Post on 08-Dec-2021
Claudin 18.2 - 4-1BB bispecific antibody induced potent tumor inhibition through tumor-specific 4-1BB activation.
Wenqing Jiang1, Lei Fang1, Zhengyi Wang1, Taylor B Guo1. Eunyoung Park2, Eunsil Sung2, Jaeho Jung2.
1. I-MAB BIOPHARMA, Shanghai, China 2. ABL Bio, INC., Gyeonggi-do, Republic of Korea.
Introduction
Claudin 18.2 (CLDN18.2) is a gastric-specific membrane protein. In the healthy
tissue, CLDN18.2 expression is restricted to the gastric mucosa as a component of
tight junction. However, it is ectopically expressed at significant levels in a variety of
primary lesion and metastases of epithelial tumor entities, including gastric,
pancreatic, esophageal, and lung adenocarcinoma cells. Taken together, CLDN18.2
is believed to be an ideal tumor antigen for immunotherapy. Here, we reported the
development of a bispecific antibody CLDN18.2-4-1BB (TJ-CD4B). TJ-CD4B showed
stronger binding capability to CLDN18.2 when compared with benchmark CLDN18.2
monoclonal antibody (IMAB362). Functional evaluation of TJ-CD4B indicated the
activation of 4-1BB signaling was solely dependent on CLDN18.2 expression on the
cell. Furthermore, TJ-CD4B showed superior 4-1BB activity than benchmark 4-1BB
monoclonal antibody (Urelumab) in the presence of cells expressing a wide range of
CLDN18.2 level including CLDN18.2-low cells. Using a humanized 4-1BB mouse
model, TJ-CD4B showed strong tumor growth inhibition (TGI) of CLDN18.2
expressing tumor cells, with an increase of tumor infiltrating lymphocytes. Our data
suggested TJ-CD4B activated 4-1BB in a CLDN18.2-dependent manner, thus
addressing the safety concern associated with 4-1BB-based therapies. TJ-CD4B is a
promising IO therapeutic option for gastric and other CLDN18.2-positive tumors.
RESULTS
Design of anti-CLDN18.2-4-1BB BsAb
CONCLUSIONS
▪ TJ-CD4B is a bispecific antibody that can recognize cells expressing wide range of CLDN18.2.
▪ TJ-CD4B activated 4-1BB signaling to enhance T cell activation in a CLDN18.2-dependent manner.
▪ TJ-CD4B showed significant inhibition of tumor growth (7/7 tumor free) in a syngeneic mouse model. Furthermore, TJ-CD4B can induce long-term protective immunological
memory.
▪ Ex vivo analysis suggested TJ-CD4B increased CD8+ T cell number in tumor microenvironment with no impact on peripheral lymphocytes.
Anti-CLDN18.2 mAbAnti-CLDN18.2 mAb
Anti-4-1BB scFvAnti-4-1BB scFv
▪ Highly potent anti-CLDN18.2 mAb
▪ Benefit patients with wide range of CLDN18.2
expression.
▪ IgG1(N297A)
▪ No ADCC or CDC
▪ Minimize FcgR mediated 4-1BB clustering
▪ Unique 4-1BB binding epitope
▪ CLDN18.2 dependent 4-1BB activation
▪ Potent 4-1BB agonism
Superior CLDN18.2 binding potency than benchmark antibody
0 .0 0 1 0 .0 1 0 .1 1 1 0 1 0 0 1 0 0 0
0
5 0 0 0
1 0 0 0 0
1 5 0 0 0
2 0 0 0 0
C H O -K 1 C 1 8 .2 H ig h *
C o n c e n tra t io n (n M )
MF
I
T J -C D 4 B
IM A B 3 6 2
0 .0 0 1 0 .0 1 0 .1 1 1 0 1 0 0 1 0 0 0
0
2 0 0 0
4 0 0 0
6 0 0 0
C H O -K 1 C 1 8 .2 L o w **
C o n c e n tra t io n (n M )
MF
I
T J -C D 4 B
IM A B 3 6 2
0 .0 1 0 .1 1 1 0 1 0 0 1 0 0 0
0
2 0 0 0
4 0 0 0
6 0 0 0
S N U 6 2 0
(E n d o g e n o u s C 1 8 .2 )
C o n c e n tra t io n (n M )
MF
I
T J -C D 4 B
IM A B 3 6 2
CLDN18.2-dependent 4-1BB agonism
CLDN18.2- cells
-6 -4 -2 0 2 4
0
5 0 0 0 0 0
1 0 0 0 0 0 0
1 5 0 0 0 0 0
2 0 0 0 0 0 0
2 5 0 0 0 0 0
C o n c e n tra t io n [n M ]
RL
U
CLDN18.2+ cells
-8 -6 -4 -2 0 2 4
0
5 0 0 0 0 0
1 0 0 0 0 0 0
1 5 0 0 0 0 0
2 0 0 0 0 0 0
2 5 0 0 0 0 0
C o n c e n tra t io n [n M ]
RL
U
T J -C D 4 B
U re lu m a b
1 A 1 0
4-1BB reporter assay
Ig G U re lu m a b T J -C D 4 B
0 .0
0 .5
1 .0
1 .5
2 .0
2 .5
IL2
(n
g/m
l)
CLDN18.2- cells
Ig G U re lu m a b T J -C D 4 B
0 .0
0 .5
1 .0
1 .5
2 .0
2 .5
IL2
(n
g/m
l)
2 0 n M
4
0 .8
0 .1 6
0 .0 3 2
0 .0 0 6 4
CLDN18.2+ cells
Primary CD8+ T / CHO-K1 coculture assay
CLDN18.2– cells
CD8+ T cell
CLDN18.2+ cells/Tumor
CD8+ T cell
Significant tumor growth inhibition and increased TIL
0 3 6 9 1 2 1 5 1 8 2 1 2 4 2 7 3 0 3 3 3 6 3 9 4 2 4 5 4 8 5 1 5 4 5 7 6 0
0
1 0 0 0
2 0 0 0
3 0 0 0
4 0 0 0
Tu
mo
r V
olu
me
mm
3
D a ys a fte r 1 s t c h a lle n g e
h Ig G (1 0 m p k )
T J -C D 4 B (1 3 .3 m p k )
C L D N 1 8 .2 m A b (1 0 m p k )
4 -1 B B m A b (1 0 m p k )
C o m b o (1 0 + 1 0 m p k )
IM A B 3 6 2 (1 0 m p k )
N a ivet u m o r r e c h a l le n g etu m o r c h a l le n g e
B IW * 6 d o s e s
Hu4-1BB mice
MC38-
huCLDN18.2 TV=102mm3
BIW × 6 doses
BIW × 2 doses TIL analysis (n=3)
TGI, Tumor Re-challenge (n=7)
MC38-
huCLDN18.2
hIg
G
TJ-C
D4B
CL
DN
18.2
mA
b
4-1
BB
mA
b
Co
mb
o
IMA
B362
0
2 0
4 0
6 0
% C
D8
+ i
n C
D3
+ T
**
C D 8
hIg
G
TJ-C
D4B
CL
DN
18.2
mA
b
4-1
BB
mA
b
Co
mb
o
IMA
B362
3 0
3 5
4 0
4 5
5 0
% C
D8
in
CD
3+
T
C D 8
hIg
G
TJ-C
D4B
CL
DN
18.2
mA
b
4-1
BB
mA
b
Co
mb
o
IMA
B362
0
1 0
2 0
3 0
4 0
% C
D4
5 i
n l
ive
ce
lls
*C D 4 5
hIg
G
TJ-C
D4B
CL
DN
18.2
mA
b
4-1
BB
mA
b
Co
mb
o
IMA
B362
8 5
9 0
9 5
1 0 0
% C
D4
5 i
n L
ive
ce
lls
C D 4 5
Tumor infiltrating lymphocytes
Peripheral blood
Cell-based binding of CLDN18.2 by CLDN18.2-4-1BB bispecific antibodies. Antibodies were 3-fold serially diluted and incubated
with 1X105 CHO-K1-C18.2 and SNU620 for 30 minutes at 4 °C in FACS buffer. Then, APC conjugated-anti-human IgG antibody was
added at 4°C for another 30 minutes. After washing, MFI of APC was evaluated by FACS. * FACS-sorted CLDN18.2 higher expression
clone;** FACS-sorted CLDN18.2 lower expression clone; ¶ SNU620 is a gastric carcinoma cell line with very low CLDN18.2
expression on the cell surface. IMAB362 is the benchmark CLDN18.2 monospecific antibody.
Generation of anti-CLDN18.2-4-1BB bispecific antibody. Lead CLDN18.2 mAbs were identified for binding to human CLDN18.2.
Binders with high affinity were fused with anti-4-1BB antibody to generate different formats of anti-CLDN18.2-4-1BB bispecific
antibodies. Final candidates were selected based on in vitro and in vivo functional evaluation and drug developability.
4-1BB reporter assay. GloResponseTM NFkB-luc2/4-1BB Jurkat cell at a density of 2.5X104 cells per well were mixed with 2.5X104
target cells in a white 96-well plate. Antibodies were serially diluted and added to a white 96-well assay plate. After 6 hours’ incubation
at 37 C, luminescence was obtained by adding the substrate of luciferase and measured by a microplate reader. Urelumab is the
benchmark 4-1BB mono-specific antibody. 1A10 is a 4-1BB human IgG, the sequence of which was used to generate TJ-CD4B.
Primary CD8+T assay. Human CD8+ T cells (1×105) stimulated with 0.5 mg/ml human anti-CD3 antibody were co-cultured with CHO-
K1-CLDN18.2 or CHO-K1. Serially diluted antibodies were added and incubated with co-culture. After 48 hours, levels of IL2 in the
culture medium were measured using IL-2 LANCE Ultra TR-FRET Detection Kit (PerkinElmer).
Primary PBMC assay. Gastric adenocarcinoma(GA) PDX-derived cells were coculture with human PBMC (1×105) from the same
donor. Coculture was stimulated with 0.5 mg/ml human anti-CD3 antibody and incubated with serially diluted antibodies. After 48 hours,
levels of IL2 in the culture medium were measured using IL-2 LANCE Ultra TR-FRET Detection Kit (PerkinElmer).
0 .0 0 1 0 .0 1 0 .1 1 1 0 1 0 0
0
5
1 0
1 5
3 0
4 5
C o n c e n tra t io n (n M )
IL2
(n
g/m
l)
G A 0 0 0 6
G A 0 0 4 4
G A 0 0 6 0
G A 3 0 5 5
P rim a ry P B M C + P D X C o c u ltu reGA0006 GA0044 GA0060
C1
8.2
IHC
IHC H score
223 156 74
In vivo efficacy study. MC38-hCLDN18.2 cells were subcutaneously implanted into hu4-1BB mice. When the tumor grew to an
average of 102 mm3, mice (n=7/group) were intraperitoneally treated with human IgG, CLDN18.2 mAb and 4-1BB mAb alone or in
combination, IMAB362 and BsAb at equal molar amount twice weekly for 6 doses. For the re-challenge study, a second dose of
MC38-hCLDN18.2 cells were injected in the contralateral flank after the initial tumor challenge. Tumor growth was monitored by
volumetric measurement. Ex vivo analysis of FACS analysis of intratumoral and peripheral CD45+ cells and CD8+ T cells were
performed in a subgroup (n=3/group). * n<0.05; **n <0.01
Primary PBMC / PDX coculture assay
4-1BB
4-1BB
CLDN18.2
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