Endogenous TWEAK Receptors in U-2 OS Cells
• TWEAKR (Fn14) is a TNFR
family member that is up-
regulated in response to
tissue damage
• TWEAKR is a therapeutic
target in multiple inflammatory
diseases (e.g. RA, MS,
atherosclerosis) and cancer
(melanoma, glioma, etc.)
• TWEAKR is endogenously
expressed in U-2 OS cells
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NIK is Stabilized in Response to Ligand Engagement of Endogenous HVEM Receptors in U-2 OS Cells
• HVEM is a TNFR family member that elicits either a co-
stimulatory or inhibitory signal depending on the ligand
• HVEM is endogenously expressed in U-2 OS cells
• LIGHT delivers a co-stimulatory signal to HVEM+ cells,
resulting in stabilization of NIK
APC (naiive T cells) T cell
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NIK is Stabilized in Response to Activation of Endogenous CD40 in U-2 OS Cells by Soluble CD40 Ligand
Bremer, E., ISRN Oncology 2013, Article ID 371854
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NIK is Stabilized in Response to Activation of Endogenous CD40 in U-2 OS Cells by Soluble and Oligomerized CD40 Ligand
Soluble CD40L
Oligomerized CD40L
Bremer, E., ISRN Oncology 2013, Article ID 371854
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NIK is Stabilized in Response to Activation of Endogenous CD40 in U-2 OS Cells by CD40 Ligand and Agonistic Antibodies
Soluble CD40L
Oligomerized CD40L
Agonistic CD40 Ab
Bremer, E., ISRN Oncology 2013, Article ID 371854
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NIK is Stabilized in Response to OX40 Ligand Engagement
• Exogenously expressed OX40 in
U-2 OS NIK Signaling Cell Line
• OX40 assay responds to soluble
ligand and agonistic antibodies
• Amenable to testing in 96-well or
384-well format (to conserve
antibodies)
96-well
384-well
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• Simple and biologically relevant assay
• Gain of signal assay
• Robust response over broad incubation time period (4-6hr)
• Compatible with biologics and small molecules
• Applicable to diverse TNFR family members
PathHunter® NIK Assay Benefits
Measures Activation of Endogenous or Exogenously Expressed TNFR Superfamily Receptors with Soluble Ligand and Agonistic Antibodies
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• Blockade of PD-1 and other inhibitory receptors
• CTLA-4, TIM-3, LAG3, TIGIT, CD244, CD160
• PD-1 blockade in combination with immunostimulators
• Anti-OX40, anti-CD137, ICOS, TLR ligands, IL-2
• PD-1 blockade in combination with small molecules or other targeted inhibitors
• e.g. angiogenesis inhibitors, HDAC or PARP inhibitors
• PD-1 blockade in combination with vaccines, CAR-T or oncolytic viruses
Immunotherapy’s Next Wave: Combination Therapy
Monospecific vs Bi-specific antibodies
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Assay Concept for Bi-specific Assays
Bi-specific Antibody
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Bi-specific Assays Developed for Immune Checkpoints
Immune Checkpoint Bi-specific Assay
• PD-1 / TIM3
• TIM3 / CEACAM
• PD-1 / LAG3
• PD-1 / TIGIT
• PD-1 / CTLA4
• PD-1 / 4-1BB
Examples of Available Bi-specific
Pools / Clones :
1 0 -1 1 1 0 -1 0 1 0 -9 1 0 -8 1 0 -7 1 0 -6 1 0 -5 1 0 -4
0
1 0 0 0 0 0
2 0 0 0 0 0
3 0 0 0 0 0
4 0 0 0 0 0
B is p e c if ic A n tib o d y [g /m L ]
Dim
eriz
ati
on
Sig
na
l (R
LU
)
A n tib o d y 1
A n tib o d y 2
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VISTA Dimerization Assay• VISTA is a negative checkpoint regulator that suppresses T-
cell activation and is highly expressed within the tumor micro-
environment.
• VISTA is expressed primarily on hematopoietic cells
• VISTA blockade may offer an immunotherapeutic strategy for
human cancer, especially in combination
• VISTA is related to PD-L1; currently the receptor for VISTA is
unknown
• Dimer assay provides tool to rank order antibodiesFigure from Cancer Immunol Res (2014); 2(6): 510-517
Highly Specific Response to
anti-VISTA antibodies
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TIM3 Dimerization Assay
• TIM3 is a negative checkpoint regulator expressed on
multiple hematological cells
• Recognizes ligands highly expressed on apoptotic cells,
leading to phagocytosis of dying cells
• Dimer assay provides tool to rank order antibodies
Figure from Science Webinar Series, part 5: Gordon J. Freeman, Ph.D.
APC T cell Highly Specific Response to
anti-TIM3 antibodies
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Assays for CSF1 (M-CSF) and GM-CSF
• Cell line responds robustly to M-CSF (CSF1) and IL-34
• Anti-M-CSF antibodies will lead to inhibition of ligand-induced dimerization
Cytokine immunotherapy with GM-CSF:
induces potent tumor-specific systemic immune
responses
~30 assays available for cytokines and interleukins
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• SH2 recruitment (signaling) assays for inhibitory receptors• Clone available for PD-1
• Assays for other targets coming soon
• Custom projects possible for additional novel checkpoint targets
• Assays for co-stimulatory receptors• Assays for OX40, TWEAKR, HVEM and CD40 are available
• Additional co-stimulatory receptors assays in progress
• Assays for Bi-specific molecules
Summary
Multiple Assay Formats for Immune Checkpoint Receptors
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Thank you for your attention!
Learn more at www.discoverx.com/checkpoint
Contact info@discoverx.com for additional information