The Impact of Genomics on Drug Discovery

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The Impact of Genomics on Drug Discovery

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Title: The Impact of Genomics on Drug Discovery

1
The Impact of Genomics on Drug Discovery

Functional Genomics andPharmacology
B. Monia (11/14 11/21)
New Approaches to Drug Discovery B.Monia (11/21)
Evaluation of Drugs in the Clinic J. Tami (11/28)
Pharmacogenomics J. Tami (12/5)

2
Functional Genomics and Pharmacology- Agenda
from Last Time -

The Human Genome Project (HGP)
Paradigm shifts in Drug Discovery resulting from
the HGP and other Genome Projects.
Target Validation The new unmet need for Drug
Discovery
Correlative Approaches to Target Validation
Comparative Genomics
Microarrays
Proteomics

3
Drug Discovery in the Post-Genomics Era Part
II- Agenda for Today -

Functional Genomics (cont.)
Causative Approaches to Target Validation
Overexpression Systems
Gene Ablation/Transgenic Animals
Small Molecule Inhibitors
Antisense
Interference RNA
New Approaches to Drug Discovery
High-Throughput Screening and Structure-based
Design
Antibodies
Protein Therapeutics
Antisense

4
Causative Approaches for Target Validation-
Reverse Genetics -
mAb
GeneKnockouts
OverexpressionSystems
DNA
RNA
Small Molecule Inhibitor
Protein
?
RNA Degradation (e.g., RNase H)Modulation of
SplicingArrest of Translation
?
RNAi
AntisenseOligonucleotides
5
Table 1. A comparison of different experimental
approaches for modulating the function of cell
signaling molecules
ProbabilityofSuccess
Relevanceto DrugDiscovery
Potentialfor DrugDevel.
RequiredResources
Method
Versatility
Specificity
Cost
OverexpressionSystems
High
Low toModerate
Moderate
Low
Low toModerate
Low
Low
Gene Knockouts(Mammalian)
High
High
High
High
Moderate
Low
None
Gene Knockouts(Non-Mammalian)
High
High
Moderate
Moderate
High
Low
None
Small MoleculeInhibitors
Low
Low
High
High
Low
High
Yes
MonoclonalAntibodies
Low
High
Moderate
High
Moderate
High
Yes
AntisenseOligonucleotides
High
High
Low toModerate
Low toModerate
High
High
Yes
InterferenceRNA
High
High
Low toModerate
Low toModerate
?
?
None (?)
6
Mouse Transgenic and Gene Knockout Models

Transgenic technology involves expressing foreign
genes in the mouse.
Foreign DNA is introduced into fertilized mouse
eggs by microinjection.
The gene knockout procedure involves inactivating
(Knocking out) genes in the mouse.
Genes are isolated, inactivated, and introduced
into embryonic stem (ES) cells.
ES cells are derived from early mouse embryos and
have the capacity to contribute genetically to
the complete development of the animal (both
somatic and germ-cell contributions).
Mice resulting from transgenic and gene knockout
experiments develop, are usually born, bred and
analyzed for the effects of gene
overexpression/inactivation.
May require the animals to be heterozygous for
the gene of interest in knockout studies.
New developments using specialized gene
regulatory elements
Conditional gene expression (e.g., diet-induced).
Tissue-specific expression (e.g., liver).

7
Additional Genetic Models for Functional Genomics

A variety of other model systems are being
employed using gene knockout approaches.
Yeast (e.g., S. cerevisiae)
Fly (e.g., Drosophila)
Plants (e.g., Arabidopsis)
Worm (C. elegans)
Caenorhabditis elegans (roundworm) in particular
has received a great deal of attention. Offers
many advantages
Multicellular organism with a defined cell number
at maturity (959).
Genome sequencing completed (2769 genes, 6
chromosomes).
Shares many of the essential biological
characteristics of humans.
Sexual reproduction
Development
Nerve function (with a brain)
Signaling pathways
Simple to use
Grows on petri dish (traditional genetic
selection procedures)
Transparent body visible with microscope
Average life span 2-3 weeks
Systematic gene ablation is straightforward.

8
Genetic Models for Functional Genomics-
Limitations -

Labor intensive/long periods of time required
(for mouse).
Phenotypic results may not reflect human biology.
Role of a gene in development vs
post-development.
Role of a gene in model organisms vs humans.
Phenotypic results may not reflect pharmacology.
Drugs do not Knockout gene products.
Drugs modulate protein activity not protein
levels.
Structural vs enzymatic roles of proteins.

9
Antisense Technology is Based on Simple
Watson-Crick Hybridization Mechanisms
Protein
Transcription
Antisense Hybridization
Antisense Suppression
Uracil
Adenine
Guanine
Cytocine
mRNA/OligonucleotideDuplex
DNADuplex
mRNA
10
Watson-Crick Binding of Antisense Inhibitor to RNA
RNA Target
Antisense Oligonucleotide
11
History Lesson

The starting point for antisense technology
occurred in the mid 1970s with the discovery of
small RNA molecules in bacteria and viruses that
regulate DNA replication and RNA processing
through antisense hybridization mechanisms
(Tomizawa and colleagues at the NIH).
A few hundred base pairs in length.
Transcribed from endogenous DNA sense strand.
The initial work of Tomizawa led to the concept
of antisense RNA expression vectors that were
first studied by Izant and Weintraub in the mid
1970s.
Recombinant DNA technology exploited.
Expression vectors that produce antisense RNA in
cells.
Isolated antisense RNA injected into cells.
The concept of using short (15-25 bases),
synthetic strands of complementary DNA to
hybridize with RNA and block mRNA function was
first tested in the late 1970s by Zamecnik and
Stephenson.
DNA synthesizers as key breakthroughs.
Viruses as targets followed by cellular targets.

12
What were the initial major hurdles for antisense
technology?

Understanding how oligonucleotides suppress gene
expression (Mechanisms of action).
Medicinal chemistry of oligonucleotides.
Metabolism
Affinity
Synthesis
Understanding oligonucleotide pharmacokinetics.
Toxicology of oligonucleotides.
Understanding anomalous behavior of
oligonucleotides.

13
Antisense Mechanisms of Action
eIFs
60S
5? UTR
60S
Intron
Coding
Coding
AAAAAn
40S
40S
AUG
3? UTR
CAP
RNaseH-MediatedDegradationof (pre)/mRNA
SplicingModulation
TranslationalArrest

Regulate
Inhibit

14
Medicinal Chemistry of Antisense Oligonucleotides
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15
Antisense Specificity and Breadth - RNase H
Dependent Mechanism -
Control
Control
21959
18259
c-Jun
None
None
c-Fos
A-raf
B-raf
C-raf
c-Jun
A-raf mRNA
JNK-1
c-Fos
B-raf mRNA
JNK-2
G3PDH
C-raf mRNA
G3PDH
Kinases (RAF)
Transcription Factors
Kinases (JNK)
Control
Control
Control
Control
Control
Control
TRAF2
TRAF6
None
H-ras
K-ras
?i2
?i3
?i1
G?i1
Ha-rasmRNA
TRAF2
G?i2
Ki-rasmRNA
TRAF6
G?i3
G3PDHmRNA
G3PDH
G3PDH
Heterotrimeric G-Proteins
Adaptor Proteins
Low MW G-Proteins
16
Antisense Specificity and Versatility In Vivo-
Intravenous Administration -
Control ASO
JNK 1 ASO
JNK 2 ASO
p38 ASO
No ASO
JNK 1
JNK 2
p38a
120
120
JNK-1
100
JNK-2
100
p38?
80
80
Target mRNA Levels( control)
60
60
40
40
20
20
0
0
CTL
JNK1ASO
JNK2ASO
p38?ASO
CTL
JNK-1ASO
JNK-2ASO
P38?ASO
Liver
Adipose Tissue
17
Antisense Technology for Functional Genomics

Advantages
Offers excellent specificity (in general)
All targets are approachable
Fast, efficient
Acts pharmacologically
Works in cell culture and in animals
Drugable
Disadvantages
Anomalous behavior under certain circumstances.
Not all cell types are easily transfectable in
vitro.
Not all tissues/cell types in animals
approachable.
Not inexpensive. Advanced chemistries not easily
accessible.

18
RNA Interference A New Functional Genomics Tool

RNA Interference (RNAi) is the process where the
introduction of double-stranded RNA into a cell
inhibits gene expression in a sequence-dependent
fashion.
First discovered in C. elegans in the mid 1990s.
RNA duplexes 20-30 bases in length injected into
worms or ingested by worms results in the
complete silencing of a homologous gene.
Soaking worms in RNAi also induces gene
silencing.
RNAi activities have now been demonstrated in
many other organisms inlcuding plants, flies and
mammals.

19
RNA Interference A New Functional Genomics Tool

Mechanism of RNAi silencing poorly understood.
Requires target RNA synthesis which becomes
cleaved in the region corresponding to the RNAi.
Input RNAi gets processed to 19-20 nucleotide
guide RNAs (siRNAs) with 2 nucleotide 3?
overhangs.
siRNAs may be amplified by RNA-dependent
polymerases.
siRNA duplexes then bind to a nuclease complex to
form a RNA-Induced Silencing Complex (RISC).
Responsible for target RNA cleavage.
Many of the key genes/proteins involved in the
RNAi process are being rapidly identified in C.
elegans.
RNAi as a tool for functional genomics is
receiving a great deal of attention.
One-third of the genes in the C. elegans genome
have been subjected to RNAi silencing.
Can RNAi be a new approach for therapeutics?

20
A Model for RNA Interference
Protein or RNPcofactor
dsRNA
Cleavage(shortening)
siRNA
Target RNA
RISC
Cleaved ormodifiedtarget RNA
Additional cellulardegradation mechanisms?
Degraded target RNA
21
New Approaches to Drug Discovery- Why the need? -

Progress in the discovery of new therapeutic
agents for the treatment of chronic,
life-threatening diseases has been disappointing.
Poor understanding of the molecular basis of
diseases.
Inadequate technologies available to maximize
drug discovery (innovation).
New approaches based on a firm molecular
understanding of disease was greatly needed.
New technologies that could produce drugs in
non-traditional ways was greatly needed.

22
483
23
Small Molecule Drugs- Drugable vs
Non-Drugable Protein Targets -
Drugable AcceptableSpecificity
Non-Drugable

Some proteins with intrinsicenzymatic activity.
Some cell surface/nuclearhormone receptors.

Everything else

5
Drugable withSmall Molecules
24
High-Throughput Screening for Drug Discovery - I

High-throughput screening (HTS) is the process by
which large numbers of compounds can be tested,
in an automated fashion, for activity as
inhibitors (antagonists) or activators (agonists)
of a particular target.
Result of advances in instrumentation
engineering(e.g., robotics) and bioinformatics.
Ten-twenty thousand compounds per day.
Typically performed on 96-well micortitre plates.
The primary goal of HTS is to identify
high-quality leads and to provide directions
for their optimization. Requires follow-up
optimization (SAR).
HTS provides leads only because it cannot
evaluate
bioavailability
pharmacokinetics
toxicity
specificity

25
High-Throughput Screening for Drug Discovery - II

HTS requires four basic elements
suitable compound libraries
assay method configured for automation
robotics workstation
computerized system capable of handling the data
Two general types of assays are employed
Cell-free assays
ligand-receptor (peptide) interactions
proximity-dependent fluorescence transfer
Cell-based assays
2nd-messenger levels (e.g., Ca2, cAMP)
Receptor gene expression
Successes
Cyclosporin A (organ transplant)
Mevastation (Lipoprotein metabolism)

26
High-Throughput Screening for Drug Discovery - III

Structure-based Drug Design
Following identification of a lead from HTS,
applying techniques to determine the
3-dimensional structure of the target protein
bound to the lead drug is being commonly employed
today for lead optimization.
Used mainly to improve binding affinity and
specificity.
Major advances in technology are making
structure-based drug design a routine component
to drug discovery.
Improved X-ray detectors
Better computers and graphics
Multidimensional NMR
Limitations of HTS
The likelihood of success in finding a lead that
eventually evolves into a drug is still low.
Expensive and time-consuming to develop HTS
assays and to perform follow-up lead
optimization.
Few biological processes are amenable to HTS.

Lead Optimization
Structure-based
SAR

TargetValidation
Optimized Drug
HTS
EstablishHTS Assays
27
Monoclonal Antibody Therapy - I

General Aspects
Monoclonal Antibody Therapies (MAT) is based on
the breakthrough findings of Kohler and Milstein
that monoclonal antibodies (mAbs) of a given
specificity could be obtained by fusing an
antibody producing B-cell with an immortalized
myeloma cell.
Hybridoma cells
Produce specific mAbs in unlimited quantities
Has revolutionized the biological sciences
(diagnostics/therapeutics).
MAT was touted as The Magic Bullet for human
therapeutics gt 25 years ago.
Therapeutic results were disappointing until
recently.
Two major hurdles were encountered.
Biologic activity in humans severely limited due
to the hosts immune response to foreign mAbs
(production of human antimouse Abs). Causes
neutralization of activity and toxicity.
Large-scale production

28
Hybridoma Technology
Immunizationwith Ag
Antibody Response/ Characterization
Isolation/Clonal Selection of B-Cells (spleen)
Immortalizationby fusion withmyeloma cells
Hybridoma
mAb Production
29
Monoclonal Antibody Therapy - II

Approaches to reduce or eliminate human
anti-mouse antibodies (mAb engineering).
Chimeric Antibodies
Cloned antibody genes are generated in which the
variable regions from the original mouse mAb are
combined with human antibody-constant regions.
Highly effective in reducing human anti-mouse
antibodies (HAMA). However, the variable
(Ag-recognition) domains are still foreign HAMA
often still occurs neutralizing efficacy.
Primatized Antibodies
Chimeric antibody approach in which
primate-derived variable regions with human
antibody constant regions.
Very time-consuming. Reduces immunogenicity to
human host further, but host reactions still
occur.

30
Monoclonal Antibody Therapy - III

Humanized mAbs
All portions of the mAb not required for antigen
binding, including framework residues in the
variable region, are replaced with human
sequences.
Gene engineering, expression, evaluation
lt 10 of optimized mAb retains mouse sequence
Highly-effective (but time-consuming) approach
New approaches under development
Phage-display libraries expressing human VH and
VL chains are assembled into libraries and
expressed as combinatorial matrices.
Assayed for immunoreactivity against antigen of
interest.
Transgenic Mouse Approach
A procedure in which the endogenous mouse Ig gene
loci is replaced by homologous recombination with
their human homologs.
Immunization of transgenic mouse followed by
standard hybridoma procedures produces a fully
humanized mAb.

31
Monoclonal Antibody Therapy - Successes I

Organ Transplantation
Rejection of allografts is an immunological
response exerted primarily by T-cells. mAb
approaches against T-cell antigens has proven
effective.
CD25 (IL2-Receptor ? chain). Highly effective
approach for the prevention of graft rejection
episodes and graft loss (e.g., renal).
basiliximab (chimeric)
dacliximab (humanized)
Coronary Artery Disease
Atherosclerotic lesions (plaques) involve
platelet aggregation followed by coagulation and
thrombus formation. Platelet receptors involved
in early steps of plaque formation.
basis of one-aspirin-a-day concept
limited efficacy in preventing platelet
aggregation
Abciximab (chimeric mAb) has been
developed/approved as an effective treatment for
the prevention of thrombosis and plaque formation
in high risk patients.
Targets the platelet receptors ?2,6?3/?V?3
(integrins)
Prevents platelet aggregation

32
Monoclonal Antibody Therapy Successes II

Rheumatologic and Autoimmune Diseases
TNF? is a proinflammatory cytokine that has been
implicated as a causal factor in a variety of
inflammatory diseases including Rheumatoid
Arthritis.
Infliximab is a chimeric mAb targeted to TNF?.
Has displayed remarkable activity against
Rheumatoid Arthritis and other inflammatory
diseases (Crohns Disease).
Approved in 1998. First for Crohns Disease now
R.A.
Cancer
Most intensively studied area (25 years of
research).
Cancer poses the highest hurdles. Two major
successes in recent years.
Also being evaluated in modified versions
involving the conjugation to radio-ionizing
particles, immunotoxins, immunoliposomes.

33
Monoclonal Antibody Therapy Successes III-
Cancer Cont. -

Rituximab (chimeric mAb)
Targets CD20 a cell surface protein expressed
exclusively on B cells.
Approved for the treatment of B cell malignancies
(NHL, CLL, ALL).
Trastuzumab (humanized mAb)
Her2 is a form of the EGF-Receptor that undergoes
amplification in approximately 25 of breast
cancers.
1st identified as a rat oncogene called neu
(HER2/neu)
Patients with amplified HER2 expression suffer a
very poor prognosis.
Trastuzumab (Herceptin) has displayed impressive
activity against HER2 breast cancer both alone
and in combination.
Improved response rates and survival
Approved in 1998
Under further evaluation to optimize dosing and
expand patients population.
New versions under development (e.g., Herceptin
conjugates with immunotherapy/radiation).

34
Protein Therapeutics - I

The application of human proteins, or derivatives
thereof, directly as drugs for the treatment of
disease.
Full-length proteins or peptide derivatives
Most commonly are derived from naturally
occurring secreted proteins that contain
consensus peptide cleavage sites and signal
sequences.
These consensus sequences are being used to fish
out and identify potentially novel protein
therapeutics from the HGP.
Therapeutic proteins are expressed in a suitable
host (e.g., yeast) and purified to very large
quantities for therapeutic applications (i.e.,
tons).
Notable successes have been achieved in the
Pre-Genome era.
Insulin and diabetes
Growth hormone and hypopituitary dwarfism
Interferon-? and hepatitis C
An explosion of new drugs based on Protein
Therapeutics is expected as a result of the HGP
(and related genome projects) and because of
advances in recombinant DNA technology.

35
Protein Therapeutics - II

Challenges for Protein Therapeutic approaches
Gene Identification
Bioavailability (absorption), distribution and
metabolism (PK)
Acceptably convenient modes of administration
Manufacturing
Modified forms of proteins and peptides often
need to be developed to make them useful as
drugs.
SAR involving amino acid substitutions and
deletions (e.g., insulin)
Conjugating to chemicals such as polyethylene
glycol
Pegylated proteins are protected from proteolysis
and display longer plasma half-lives than
unpegylated forms.
Conjugating to other proteins or peptides
Conjugation to human serum albumin using
recombinant DNA technology provides a sustained
plasma half-life.
Formulations

36
(No Transcript)
37
Properties of Modified Insulins
HMR 1964
Glargine
Onset of Actions (Hrs)
1.11
0.71
Duration of Action (Hrs)
22.8
13.8
Peak Effect (Hrs)
Peakless
7.5
38
Protein Therapeutics - III- New Drugs on the
Horizon Based on Genomics -

Osteoprotegrin (Amgen) An inhibitor of
osteoclast activity for the treatment of
osteoporosis (Phase 2).
Pegasys (Roche) New form of ?-interferon for
the treatment of viral infection (Phase 1).
SD-01 (Amgen) Pegylated granulocyte-colony
stimulating factor for lymphocyte/stem cell
mobilization (Phase 1).
Repifermin (SKB) Keratinocyte growth factor 2
as a stimulator of wound healing (Phase 2).
Xigris (Lilly) Protein C for the treatment of
Sepsis (Phase 3).

39
Antisense Technology is Based on Simple
Watson-Crick Hybridization Mechanisms
Protein
Transcription
Antisense Hybridization
Antisense Suppression
Uracil
Adenine
Guanine
Cytocine
mRNA/OligonucleotideDuplex
DNADuplex
mRNA
40
Critical Factors to be Considered for Optimizing
Antisense Efficacy

Medicinal Chemistry of Oligonucleotides
Affinity Potency
Toxicological considerations
Metabolism
Pharmacokinetics
Selection of Optimized Antisense Sequences
Small of ASOs actually bind to target RNA
Extensive screening often required
Choice of Terminating Mechanism (e.g., RNaseH)
In-depth Understanding of ASO Pharmacokinetics
Tissue/cellular distribution
Pharmacokinetic/Pharmacodynamic relationships

41
Antisense Drug Discovery (Therapeutics)-
Shortening the Timelines between Concept and
Clinical Trials -

Rapid identification of drug entity.
100 success rate in identifying an inhibitor.
All targets are Drugable.
Predictable pharmacokinetics (same from drug to
drug).
Predictable chemical class-related toxicology
(same from drug to drug).
Identical manufacturing procedures.

42
Antisense Drug Pipeline Isis Pharmaceuticals
Pre-Clinical
Product (form)
Target
Lead Indication
Phase 1
Phase 2
Phase 3
On Market
Vitravene (I)
Antiviral
CMV Retinitis
ISIS 3521 (P)
PKC-a
Cancer - NSCLC., others
ISIS 5132 (P)
C-Raf
Cancer - ovarian, others
ISIS 2503 (P)
H-ras
Cancer - pancreatic, other
ISIS 2302 (P)
ICAM-1
Crohn's Disease
'01
ISIS 2302 (T)
ICAM-1
Topical Psoriasis
ISIS 14803 (P)
Antiviral
Hepatitis C
ISIS 104838 (P, O)
TNF-a
RA, Crohn's
4Q00
ISIS 104838 (T)
TNF-a
Topical Psoriasis, et. al
1Q01
ISIS 107248 (P, O)
VLA-4
MS, Inflammatory
ISIS 107772 (P, O)
PTP-1B
Diabetes
ISIS 13650 (I)
C-Raf
Diabetic Retinopathy, AMD
I Intravitreal
P Parenteral
T Topical
O Oral
43
PKC Signaling
Extracellular
GF
GFR
FAS
GFR
PLC
P
Cytoplasm
DAXX
RAS
Grb2
SOS
P
P
DAG
PI3K
GTP
GDP
IP3
PKC
Mitochondria
PTEN
P
P
BAD
BAD
Bcl2
MAP Kinase
Anti-Apoptotic
Pro-Apoptotic
P04
AKT
Apoptosis
Transcription FactorActivation
GeneActivation
P
P
P
P
P
P
P
P
Nucleus
44
Isozyme-specific Reduction in PKC-a mRNA and
Protein Expression by ISIS 3521
ISIS3521
ISIS 3521
Saline
Control
No oligo
PKC?
PKC?
PKC?
PKC?
Protein
mRNA
45
Activity of ISIS 3521 AgainstCalu-1 (lung) Human
Tumor Xenograft
2.25
.9 NaCl
2
375 mM 3521
Treatment ( T/C) ISIS 3521 (25
mg/kg) 47 Taxol 42 Taxol ISIS 3521 21
1.75
1.5
1.25
Tumor Volume (cm3)
1
.75
.5
.25
0
Day 25
Day 32
Day 40
Day 46
46
ISIS 3521 a Potent Inhibitor of PKC-?
inNon-Small Cell Lung Cancer
Phase 2 Trial in combination with
carboplatin/taxol
Overall Survival And Time To Progression (TTP)
(N53, period ending May 2001)
Expectation for ISIS 3521
Chemotherapy Chemotherapy
Median TTP ? 5 months 6.3
months Survival ? 8 months 15.9 months
1.00
Survival
0.75
TTP
Survival Distribution Function
0.50
Overall Survival
0.25
Censored Observation
Time To Progression
TTP
Survival
Censored Observation
0.00
0
5
10
15
20
25
30
35
6.3
15.9
Months
Typical results with carboplatin/taxol only
47
Evidence Supporting PTP-1B as a Validated
Therapeutic Target for Type 2 Diabetes
a
a
ß
ß

Abundant in insulinsensitive tissues.
Non-specific PTP-1Binhibitors (e.g.,
Vanadate)enhance insulin signalingin vitro/in
vivo.
Over-expression ofPTP-1B inhibits
insulin-mediated IR/IRSphosphorylation/insulins
ignaling.

PIP4,5
SHC
IRS-1
RAS
PI3K
PTEN
Raf
PTP-1B
PIP3,4,5
PDK1
MAPKK
AKT
MAPK
Metabolic ActionsAnti-Apoptosis
Cell Growth
48
Evidence Supporting PTP-1B as a Validated
Therapeutic Target for Type 2 Diabetes
ß
ß
a
a

PTP-1B Knockout Mice
Enhanced phosphorylationof IR/IRS in
muscle/liver inresponse to insulin.
Reduced fed blood glucoseand insulin levels.
Improved performance ininsulin and
glucosetolerance tests.
Gain less weight on normal andhigh fat diets.
Decreased fat cell mass.
No adverse observations gt 2 years.

PIP4,5
SHC
IRS-1
RAS
PI3K
PTEN
Raf
PTP-1B
PIP3,4,5
PDK1
MAPKK
AKT
MAPK
Metabolic ActionsAnti-Apoptosis
Cell Growth
49
Phylogenetic Tree of Protein Tyrosine
Phosphatases- R. Hooft van Huijsduijnen / Gene
225 (1998) 1-8 -
50
Specific Inhibition of PTP-1B Expressionin HEPG2
Cells
120
PTP-1B ASO
PTP-1B
100
TC-PTPase
100
nM
80
PTEN
10
50
PTP-1B
mRNA ( no oligo)
60
40
TC-PTPase
20
PTEN
0
nM
10
50
100
100
PTP-1B ASO
Control ASO
51
Dose-Dependent Lowering of Blood Glucose Levels
in Diabetic Mice (db/db) Following PTP-1B
Antisense Drug
450
Saline
400
PTP-1B ASO50 mg/kg
350
PTP-1B ASO25 mg/kg
300
250
PTP-1B ASO10 mg/kg
Blood glucose concentration (mg/dL)
200
Control ASO50 mg/kg
150
Normal
100
50
0
0
1
2
3
4
Time after treatment initiation (weeks)
52
ISIS 113715 / L-888, 728 (PTP-1B Antisense)A
Novel Therapeutic Agent to Treat Type 2 Diabetes

ISIS 113715 displays a very attractive
pharmacology profile as an antidiabetic agent
Normalized blood glucose in mouse and rat models
of diabetes
No hypoglycemia observed Prevention of diabetes
onset
Decreased hyperinsulinemia
Improved insulin sensitivity and glucose
homeostasis
Reduction in weight gain on high fat diet
Subcutenous dosing potentially as infrequent as
once/month
Suppression of PTP-1B protein levels and improved
insulin sensitivity in non-human primates
Mechanism of action is well understood
Attractive safety profile
Rodents
Primates