NZ729218B2 - Neonatal Fc Receptor Binding Dimer and Methods of Use - Google Patents
Neonatal Fc Receptor Binding Dimer and Methods of Use Download PDFInfo
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- NZ729218B2 NZ729218B2 NZ729218A NZ72921815A NZ729218B2 NZ 729218 B2 NZ729218 B2 NZ 729218B2 NZ 729218 A NZ729218 A NZ 729218A NZ 72921815 A NZ72921815 A NZ 72921815A NZ 729218 B2 NZ729218 B2 NZ 729218B2
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Abstract
The present disclosure relates to dimers of engineered polypeptides having a binding affinity for the neonatal Fc receptor FcRn, and provides an FcRn binding dimer, comprising a first monomer unit, a second monomer unit and an amino acid linker, wherein said first and second monomer unitseach comprisesan FcRn binding motif. Said FcRn binding dimerbinds FcRn with higher capacity compared to said first monomer unitor second monomer unit alone.The present disclosure also relates to the use of said FcRn binding dimeras an agent for modifying pharmacokinetic and pharmacodynamic properties and as a therapeutic agent. sesan FcRn binding motif. Said FcRn binding dimerbinds FcRn with higher capacity compared to said first monomer unitor second monomer unit alone.The present disclosure also relates to the use of said FcRn binding dimeras an agent for modifying pharmacokinetic and pharmacodynamic properties and as a therapeutic agent.
Description
NEONATAL FC RECEPTOR BINDING DIMER AND METHODS OF USE
Technical field of the invention
The present disclosure relates to dimers of engineered polypeptides
having a binding affinity for the neonatal Fc receptor (in the following referred
to as FcRn). The present disclosure also relates to the use of such dimers as
agents for modifying pharmacokinetic and codynamic ties of a
biomolecule, e.g. a pharmaceutical, and as therapeutic agents.
Background
The neonatal Fc receptor (FcRn) is a heterodimeric protein consisting
of a transmembrane MHC class I-like heavy chain (FcRn α-chain) and the β2-
microglobulin light chain, the latter also forming a part of MHC class I
molecules (Simister and Mostov (1989) Nature 337:184-7; Burmeister et al.
(1994) Nature 372:379-83).
FcRn is predominantly located in endosomes and is able to bind to
serum n and immunoglobulin G (IgG) at pH ≤ 6.5 and release them at
pH ≥ 7.0 wed in Roopenian (2007) Nat Rev Immunol 7:715-25).
FcRn carries out several distinct tasks in mammals (Roopenian,
supra). FcRn is involved in recycling of endocytosed IgG and serum albumin,
thus avoiding their degradation in the lysosome, giving them longer half-life
and higher availability in the blood than other serum proteins. When IgG,
serum albumin and other serum proteins are passively pinocytosed by cells in
contact with blood, the pH becomes gradually lower in the formed
endosomes, which permits the binding of IgG and serum albumin to FcRn.
The receptor is then, together with its bound ligand, orted via ing
endosomes back to the plasma ne. After returning to the plasma
membrane, the pH increases to above 7, at which point the bound ligand is
released.
FcRn is also ized for its ability to transport IgG over barriers
such as the placenta, the upper airway lium, the blood-brain barrier and
the proximal small intestine.
W0 2016;042083 2015/071339
In mammals, the properties of FcRn are used to transcytose lgG from
a mother to a fetus via the placenta, and to transcytose lgG from a mother’s
milk to the blood stream of an infant in the proximal small intestine.
The expression pattern of FcRn differs between species. However,
FcRn is widely expressed by cells in the blood brain barrier, upper airway
epithelium, kidneys and vascular endothelia, and by antigen ting cells
as well as by other cells of hematopoietic origin in most species (Roopenian
(2007), supra).
Antibodies and peptides with affinity towards FcRn (Liu et al. (2007) J
Immunol 179:2999-3011, Mezo et al. (2008) Proc Natl Acad Sci U S A
105:2337—42) and B2-microglobulin (Getman and Balthasar (2005) J Pharm
Sci 94:718—29) have been developed with a view to t the binding
between endogenous lgG and FcRn. r approach has been to mutate
the Fc region of the lgG to get a higher affinity for FcRn (Petkova et al. (2006)
Int Immunol 9-69, o etal. (2005) Nat Biotechnol 23:1283-8).
Fusion to the Fc domain or to albumin is a widely used strategy to
increase the in vivo half-life of proteins. r, the large size of such fusion
proteins adversely affects tissue penetration and reduces the specificity to the
fusion partner s et al. (2011) J Interferon Cytokine Res 32:178—184). On
the other hand, mutations have been made in the Fc fragment of antibodies
administered to non human primates to prolong half-life (Hinton etal. (2004) J
Biol Chem 279:6213—6). However, this approach is only limited in use to
therapeutic antibodies, and cannot be extrapolated to other therapeutic
proteins unless the proteins in on are fused to F0 fragments, which also
results in large size molecules. A number of chemical and recombinant
methods have been devised to improve protein half-life, such as PEGylation
and genetic fusions of the protein to the Fc domain of lgG or albumin
(reviewed in Schellenberger et al. (2009) Nat Biotechnol 21:1186-1190).
PEGylation of ns has been reported to decrease their potency and
contribute to their immunoreactivity.
Fc—fusion proteins have also been used for oral and pulmonary ry
mediated by the FcRn (Low et al., (2005) Human reproduction Jul;20(7):1805-
13), however similar problems relating to tissue ation and reduced
specificity remain, due to the size of the fusion molecules.
Hence, there is large need in the field for the ued provision of
molecules with high affinity for FcRn. In particular, small binding molecules
W0 2016;042083
are needed that, when present as a fusion r, do not adversely affect the
properties of the molecules they are fused to and do not contribute to
immunoreactivity.
Summary of the invention
The present disclosure is based on the unexpected realization that
FcRn binding ptides in dimeric form exhibit significantly improved FcRn
binding properties as compared to corresponding FcRn binding polypeptides
in monomeric form. The present inventors have found that the improvement in
the binding properties of said FcRn binding polypeptides in dimeric form is
greater than anticipated by the mere fusion of two FcRn binding polypeptides.
Thus, it is an object of the present sure to provide new FcRn
binding agents.
It is also an object of the present disclosure to provide such agents for
use in modifying pharmacokinetic and/or pharmacodynamic properties of a
biomolecule, eg. a pharmaceutical.
It is also an object of the present disclosure to provide such agents for
use as therapeutic agents in their own right, alone or as combination
treatment.
It is an object of the t disclosure to provide a molecule allowing
for efficient targeting of FcRn, while alleviating the above-mentioned and
other drawbacks of t therapies.
These and other s which are evident to the skilled person from
the present disclosure are met by different aspects of the ion as
claimed in the appended claims and as generally disclosed herein.
Thus, in the first aspect of the disclosure, there is ed a neonatal
Fc receptor (FcRn) binding ptide in dimeric form, i.e. an “FcRn g
dimer”, comprising a first monomer unit, a second monomer unit and an
amino acid linker, wherein said first and second monomer unit each
comprises an FcRn binding motif (BM), which motif consists of the amino acid
sequence
EX2 X3 X4 AXe X7 EIR WLPNLX15 X17 X18 QR X21 AF|X25 X25LX28 X29
wherein, independently from each other,
W0 42083
X2 is selected from A, D, E, F, H, I, K, L, N, Q, R, S, T, V, W and Y;
X3 is selected from A, D, E, F, G, H, I, K, L, M, N, Q, R, S, T, V, W and
X4 is selected from A, D, E, F, G, H, l, K, L, N, Q, R, S, T, V, W and Y;
X5 is selected from A, D, E, F, G, H, l, K, L, N, Q, R, S, T, V, W and Y;
X7 is selected from A, F, H, l, K, L, N, Q, R, S, T, V, W and Y;
X16 is selected from N and T;
X17 is selected from F, W and Y;
X18 is ed from A, D, E and N;
X21 is selected from A, S, V and W;
X25 is selected from A, D, E, F, G, H, l, K, L, N, Q, R, S, T, V, W and Y;
X26 is selected from K and S;
X28 is selected from A, D, E, F, H, l, K, L, N, Q, R, S, T, V, W and Y;
X29 is selected from D and R,
and n said FcRn binding dimer binds FcRn with a higher binding
ty compared to said first monomer unit or said second monomer unit
alone.
The above definition of a class of sequence related, FcRn binding
motifs is based on a tical analysis of a number of random polypeptide
monomer variants of a parent scaffold, that were selected for their interaction
with FcRn in several different selection experiments. The identified FcRn
binding motif, or “Bll/f’, ponds to the target binding region of the parent
scaffold, which region constitutes two alpha helices within a three-helical
bundle protein domain. In the parent scaffold, the varied amino acid residues
of the two BM helices constitute a binding surface for interaction with the
constant Fc part of antibodies. In the present disclosure, the random variation
of binding surface residues and subsequent selection of variants have
replaced the Fc interaction capacity with a capacity for ction with FcRn.
In one embodiment, the FcRn binding motif of at least one of said first
and second monomer units consists of the amino acid sequence
EX2 X3 X4 AXB X7 EIR WLPNLTX17 X18 QR X21 AF|X25 KLX28 D
W0 42083
wherein, independently from each other,
X2 is selected from A, D, E, F, H, I, K, L, N, Q, R, S, T, V, W and Y;
X3 is selected from A, D, E, F, G, H, l, K, L, M, N, Q, R, S, T, V, W and
Y;
X4 is selected from A, D, E, F, G, H, l, K, L, N, Q, R, S, T, V, W and Y;
X5 is selected from A, D, E, F, G, H, l, K, L, N, Q, R, S, T, V, W and Y;
X7 is selected from A, F, H, l, K, L, N, Q, R, S, T, V, W and Y;
X17 is selected from F, W and Y;
X13 is selected from A, D, E and N;
X21 is ed from A, S, V and W;
X25 is selected from A, D, E, F, G, H, l, K, L, N, Q, R, S, T, V, W and Y;
X23 is selected from A, D, E, F, H, l, K, L, N, Q, R, S, T, V, W and Y.
In one embodiment of the first aspect of the disclosure, said binding
motif of at least one of said first and second monomer units ts of the
amino acid sequence
EX2 X3 X4 AXe X7 EIR WLPNLX16X17 X18 QR X21 AF|X25 X26LX28 X29
wherein, independently from each other,
X2 is selected from A, D, E, F, H, l, K, L, N, Q, R, S, T, V, W and Y;
X3 is selected from A, D, E, F, G, H, l, K, L, M, N, Q, R, S, T, V, W and
X4 is selected from A, D, E, F, G, H, l, K, L, N, Q, R, S, T, V, W and Y;
X3 is selected from A, E, F, G, H, l, K, Q, R, S and V;
X7 is selected from A, F, H, K, N, Q, R, S and V;
X13 is selected from N and T;
X17 is selected from F, W and Y;
X13 is selected from A, D, E and N;
X21 is selected from A, S, V and W;
X25 is selected from D, E, G, H, l, K, L, N, Q, R, S, T, V, W and Y;
X26 is selected from K and S;
X28 is selected from A, D, E, F, H, l, K, L, N, Q, R, S, T, V, W and Y;
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X29 is selected from D and R.
In another embodiment of the first aspect, said binding motif of at least
one of said first and second monomer units consists of such an amino acid
sequence wherein, independently from each other,
X2 is selected from A, D, E, F, H, l, K, L, N, Q, R, S, T, V, W and Y;
X3 is selected from A, D, E, F, H, I, K, L, M, N, Q, R, S, T, V, W and Y;
X4 is selected from A, D, E, F, H, l, K, L, N, Q, R, S, T, V, W and Y;
X5 is selected from A, E, F, G, H, l, K, Q, R and 8;
X7 is selected from A, F, H, K, N, Q, R, S and V;
X16 is selected from N and T;
X17 is selected from F and Y;
X18 iS D;
X21 iS Vi
X25 is ed from D, E, H, l, K, L, N, Q, R, S, T, V, W and Y;
X2; is selected from K and S;
X28 is selected from A, D, E, F, H, l, K, L, N, Q, R, S, T, V and W and.
X29 is selected from D and R.
In r embodiment of the first aspect, said BM in at least one of
said first and second monomer units consists of an amino acid sequence
ed from
i) EX2 X3 X4 AXB HEIR WLPNLTX17 X18 QR X21 AFlX25 KLX23 D
wherein, independently from each other,
X2 is selected from A, D, E, F, H, l, K, L, N, Q, R, S, T, V, W and Y;
X3 is selected from A, D, E, G, H, K, L, M, N, Q, R, S, T, V and Y;
X4 is selected from A, D, E, F, G, l, K, L, N, Q, R, S, T, V and Y;
X6 is selected from A, G, K, R, S and V;
X17 is selected from F, W and Y;
X18 is selected from A, D, E and N;
X21 is selected from A, S, V and W;
X25 is selected from D, G, H, K, L, N, R, V and W;
X28 is selected from A, D, E, H, K, L, N, Q, R, S, T, W and Y;
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ii) an amino acid sequence which has at least 96 % identity to said
sequence.
In yet another embodiment of said aspect, said BM in sequence i) consists
of an amino acid sequence selected from
EX2 X3 X4 AX6 HEIR WLPNLTX17 X18 QR X21 AF|X25 KLX28 D
wherein, independently from each other,
X2 is selected from A, D, E, F, N, Q, R, S and W;
X3 is ed from D, E, G, H, K, M, N, Q, S and T;
X4 is selected from A, D, E, G, N, Q, R, S, T, V and Y;
X5 is selected from A, G, S and V;
X17 is selected from F, W and Y;
X18 is selected from A, D, E and N;
X21 is selected from A, S, V and W;
X25 is selected from D, G, H, K, L, N, R and V; and
X28 is selected from A, E, H, L, N, Q, R, S, T, W and Y.
As the skilled person will realize, the function of any polypeptide,
including the FcRn binding capacity of the dimer of the present disclosure, is
dependent on the tertiary structure of the ptide. It is ore possible
to make minor changes to the sequence of amino acids in a polypeptide
without affecting the function thereof. Thus, the disclosure encompasses
variants of the FcRn g dimer, for example variants wherein at least one
of said first and second monomeric units is modified but the FcRn binding
characteristics retained.
Therefore, as described above, also encompassed by the present
disclosure is an FcRn binding dimer, n at least one of said first and
second monomer units comprises an FcRn g motif (BM) comprising an
amino acid sequence with 96 % or greater ty to a polypeptide as defined
in i).
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In some embodiments, such changes may be made in all positions of
the ces of the BM as disclosed herein. In other embodiments, such
changes may be made only in the non-variable positions, also denoted as
scaffold amino acid residues. In such cases, changes are not allowed in the
variable positions, i.e. positions denoted with an “X” in sequence i). For
example, it is possible that an amino acid residue belonging to a certain
onal grouping of amino acid residues (e.g. hydrophobic, hydrophilic,
polar etc) could be exchanged for r amino acid residue from the same
functional group.
The term ”% identity”, as used throughout the specification, may for
example be calculated as follows. The query sequence is aligned to the target
sequence using the L W algorithm (Thompson et al. (1994) Nucleic
Acids ch 22:4673-4680). A comparison is made over the window
corresponding to the shortest of the aligned sequences. The shortest of the
aligned sequences may in some ces be the target sequence. In other
instances, the query ce may constitute the shortest of the aligned
sequences. The amino acid residues at each position are compared, and the
percentage of positions in the query ce that have identical
correspondences in the target sequence is reported as % identity.
As used herein “Xn” and “Xm” are used to indicate amino acids in
positions n and m in the sequence of the BM as d above, wherein n and
m are integers which indicate the position of an amino acid within said
sequence as counted from the N-terminal end of said sequence. For
example, X3 and X7 indicate the amino acid in position three and seven,
respectively, from the N-terminal end of said BM.
ln embodiments according to the first aspect, there is provided an
FcRn binding dimer, in which at least one of said first and second monomer
units comprises an FcRn binding motif, wherein Xn is independently selected
from a group of possible residues ing to Table 1. The skilled person will
appreciate that Xn may be selected from any one of the listed groups of
possible residues and that this ion is ndent from the selection of
amino acids in Xm, wherein n¢m. Thus, any of the listed possible residues in
position Xn in Table 1 may be independently combined with any of the herein
disclosed possible residues in any other variable position in Table 1.
The skilled person will appreciate that Table 1 is to be read as follows:
In one embodiment according to the first aspect, there is provided an FcRn
WO 2016042083
binding dimer, wherein said first monomer unit and said second monomer unit
each comprise an FcRn binding motif (BM) and wherein amino acid residue
“X,” in the BM of at least one of said first monomer unit and said second
r unit is ed from “Possible residues”. The skilled person will
appreciate that the amino acid residue “X,” in BM of the first monomer unit is
selected independently of the amino acid residue “Xn” in BM of the second
monomer unit. Thus, Table 1 discloses several specific and individualized
variants of the first r unit and the second monomer unit of the present
disclosure. For example, in one ment, there is provided an FcRn
binding dimer, comprising at least one first or second monomer unit, wherein
X2 in BM is selected from A, l, L, N, Q, S, T, V and W, and in another
embodiment, there is provided provided an FcRn binding dimer, comprising at
least one first or second monomer unit, wherein X2 in BM is selected from A,
l, L and Q. For avoidance of doubt, said first and second monomer units may
be freely combined in other ments. For example, in one such
ment, X3 is selected from A, D, E, G, H, K, L, M, N, Q, R, S and T,
while X7 is selected from A and H, and X25 is selected from H, L, R, V and W.
Table 1: Possible residues in variable positions of the FcRn binding motif of
the present disclosure.
Xn Possible residues Xn POSSIble reSIdues
X2 A, D, E, F, I, L, N, Q, R, S, T, R, S, T, V, Y
V, W, Y X3 A, D, E, H, K, L, M, N, Q, R,
X2 A, D, F, I, L, N, Q, R, S, T, V, S, T, V, Y
W, Y X3 A, D, E, G, H, K, L, M, N, Q,
X2 A, D, F, I, L, N, Q, R, S, V, W R, S, T
X2 A, I, L, N, Q, R, S, T, V, W, Y X3 A, D, E, G, H, K, M, N, Q, S,
X2 A, I, L, N, Q, S, T, V, W T
X2 A, I, L, N, Q, V, W X3 A, D, E, G, H, M, N, Q, S, T
X2 A, I, L, Q, V, W X3 A, D, E, K, N, Q, S, T
X2 A, I, L, Q, W X3 A, D, E, K, Q, T
X2 A, I, L, Q X3 A, D, E, Q, T
X2 I, L, Q X3 D, E, T
X2 I, Q X3 D, Q, T
X2 A, W X3 D, E
X2 A X3 D, Q
X2 W X3 D, T
X2 I X3 Q, T
X2 Q X3 D
X3 A, D, E, G, H, K, L, M, N, Q, X3 E
WO 20161042083 2015/071339
hhkh PTQASAAIAAAAAAAAAAAAADEQAAAAAAAAAAGAAHTNm mm mm VQQQQQQQQQDEQ EMEEIve}fiJ K L:N, are%ma mYM
Q, R , QD E
MM NAQK a R: Qu, v,
N, AU; T, L R, S, W
Q m, T., - XXXXXXXXX nnnmmmmmm
Mhnhhhhhhhhhflhhhkk&k&&&&&&&M&kfifi EELEKEKKK twmxsxbKKQfi MQS K, N S I L Q R
S T:
X PEFAADMVQMQWEQHHHHHHHKSAIAWAAAAAQARDDR EWE HNQ % H, K L N Q R M
A XXXXXXXXXXXXgamgggggg%%m HQLRRLRV LHRMVR N,K, QLW RN IR MM WWV,W
QWQNQQQQRRENE H, K L M Q R S QQQQQQQQG KKKKKKKV bfifiswsRfififlfiN V, X% K, L M Q R S I
XXXXXXXXXXXmgmwmmmmmmm EKKR L,
L, Y? W IR W&
N. RNR SQW
HH KR
In one embodiment, there is provided an FcRn binding dimer, wherein
X6X7 is selected from AH and GH in at least one of said first and second
monomer units. In one embodiment, X5X7 is AH. In one embodiment, X6X7 is
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GH. In one embodiment, X17X18 is selected from FD and YD in at least one of
said first and second monomer units. In one embodiment, X17X18 is FD.
In a more specific embodiment defining a sub-class of FcRn binding
dimers, the sequence of the BM of at least one of said first and second
r units fulfills at least three of the six conditions I-Vl:
I. X5 is selected from A, G, K and S, such as in particular A;
ll. X7 is H;
III. X17 is selected from F and Y, such as in particular F;
IV. X18 IS D;
V. X21 is selected from V and W, such as in particular V;
VI. X25 is selected from H and R, such as in particular H.
In some examples of an FcRn binding dimer according to the first
, said sequence fulfills at least four of the six conditions l-Vl. More
specifically, the sequence may fulfill at least five of the six conditions l-VI,
such as all of the six conditions l-Vl.
In one embodiment, the BM sequences of said first and second
monomer units are identical. In another embodiment, the BM sequences of
said first and second monomer units are different.
As bed in detail in the experimental section to follow, the
selection of FcRn binding polypeptide r units has led to the
identification of a number of individual FcRn binding motif (BM) ces.
These sequences constitute individual ts useful as first and second
monomer units as disclosed herein. The sequences of dual FcRn
binding motifs (BMs) are presented in Figure 1 and correspond to the
sequence from position 8 to position 36 in a sequence selected from the
group consisting of SEQ ID NO:1-353. Hence, in one embodiment of the
FcRn binding dimer according to the first aspect, at least one of said first and
second monomer units comprises a BM ponding to the sequence from
position 8 to position 36 in a sequence selected from the group consisting of
SEQ ID NO:1-353, such as selected from the group consisting of SEQ ID
NO:17-352. In one embodiment, said BM ce corresponds to the
sequence from position 8 to position 36 in a sequence selected from the
group consisting of SEQ ID 5, SEQ ID NO:17-140 and SEQ ID
, such as the group consisting of SEQ ID NO:17-140. In one
embodiment, said sequence corresponds to the sequence from position 8 to
position 36 in a sequence ed from the group consisting of SEQ ID
NO:1-2 and SEQ ID NO:17-140. In one embodiment, said sequence
corresponds to the sequence from position 8 to position 36 in a sequence
selected from the group consisting of SEQ ID NO:1-2, SEQ ID NO:17-92,
SEQ ID NO:94-103, SEQ ID -125 and SEQ ID N02127-‘I40, such as
the group consisting of SEQ ID NO:17-92, SEQ ID NO:94-103, SEQ ID
NO:105-125 and SEQ ID NO:127-140. In one embodiment, said sequence
corresponds to the sequence from position 8 to position 36 in a sequence
selected from the group consisting of SEQ ID NO:1-8, SEQ ID NO:13, SEQ
ID NO:19-20, SEQ ID NO:23, SEQ ID NO:28, SEQ ID NO:41, SEQ ID NO:44,
SEQ ID NO:65, SEQ ID NO:70, SEQ ID NO:73, SEQ ID NO:75-77 and SEQ
ID NO:353, such as the group consisting of SEQ ID NO:19-20, SEQ ID
NO:23, SEQ ID NO:28, SEQ ID NO:41, SEQ ID NO:44, SEQ ID NO:65, SEQ
ID NO:70, SEQ ID NO:73 and SEQ ID NO:75-77. In another embodiment,
said sequence corresponds to the ce from position 8 to on 36 in
a sequence selected from the group consisting of SEQ ID NO:1, SEQ ID
NO:23, SEQ ID NO:28, SEQ ID NO:41, SEQ ID NO:44, SEQ ID NO:65, SEQ
ID NO:73 and SEQ ID NO:75-77, such as the group consisting of SEQ ID
NO:23, SEQ ID NO:28, SEQ ID NO:41, SEQ ID NO:44, SEQ ID NO:65, SEQ
ID NO:73 and SEQ ID NO:75-77. In another embodiment, said sequence
corresponds to the sequence from position 8 to position 36 in a sequence
selected from the group consisting of SEQ ID NO:1, SEQ ID NO:20, SEQ ID
NO:23, SEQ ID NO:28, SEQ ID NO:41, SEQ ID NO:44, SEQ ID NO:65, SEQ
ID NO:73 and SEQ ID NO:75-77, such as the group consisting ofSEQ ID
NO:20, SEQ ID NO:23, SEQ ID NO:28, SEQ ID NO:41, SEQ ID NO:44, SEQ
ID NO:65, SEQ ID NO:73 and SEQ ID NO:75-77. In yet r embodiment,
said ce corresponds to the sequence from position 8 to position 36 in
a sequence ed from the group consisting of SEQ ID NO:1, SEQ ID
NO:23, SEQ ID NO:44, SEQ ID NO:65, SEQ ID NO:75 and SEQ ID NO:77,
such as the group consisting of SEQ ID NO:1, SEQ ID NO:23, SEQ ID
NO:44, SEQ ID NO:65 and SEQ ID NO:75. In yet another embodiment, said
sequence corresponds to the sequence from position 8 to position 36 in a
sequence selected from the group consisting of SEQ ID N021, SEQ ID
NO:20, SEQ ID NO:23, SEQ ID NO:41, SEQ ID NO:44, SEQ ID NO:65, SEQ
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ID NO:75 and SEQ ID NO:77, such as the group consisting of SEQ ID NO:1,
SEQ ID NO:20, SEQ ID NO:23, SEQ ID NO:41, SEQ ID NO:44, SEQ ID
NO:65 and SEQ ID NO:75. In yet another embodiment, said sequence
corresponds to the sequence from on 8 to position 36 in a sequence
selected from the group consisting of SEQ ID NO:23, SEQ ID NO:44, SEQ ID
NO:65, SEQ ID NO:75 and SEQ ID NO:77, such as the group consisting of
SEQ ID NO:23, SEQ ID NO:44, SEQ ID NO:65 and SEQ ID NO:75. In yet
another embodiment, said sequence corresponds to the sequence from
on 8 to position 36 in a sequence selected from the group consisting of
SEQ ID NO:20, SEQ ID NO:23, SEQ ID NO:41, SEQ ID NO:44, SEQ ID
NO:65, SEQ ID NO:75 and SEQ ID NO:77, such as the group consisting of
SEQ ID NO:20, SEQ ID NO:23, SEQ ID NO:41, SEQ ID NO:44, SEQ ID
NO:65 and SEQ ID NO:75, such as the group consisting of SEQ ID NO:20,
SEQ ID NO:23, SEQ ID NO:41, SEQ ID NO:44 and SEQ ID NO:75. In one
embodiment, said sequence corresponds to the sequence from position 8 to
position 36 in a sequence selected from the group consisting of SEQ ID
NO:1, SEQ ID N023 and SEQ ID NO:75, such as the group consisting of
SEQ ID N023 and SEQ ID NO:75. In one embodiment, said sequence
corresponds to the sequence from position 8 to position 36 in a sequence
selected from the group consisting of SEQ ID NO:20, SEQ ID NO:41 and
SEQ ID NO:44, such as the group consisting of SEQ ID N020 and SEQ ID
NO:41; the group consisting of SEQ ID N020 and SEQ ID NO:44; or the
group consisting of SEQ ID NO:41 and SEQ ID NO:44. In one embodiment,
said sequence corresponds to the sequence from position 8 to position 36 in
a sequence selected from the group consisting of SEQ ID NO:1, SEQ ID
N023 and SEQ ID NO:44, such as the group consisting of SEQ ID N023
and SEQ ID NO:44. In one embodiment, said sequence corresponds to the
sequence from on 8 to on 36 in SEQ ID NO:1 or SEQ ID NO:23 or
SEQ ID NO:44. In one ment, said sequence corresponds to the
sequence from position 8 to position 36 in SEQ ID NO:20 or SEQ ID NO:41 or
SEQ ID NO:44
In one embodiment of the FcRn binding dimer as disclosed herein,
both said first and second monomer units comprise a BM ponding to
the sequence from position 8 to position 36 in a ce selected from one
of the groups defined above. In one embodiment, said group consists of SEQ
ID NO:1, SEQ ID NO:20, SEQ ID NO:23, SEQ ID NO:41, SEQ ID NO:44,
SEQ ID NO:65 and SEQ ID NO:75. In one embodiment, said group consists
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of SEQ ID NO:20, SEQ ID NO:23, SEQ ID NO:41, SEQ ID NO:44 and SEQ
ID NO:75. In one embodiment, said group consists of SEQ ID N021, SEQ ID
NO:23, SEQ ID NO:44, SEQ ID NO:65 and SEQ ID NO:75. In another
embodiment, said group consists of SEQ ID NO:1, SEQ ID N023 and SEQ
ID NO:44. In yet another embodiment, said group consists of SEQ ID NO:20,
SEQ ID NO:41 and SEQ ID NO:44. In one particular embodiment, both said
first and second monomer units comprise a BM corresponding to the
sequence from position 8 to position 36 in SEQ ID NO:1. In one embodiment,
said BM corresponds to the sequence from position 8 to position 36 in SEQ
ID NO:20. In one embodiment, said BM corresponds to the ce from
position 8 to position 36 in SEQ ID NO:23. In one embodiment, said BM
corresponds to the sequence from position 8 to position 36 in SEQ ID NO:41.
In one embodiment, said BM corresponds to the sequence from position 8 to
on 36 in SEQ ID NO:44.
In some embodiments of the t disclosure, the BM as defined
above “forms part of’ a helix bundle protein domain. This is understood
to mean that the ce of the BM is “inserted” into or “grafted” onto the
sequence of the original three-helix bundle domain, such that the BM
es a similar structural motif in the original domain. For example, without
wishing to be bound by theory, the BM is thought to constitute two of the three
helices of a three-helix bundle, and can therefore replace such a two-helix
motif within any three-helix bundle. As the d person will realize, the
replacement of two helices of the three-helix bundle domain by the two BM
helices has to be performed so as not to affect the basic structure of the
polypeptide. That is, the l folding of the Ca backbone of the polypeptide
according to this embodiment of the invention is substantially the same as
that of the three-helix bundle protein domain of which it forms a part, e.g.
having the same elements of secondary structure in the same order etc.
Thus, a BM according to the disclosure “forms part” of a three-helix bundle
domain if the polypeptide according to this embodiment of the aspect has the
same fold as the original domain, implying that the basic structural properties
are shared, those properties e.g. resulting in similar CD spectra. The skilled
person is aware of other parameters that are relevant.
In particular embodiments, the FcRn binding motif (BM) in at least one
of said first and second monomers thus forms part of a helix bundle
protein domain. For example, the BM may essentially constitute two alpha
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helices with an interconnecting loop, within said helix bundle protein
domain. In particular embodiments, said three-helix bundle protein domain is
selected from domains of bacterial receptor proteins. Non-limiting examples
of such domains are the five different helical domains of Protein A from
lococcus aureus, such as domain B, and tives f. In some
embodiments, the helical bundle protein domain is a variant of protein
Z, which is derived from domain B of staphylococcal Protein A.
In embodiments where the FcRn binding motif as disclosed herein
forms part of a three-helix bundle protein domain, at least one of said first and
second monomer units of the FcRn binding dimer may comprise a binding
module (BMod), which module consists of an amino acid ce selected
from:
iii) K-[BM]—DPSQS XaXbLLXC EAKKL XdXeXfQ;
wherein
[BM] is an FcRn binding motif as defined herein, provided that X29 is D;
Xa is selected from A and S;
Xb is selected from N and E;
X0 is selected from A, S and C;
Xd is selected from E, N and S;
Xe is selected from D, E and S;
Xf is selected from A and S;
and
iv) an amino acid sequence which has at least 93 % identity to a
sequence defined by iii).
In embodiments where the FcRn binding motif as disclosed herein
forms part of a three-helix bundle protein domain, at least one of said first and
second monomer units of the FcRn binding dimer may comprise a binding
module (BMod), which module consists of an amino acid ce selected
from:
v) K-[BM]—QPEQS XaXbLLXc EAKKL XdXeXfQ;
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wherein
[BM] is an FcRn binding motif as defined herein, provided that X29 is R;
Xa is selected from A and S;
Xb is selected from N and E;
XC is selected from A, S and C;
Xd is selected from E, N and S;
Xe is selected from D, E and S;
Xf is selected from A and S;
vi) an amino acid sequence which has at least 93 % identity to a
sequence defined by v).
As sed above, polypeptides sing minor s as
compared to the above amino acid sequences which do not largely affect the
tertiary structure and the function thereof are also within the scope of the
present disclosure. Thus, in some embodiments, sequence iv) or sequence
vi) has at least 95 %, for example at least 97 % identity to a sequence defined
by iii) and v), respectively.
In one embodiment, there is provided an FcRn binding dimer, wherein
at least one of said first and second monomer units comprises sequence iii)
or v) wherein Xa is A. In an alternative embodiment, Xa in sequence iii) or v) is
S. In one embodiment, X2] in sequence iii) or v) is A. In one embodiment, X2] in
sequence iii) or v) is S.
In one embodiment, there is provided an FcRn g dimer, wherein
at least one of said first and second monomer units ses sequence iii)
or v) wherein Xb is N. In one embodiment, Xb in sequence iii) or v) is E.
In one embodiment, there is provided an FcRn binding dimer, wherein
at least one of said first and second monomer units ses sequence iii)
or v) wherein XC is A. In one embodiment, XC in sequence iii) or v) is S. In one
embodiment, XC in sequence iii) or v) is C.
In one embodiment, there is provided an FcRn binding dimer, wherein
at least one of said first and second monomer units comprises sequence iii)
or v) wherein Xd is E. In one embodiment, Xd in sequence iii) or v) is N. In one
embodiment, Xd in sequence iii) or v) is S.
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In one embodiment, there is ed an FcRn binding dimer, wherein
at least one of said first and second monomer units comprises sequence iii)
or v) wherein Xe is D. In one embodiment, Xe in sequence iii) or v) is E. In one
embodiment, Xe in sequence iii) or v) is S.
In one embodiment, there is provided an FcRn binding dimer, wherein
at least one of said first and second monomer units comprises ce iii)
or v) wherein dee is selected from EE, ES, SD, SE and SS. In one
embodiment, dee in sequence iii) or v) is ES. In one embodiment, dee in
sequence iii) or v) is SE. In one embodiment, dee in sequence iii) or v) is SD.
In one embodiment, there is provided an FcRn binding dimer, wherein
at least one of said first and second monomer units comprises sequence iii)
or v) wherein Xf is A. In one embodiment, Xf in ce iii) or v) is S.
In one embodiment, there is ed an FcRn binding dimer, wherein
at least one of said first and second monomer units comprises sequence iii)
or v), wherein Xa is A; Xb is N; XC is A and Xf is A.
In one embodiment, in sequence iii) or v), X3 is S; Xb is E; XC is A and
X is A.
In one ment, in sequence iii) or v), X3 is A; Xb is N; XC is C and
Xf is A.
In one embodiment, in sequence iii) or v), X3 is S; Xb is E; XC is S and
Xf IS S.
In one embodiment, in sequence iii) or v), X3 is S; Xb is E; XC is C and
Xf IS S.
In one embodiment, in sequence iii) or v), X3 is A; Xb is N; XC is A; dee
is ND and Xf is A.
In one embodiment, in sequence iii) or v), X3 is S; Xb is E; XC is A; dee
is ND and Xf is A.
In one embodiment, in sequence iii) or v), X3 is A; Xb is N; XC is C; dee
is ND and Xf is A.
In one embodiment, in sequence iii) or v), X3 is S; Xb is E; XC is S; dee
is ND and Xf is S.
In one embodiment, in sequence iii) or v), X3 is S; Xb is E; XC is C; dee
is ND and Xf is S.
In one embodiment, in sequence iii) or v), X3 is A; Xb is N; XC is A; dee
is SE and Xf is A.
In one embodiment, in sequence iii) or v), X3 is S; Xb is E; XC is A; dee
is SE and Xf is A.
In one ment, in sequence iii) or v), Xa is A; Xb is N; XC is C; dee
is SE and Xf is A.
In one embodiment, in sequence iii) or v), Xa is S; Xb is E; XC is S; dee
is SE and Xf is S.
In one embodiment, in sequence iii) or v), Xa is S; Xb is E; XC is C; dee
is SE and Xf is S.
In one ment, in sequence iii) or v), Xa is A; Xb is N; XC is A; dee
is ES and Xf is A.
In one embodiment, in sequence iii) or v), Xa is S; Xb is E; XC is A; dee
is ES and Xf is A.
In one embodiment, in sequence iii) or v), Xa is A; Xb is N; XC is C; dee
is ES and Xf is A.
In one ment, in sequence iii) or v), Xa is S; Xb is E; XC is S; dee
is ES and Xf is S.
In one embodiment, in ce iii) or v), Xa is S; Xb is E; XC is C; dee
is ES and Xf is S.
In one embodiment, in sequence iii) or v), X3 is A; Xb is N; XC is A; dee
is SD and Xf is A.
In one embodiment, in sequence iii) or v), X3 is S; Xb is E; XC is A; dee
is SD and Xf is A.
In one embodiment, in sequence iii) or v), X3 is A; Xb is N; XC is C; dee
is SD and Xf is A.
In one embodiment, in sequence iii) or v), Xa is S; Xb is E; XC is S; dee
is SD and Xf is S.
In one embodiment, in sequence iii) or v), X6] is S; Xb is E; XC is C; dee
is SD and Xf is S.
In one embodiment of the FcRn binding dimer according to the first
aspect, at least one of said first and second monomer units comprises a
Bil/10d according to sequence iii) corresponding to the sequence from position
7 to on 55 in a sequence selected from the group consisting of SEQ ID
NO:1-353, SEQ ID NO:358 and SEQ ID NO:360-364. Hence, in one
embodiment of the FcRn binding dimer according to the first aspect, at least
one of said first and second monomer units comprises a BMod corresponding
to the sequence from position 7 to position 55 in a sequence selected from
the group consisting of SEQ ID NO:1-353, SEQ ID NO:358 and SEQ ID
NO:360-364, such as the group consisting of SEQ ID NO:17-352 and SEQ ID
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NO:360-364. In one embodiment, said BMod corresponds to the sequence
from position 7 to position 55 in a sequence selected from the group
ting of SEQ ID NO:1-15, SEQ ID NO:17-140,SEQ ID NO:353, SEQ ID
NO:358 and SEQ ID NO:360-364, such as the group consisting of SEQ ID
NO:17-140 and SEQ ID NO:360-364. In one embodiment, said BMod
corresponds to the sequence from position 7 to on 55 in a sequence
selected from the group consisting of SEQ ID NO:1-2,SEQ ID NO:17-140,
SEQ ID NO:358 and SEQ ID NO:360-364. In one embodiment, said BMod
corresponds to the sequence from position 7 to position 55 in a sequence
selected from the group consisting of SEQ ID NO:1-2, SEQ ID NO:17-92,
SEQ ID NO:94-103, SEQ ID NO:105-125, SEQ ID NO:127-140, SEQ ID
NO:358 and SEQ ID NO:360-364, such as the group consisting of SEQ ID
NO:17-92, SEQ ID NO:94-103, SEQ ID NO:105-125, SEQ ID -140
and SEQ ID NO:360-364. In one embodiment, said BMod corresponds to the
sequence from position 7 to position 55 in a sequence selected from the
group consisting of SEQ ID NO:1-8, SEQ ID NO:13, SEQ ID NO:19-20, SEQ
ID NO:23, SEQ ID NO:28, SEQ ID NO:41, SEQ ID NO:44, SEQ ID NO:65,
SEQ ID NO:70, SEQ ID NO:73, SEQ ID NO:75-77, SEQ ID NO:353, SEQ ID
NO:358 and SEQ ID NO:360-364, such as the group consisting of SEQ ID
NO:19-20, SEQ ID NO:23, SEQ ID NO:28, SEQ ID NO:41, SEQ ID NO:44,
SEQ ID NO:65, SEQ ID NO:70, SEQ ID NO:73, SEQ ID NO:75-77 and SEQ
ID NO:360-364. In another embodiment, said BMod corresponds to the
sequence from on 7 to position 55 in a sequence ed from the
group consisting of SEQ ID N021, SEQ ID NO:20, SEQ ID NO:23, SEQ ID
NO:28, SEQ ID NO:41, SEQ ID NO:44, SEQ ID NO:65, SEQ ID NO:73, SEQ
ID NO:75-77, SEQ ID NO:358 and SEQ ID NO:360-364, such as the group
ting of SEQ ID NO:20, SEQ ID NO:23, SEQ ID NO:28, SEQ ID NO:41,
SEQ ID NO:44, SEQ ID NO:65, SEQ ID NO:73, SEQ ID NO:75-77 and SEQ
ID NO:360-364. In another embodiment, said BMod corresponds to the
sequence from on 7 to position 55 in a sequence selected from the
group consisting of SEQ ID NO:1, SEQ ID NO:20, SEQ ID NO:23, SEQ ID
NO:28, SEQ ID NO:41, SEQ ID NO:44, SEQ ID NO:65, SEQ ID NO:73 and
SEQ ID NO:75-77, such as the group ting of SEQ ID NO:20, SEQ ID
NO:23, SEQ ID NO:28, SEQ ID NO:41, SEQ ID NO:44, SEQ ID NO:65, SEQ
ID NO:73 and SEQ ID NO:75—77. In r embodiment, said BMod
corresponds to the sequence from position 7 to position 55 in a sequence
selected from the group consisting of SEQ ID NO:1, SEQ ID NO:23, SEQ ID
NO:28, SEQ ID NO:41, SEQ ID NO:44, SEQ ID NO:65, SEQ ID NO:73 and
SEQ ID 77, such as the group consisting of SEQ ID NO:23, SEQ ID
NO:28, SEQ ID NO:41, SEQ ID NO:44, SEQ ID NO:65, SEQ ID NO:73 and
SEQ ID NO:75-77. In yet another embodiment, said BMod corresponds to the
ce from position 7 to position 55 in a sequence selected from the
group consisting of SEQ ID NO:1, SEQ ID NO:20, SEQ ID NO:23, SEQ ID N
0:41, SEQ ID NO:44, SEQ ID NO:65, SEQ ID NO:75, SEQ ID NO:77, SEQ
ID NO:358 and SEQ ID NO:360-364, such as the group consisting of, SEQ ID
NO:20, SEQ ID NO:23, SEQ ID NO:41, SEQ ID NO:44, SEQ ID NO:65, SEQ
ID NO:75 and SEQ ID -364. In r embodiment, said BMod
corresponds to the sequence from position 7 to position 55 in a sequence
selected from the group consisting of SEQ ID NO:20, SEQ ID NO:23, SEQ ID
NO:41, SEQ ID NO:44, SEQ ID NO:65, SEQ ID NO:75 and SEQ ID -
364. In yet another embodiment, said BMod corresponds to the sequence
from position 7 to position 55 in a sequence selected from the group
consisting of SEQ ID NO:1, SEQ ID NO:20, SEQ ID NO:23, SEQ ID NO:41,
SEQ ID NO:44, SEQ ID NO:65, SEQ ID NO:75, SEQ ID NO:358 and SEQ ID
NO:360-364, such as the group consisting of SEQ ID NO:20, SEQ ID NO:23,
SEQ ID NO:41, SEQ ID NO:44, SEQ ID NO:75 and SEQ ID NO:360-364. In
yet another embodiment, said BMod corresponds to the sequence from
position 7 to position 55 in a sequence selected from the group consisting of
SEQ ID NO:1, SEQ ID NO:23, SEQ ID NO:44, SEQ ID NO:65, SEQ ID NO:75
and SEQ ID NO:77, such as the group consisting of SEQ ID NO:1, SEQ ID
NO:23, SEQ ID NO:44, SEQ ID NO:65 and SEQ ID NO:75. In another
ment, said BMod corresponds to the sequence from position 7 to
position 55 in a sequence selected from the group consisting of SEQ ID
NO:20, SEQ ID NO:23, SEQ ID NO:41, SEQ ID NO:44, SEQ ID NO:65, SEQ
ID NO:75 and SEQ ID NO:77, such as the group consisting of SEQ ID NO:20,
SEQ ID NO:23, SEQ ID NO:41, SEQ ID NO:44, SEQ ID NO:65 and SEQ ID
NO:75, such as the group consisting of SEQ ID NO:20, SEQ ID NO:23, SEQ
ID NO:41, SEQ ID NO:44 and SEQ ID NO:75. In yet r embodiment,
said BMod corresponds to the sequence from position 7 to position 55 in a
sequence selected from the group consisting of SEQ ID NO:23, SEQ ID
NO:44, SEQ ID NO:65, SEQ ID NO:75 and SEQ ID NO:77, such as the group
consisting of SEQ ID NO:23, SEQ ID NO:44, SEQ ID NO:65 and SEQ ID
NO:75. In one embodiment, said BMod corresponds to the sequence from
position 7 to position 55 in a sequence selected from the group consisting of
SEQ ID NO:1, SEQ ID NO:23 SEQ ID NO:75, SEQ ID NO:358, SEQ ID
NO:361 and SEQ ID NO:364, such as the group consisting of SEQ ID NO:23,
SEQ ID NO:75, SEQ ID NO:361 and SEQ ID NO:364. In one ment,
said BMod corresponds to the ce from position 7 to position 55 in a
sequence selected from the group consisting of SEQ ID NO:1, SEQ ID N023
and SEQ ID NO:75, such as the group consisting of SEQ ID N023 and SEQ
ID NO:75.
In one ment, said BMod corresponds to the sequence from
position 7 to position 55 in a sequence selected from the group consisting of
SEQ ID NO:20, SEQ ID NO:41, SEQ ID NO:44, SEQ ID NO:360, SEQ ID
NO:362 and SEQ ID NO:363, such as the group consisting of SEQ ID NO:20,
SEQ ID NO:41, SEQ ID NO:360 and SEQ ID NO:362; the group consisting of
SEQ ID NO:20, SEQ ID NO:44, SEQ ID NO:360 and SEQ ID NO:363; or the
group consisting of SEQ ID NO:41, SEQ ID NO:44, SEQ ID NO:362 and SEQ
ID NO:363.
In one embodiment, said BMod corresponds to the sequence from
position 7 to position 55 in a sequence selected from the group consisting of
SEQ ID NO:1, SEQ ID NO:23, SEQ ID NO:44, SEQ ID NO:358, SEQ ID
NO:361 and SEQ ID NO:363, such as the group consisting of SEQ ID NO:23,
SEQ ID NO:44, SEQ ID NO:361 and SEQ ID NO:363. In one embodiment,
said BMod corresponds to the sequence from position 7 to position 55 in a
sequence selected from the group ting of SEQ ID NO:1, SEQ ID N023
and SEQ ID NO:44, such as the group consisting of SEQ ID N023 and SEQ
ID NO:44. In one embodiment, said BMod corresponds to the sequence from
position 7 to position 55 in SEQ ID NO:1 or SEQ ID NO:23 or SEQ ID NO:44.
In one embodiment, said BMod corresponds to the sequence from position 7
to position 55 in SEQ ID NO:20 or SEQ ID NO:41 or SEQ ID NO:44. In one
embodiment, said BMod corresponds to the ce from position 7 to
position 55 in SEQ ID NO:360 or SEQ ID NO:362 or SEQ ID NO:363.
In one embodiment of the FcRn binding dimer as disclosed herein,
both of said first and second monomer units comprise a BMod corresponding
to the sequence from position 7 to position 55 in a sequence ed from
one of the groups defined above. In one embodiment, said group consists of
SEQ ID NO:1, SEQ ID NO:20, SEQ ID NO:23, SEQ ID NO:41, SEQ ID
NO:44, SEQ ID NO:65, SEQ ID NO:75, SEQ ID NO:358 and SEQ ID NO:360-
364. In one ment, said group consists of SEQ ID NO:20, SEQ ID
NO:23, SEQ ID NO:41, SEQ ID NO:44, SEQ ID NO:75 and SEQ ID N02360-
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364. In one ment, said group consists of SEQ ID NO:20, SEQ ID
NO:23, SEQ ID NO:41, SEQ ID NO:44 and SEQ ID NO:75. In another
embodiment, said group consists of SEQ ID NO:360-364. In one
embodiment, said group consists of SEQ ID NO:1, SEQ ID NO:23, SEQ ID
NO:44, SEQ ID NO:65 and SEQ ID NO:75. In another embodiment, said
group consists of SEQ ID N021, SEQ ID N023 and SEQ ID NO:44. In one
embodiment, said group consists ofSEQ ID NO:20, SEQ ID NO:41, SEQ ID
NO:44, SEQ ID NO:360, SEQ ID NO:362 and SEQ ID NO:363. In another
embodiment, said group consists of SEQ ID NO:20, SEQ ID NO:41 and SEQ
ID NO:44. In another embodiment, said group consists of SEQ ID NO:360,
SEQ ID NO:362 and SEQ ID . In one particular embodiment, both
said first and second monomer units comprise a BMW corresponding to the
sequence from position 7 to position 55 in SEQ ID NO:1 or SEQ ID NO:358.
In one embodiment, said BMod corresponds to the sequence from position 7
to position 55 in SEQ ID NO:20 or SEQ ID NO:360. In one embodiment, said
BMod corresponds to the sequence from position 7 to position 55 in SEQ ID
NO:23 or SEQ ID . In one embodiment, said BMod corresponds to the
sequence from position 7 to position 55 in SEQ ID NO:41 or SEQ ID NO:362.
In one embodiment, said BMod corresponds to the sequence from position 7
to position 55 in SEQ ID NO:44 or SEQ ID . In one embodiment, said
BMod corresponds to the sequence from on 7 to position 55 in SEQ ID
NO:75 or SEQ ID NO:364.
Also, in a further embodiment, there is provided an FcRn binding dimer
as d above, n at least one of said first and second monomer
units comprises a sequence selected from the group consisting of:
vii) YAK-[BM]-DPSQS SELLXC EAKKL NDSQA P;
wherein [BM] is an FcRn binding motif as d above and Xc is selected
from A, S and C; and
viii) an amino acid sequence which has at least 94 % ty to a
sequence defined by vii).
In another embodiment, there is provided an FcRn binding dimer as
defined above, wherein at least one of said first and second r units
comprises a sequence selected from the group consisting of:
ix) FAK-[Bll/I]-DPSQS SELLXC EAKKL SESQA P;
wherein [BM] is an FcRn binding motif as defined above and XC is selected
from A, S and C; and
x) an amino acid sequence which has at least 94 % ty to a
sequence defined by ix).
In one embodiment, XC in the sequence defined by ix) is 8.
Alternatively, there is ed an FcRn binding dimer as defined
above, wherein at least one of said first and second monomer units
comprises a sequence selected from the group consisting of:
xi) FNK-[BM]-DPSQS ANLLXC EAKKL NDAQA P;
wherein [BM] is an FcRn binding motif as defined above and XC is selected
from A and C; and
xii) an amino acid sequence which has at least 94 % identity to a
sequence defined by xi).
As discussed above, polypeptides comprising minor s as
compared to the above amino acid sequences that do not largely affect the
tertiary structure and the function thereof are also within the scope of the
t disclosure. Thus, in some ments, the FcRn binding dimer as
defined above may comprise a sequence viii), x) or xii) which is at least 96 %,
such as at least 98 % identical to a sequence defined by vii), ix) or xi),
respectively.
In some embodiments of the FcRn binding dimer, at least one of said
first and second monomer units may comprise an amino acid sequence
ed from
ADNNFNK-[BMj-DPSQSANLLSEAKKLNESQAPK;
ADNKFNK-[BM]—DPSQSANLLAEAKKLNDAQAPK;
ADNKFNK-[BM]—DPSVSKEILAEAKKLNDAQAPK;
ADAQQNNFNK-[BM]-DPSQSTNVLGEAKKLNESQAPK;
AQHDE-[BM]—DPSQSANVLGEAQKLNDSQAPK;
VDNKFNK-[BMj-DPSQSANLLAEAKKLNDAQAPK;
K-[BM]-DPSESSELLSEAKKLNKSQAPK;
VDAKYAK-[BM]—DPSQSSELLAEAKKLNDAQAPK;
VDAKYAK-[BM]—DPSQSSELLAEAKKLNDSQAPK;
AEAKYAK-[BM]—DPSQSSELLSEAKKLNDSQAPK;
AEAKYAK-[BM]—DPSQSSELLSEAKKLNDSQAP;
AEAKFAK-[BM]—DPSQSSELLSEAKKLNDSQAPK;
AEAKFAK-[BM]—DPSQSSELLSEAKKLNDSQAP;
AEAKYAK-[BM]—DPSQSSELLAEAKKLNDAQAPK;
AEAKYAK-[BMJ-DPSQSSELLSEAKKLSESQAPK;
AEAKYAK-[BM]—DPSQSSELLSEAKKLSESQAP;
AEAKFAK-[BMj-DPSQSSELLSEAKKLSESQAPK;
AEAKFAK-[BM]—DPSQSSELLSEAKKLSESQAP;
AEAKYAK-[BMJ-DPSQSSELLAEAKKLSEAQAPK;
AEAKYAK-[BM]—QPEQSSELLSEAKKLSESQAPK;
AEAKYAK-[BMJ-DPSQSSELLSEAKKLESSQAPK;
AEAKYAK-[BM]-DPSQSSELLSEAKKLESSQAP;
AEAKYAK-[BMJ-DPSQSSELLAEAKKLESAQAPK;
AEAKYAK-[BM]—QPEQSSELLSEAKKLESSQAPK;
AEAKYAK-[BMJ-DPSQSSELLSEAKKLSDSQAPK;
AEAKYAK-[BM]-DPSQSSELLSEAKKLSDSQAP;
AEAKYAK-[BMJ-DPSQSSELLAEAKKLSDAQAPK;
AEAKYAK-[BMj-QPEQSSELLSEAKKLSDSQAPK;
VDAKYAK-[BMj-DPSQSSELLSEAKKLNDSQAPK'
K-[BMj-DPSQSSELLSEAKKLNDSQAPK;
VDAKYAK-[BMJ-DPSQSSELLAEAKKLNDAQAPK'
VDAKYAK-[BMj-DPSQSSELLSEAKKLSESQAPK;
VDAKFAK-[BMj-DPSQSSELLSEAKKLSESQAPK;
VDAKYAK-[BMj-DPSQSSELLAEAKKLSEAQAPK;
VDAKYAK-[BMJ-QPEQSSELLSEAKKLSESQAPK;
VDAKYAK-[BMj-DPSQSSELLSEAKKLESSQAPK;
K-[BMj-DPSQSSELLAEAKKLESAQAPK;
VDAKYAK-[BMJ—QPEQSSELLSEAKKLESSQAPK;
K-[BMj-DPSQSSELLSEAKKLSDSQAPK;
VDAKYAK-[BMj-DPSQSSELLAEAKKLSDAQAPK;
VDAKYAK-[BMj-QPEQSSELLSEAKKLSDSQAPK;
VDAKYAK-[BMJ-DPSQSSELLAEAKKLNKAQAPK;
AEAKYAK-[BMJ-DPSQSSELLAEAKKLNKAQAPK; and
ADAKYAK-[BMJ-DPSQSSELLSEAKKLNDSQAPK;
wherein [BM] is an FcRn g motif as defined above.
In one embodiment, at least one of said first and second monomer
units of the FcRn binding dimer may comprise an amino acid sequence
selected from:
xiii) AEAKYAK-[BM]—DPSQSSELLSEAKKLNDSQAPK;
wherein [BM] is an FcRn binding motif as defined above; and
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xiv) an amino acid sequence which has at least 94 % identity to the
sequence defined in xiii).
In one embodiment, sequence xiii) is selected from the group
ting of SEQ ID NO:354-357, such as in particular selected from the
group ting of SEQ ID NO:354 and 357.
In one embodiment, both said first and second r units
comprise a ce xiii) selected from the group consisting of SEQ ID
NO:354-357, such as in particular selected from the group consisting of SEQ
ID NO:354 and 357. In one embodiment, said sequence xiii) is SEQ ID
NO:354 in both said first and second monomer units. In one embodiment,
said sequence xiii) is SEQ ID NO:357 in both said first and second monomer
units.
In one embodiment, at least one of said first and second monomer
units of the FcRn binding dimer may comprise an amino acid sequence
selected from:
xv) AEAKFAK-[BM]—DPSQSSELLSEAKKLSESQAPK;
wherein [BM] is an FcRn binding motif as defined above; and
xvi) an amino acid sequence which has at least 94 % identity to the
ce defined in xv).
In one embodiment, sequence xv) is selected from the group
consisting of SEQ ID NO:365-367. In one embodiment, ce xv) is SEQ
ID NO:365, SEQ ID NO:366 or SEQ ID NO:367.
In one embodiment, at least one of said first and second monomer
units of the FcRn binding dimer may comprise an amino acid sequence
selected from:
xvii) VDAKYAK-[BM]—DPSQSSELLSEAKKLSESQAPK;
wherein [BM] is an FcRn binding motif as defined above; and
xviii) an amino acid sequence which has at least 94 % identity to the
sequence defined in xvii).
In one ment, sequence xvii) is selected from the group
consisting of SEQ ID NO:360-364. In one embodiment, sequence xvii) is SEQ
ID NO:360, SEQ ID NO:361. SEQ ID NO:362, SEQ ID NO:363 or SEQ ID
NO:364.
In one ment, at least one of said first and second monomer
units of the FcRn binding dimer may comprise an amino acid sequence
selected from:
xix) AEAKYAK-[BM]—RQPESSELLSEAKKLSESQAPK;
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wherein [BM] is an FcRn binding motif as d above; and
xx) an amino acid sequence which has at least 94 % identity to the
sequence defined in xix).
In one embodiment, ce xix) is SEQ ID NO:359.
In one embodiment, at least one of said first and second monomer
units of the FcRn binding dimer may comprise an amino acid sequence
selected from:
xxi) VDAKYAK-[BM]—DPSQSSELLSEAKKLNDSQAPK;
wherein [BM] is an FcRn binding motif as defined above; and
xxii) an amino acid sequence which has at least 94 % identity to the
sequence defined in xxi).
Again, polypeptides comprising minor changes as compared to the
above amino acid sequences which do not largely affect the tertiary structure
and the on thereof are also within the scope of the present disclosure.
Thus, in some embodiments, the FcRn binding dimer as defined above may
comprise a sequence xiv), xvi), xviii), xx) or xxii) which is at least 96 %, such
as at least 98 % identical to a sequence defined by xiii), xv), xvii), xix) or xxi),
tively.
In one embodiment of the FcRn binding dimer according to the first
aspect, at least one of said first and second monomer units comprises a
sequence xxi) selected from the group consisting of SEQ ID 53, such
as the group consisting of SEQ ID NO:17-352. In one embodiment, said
ce xxi) is a sequence ed from the group consisting of SEQ ID
NO:1-15, SEQ ID NO:17-140 and SEQ ID NO:353, such as the group
consisting of SEQ ID NO:17-140. In one embodiment, said sequence xxi) is a
sequence selected from the group consisting of SEQ ID NO:1-2 and SEQ ID
NO:17-140. In one embodiment, said sequence xxi) is a ce selected
from the group consisting of SEQ ID , SEQ ID NO:17-92, SEQ ID
NO:94-103, SEQ ID NO:105-125 and SEQ ID NO:127-140, such as the group
consisting of SEQ ID NO:17-92, SEQ ID NO:94-103, SEQ ID NO:105-125
and SEQ ID NO:127-140. In one embodiment, said sequence xxi) is a
sequence selected from the group consisting of SEQ ID NO:1-8, SEQ ID
NO:13, SEQ ID NO:19—20, SEQ ID NO:23, SEQ ID NO:28, SEQ ID NO:41,
SEQ ID NO:44, SEQ ID NO:65, SEQ ID NO:70, SEQ ID NO:73, SEQ ID
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NO:75-77 and SEQ ID NO:353, such as the group consisting of SEQ ID
NO:19-20, SEQ ID NO:23, SEQ ID NO:28, SEQ ID NO:41, SEQ ID NO:44,
SEQ ID NO:65, SEQ ID NO:70, SEQ ID NO:73 and SEQ ID NO:75-77. In
another embodiment, said sequence xxi) is a sequence selected from the
group consisting of SEQ ID NO:1, SEQ ID NO:20, SEQ ID NO:23, SEQ ID
NO:28, SEQ ID NO:41, SEQ ID NO:44, SEQ ID NO:65, SEQ ID NO:73 and
SEQ ID NO:75-77, such as the group consisting of SEQ ID NO:20, SEQ ID
NO:23, SEQ ID NO:28, SEQ ID NO:41, SEQ ID NO:44, SEQ ID NO:65, SEQ
ID NO:73 and SEQ ID 77. In another embodiment, said ce xxi)
is a sequence selected from the group consisting of SEQ ID NO:1, SEQ ID
NO:23, SEQ ID NO:28, SEQ ID NO:41, SEQ ID NO:44, SEQ ID NO:65, SEQ
ID NO:73 and SEQ ID NO:75-77, such as the group consisting of SEQ ID
NO:23, SEQ ID NO:28, SEQ ID NO:41, SEQ ID NO:44, SEQ ID NO:65, SEQ
ID NO:73 and SEQ ID NO:75-77. In yet another embodiment, said sequence
xxi) is a sequence selected from the group consisting of SEQ ID NO:1, SEQ
ID NO:20, SEQ ID NO:23, SEQ ID NO:41, SEQ ID NO:44, SEQ ID NO:65,
SEQ ID NO:75 and SEQ ID NO:77, such as the group consisting of SEQ ID
NO:1, SEQ ID NO:20, SEQ ID NO:23, SEQ ID NO:41, SEQ ID NO:44, SEQ
ID NO:65, SEQ ID NO:75 and SEQ ID NO:77. In yet another embodiment,
said sequence xxi) is a ce selected from the group consisting of SEQ
ID NO:1, SEQ ID NO:23, SEQ ID NO:44, SEQ ID NO:65, SEQ ID NO:75 and
SEQ ID NO:77, such as the group consisting of SEQ ID NO:1, SEQ ID
NO:23, SEQ ID NO:44, SEQ ID NO:65 and SEQ ID NO:75. In yet another
embodiment, said sequence xxi) is a sequence selected from the group
consisting of SEQ ID NO:20, SEQ ID NO:23, SEQ ID NO:41, SEQ ID NO:44,
SEQ ID NO:65, SEQ ID NO:75 and SEQ ID NO:77, such as the group
consisting of SEQ ID NO:20, SEQ ID NO:23, SEQ ID NO:41, SEQ ID NO:44,
SEQ ID NO:65 and SEQ ID NO:75, such as the group ting of SEQ ID
NO:20, SEQ ID NO:23, SEQ ID NO:41, SEQ ID NO:44 and SEQ ID NO:75. In
yet another embodiment, said sequence xxi) is a sequence selected from the
group consisting of SEQ ID NO:23, SEQ ID NO:44, SEQ ID NO:65, SEQ ID
NO:75 and SEQ ID NO:77, such as the group consisting of SEQ ID NO:23,
SEQ ID NO:44, SEQ ID NO:65 and SEQ ID NO:75. In one embodiment, said
sequence xiii) is a sequence selected from the group consisting of SEQ ID
NO:1, SEQ ID N023 and SEQ ID NO:75, such as the group consisting of
SEQ ID N023 and SEQ ID NO:75. In one embodiment, said sequence xxi) is
a sequence ed from the group consisting of SEQ ID NO:20, SEQ ID
NO:41 and SEQ ID NO:44, such as the group ting of SEQ ID N020
and SEQ ID NO:41; the group consisting of SEQ ID N020 and SEQ ID
NO:44; or the group consisting of SEQ ID NO:41 and SEQ ID NO:44. In one
embodiment, said sequence xxi) is a sequence selected from the group
ting of SEQ ID NO:1, SEQ ID N023 and SEQ ID NO:44, such as the
group consisting of SEQ ID N023 and SEQ ID NO:44. In one embodiment,
said sequence xxi) is SEQ ID NO:1, or is SEQ ID NO:20, or is SEQ ID NO:23,
or is SEQ ID NO:41, or is SEQ ID NO:44.
In one embodiment of the FcRn binding dimer as disclosed herein,
both said first and second monomer units comprise a sequence xxi) or xiii)
selected from one of the groups defined above. In one embodiment, said
group consists of SEQ ID NO:1, SEQ ID NO:23, SEQ ID NO:44, SEQ ID
NO:65, SEQ ID NO:75, SEQ ID NO:354 and SEQ ID NO:357, such as the
group consisting of SEQ ID NO:1, SEQ ID NO:23, SEQ ID NO:44, SEQ ID
NO:354 and SEQ ID NO:357, such as the group consisting of SEQ ID NO:1,
SEQ ID N023 and SEQ ID NO:44 or the group consisting of SEQ ID NO:23,
SEQ ID NO:44, SEQ ID NO:354 and SEQ ID NO:357.
In one embodiment of the FcRn g dimer as disclosed herein,
both said first and second monomer units comprise a sequence xiii), xv), xvii),
xix) or xxi) selected from one of the groups defined above.
In one ment, said group consists of SEQ ID NO:1, SEQ ID
NO:20; SEQ ID NO:23, SEQ |D:41; SEQ ID NO:44, SEQ ID NO:65, SEQ ID
NO:75, SEQ ID NO:354, SEQ ID NO:357 and SEQ ID NO:360-367, such as
the group consisting of SEQ ID NO:20; SEQ ID NO:23, SEQ ID:41; SEQ ID
NO:44, SEQ ID NO:75, SEQ ID NO:357 and SEQ ID NO:360-367, such as
the group consisting of SEQ ID NO:20, SEQ ID NO:41, SEQ ID NO:44, SEQ
ID NO:357, SEQ ID NO:360, SEQ ID , SEQ ID NO:363, SEQ ID
NO:365, SEQ ID NO:366 and SEQ ID NO:367, such as the group consisting
of SEQ ID NO:357, SEQ ID NO:360, SEQ ID NO:362, SEQ ID NO:363, SEQ
ID NO:365, SEQ ID NO:366 and SEQ ID NO:367. In one particular
embodiment, both said first and second monomer units se a sequence
xxi) selected from the group ting ofSEQ ID NO:1, SEQ ID NO:23, SEQ
ID NO:44, SEQ ID NO:65 and SEQ ID NO:75, such as the group consisting of
SEQ ID NO:23, SEQ ID NO:44, SEQ ID NO:65 and SEQ ID NO:75, such as
the group consisting ofSEQ ID N023 and SEQ ID NO:44. In one particular
embodiment, both said first and second monomer units comprise a sequence
xxi) corresponding to SEQ ID N021. In one embodiment, said sequence xxi)
is SEQ ID N0220. In one ment, said sequence xxi) is SEQ ID N0223.
In one embodiment, said sequence xxi) is SEQ ID N0241. In one
embodiment, said sequence xxi) is SEQ ID N0244. In one embodiment, said
sequence xxi) is SEQ ID N0275.
In another embodiment, both said first and second monomer units
comprise a sequence xiii) corresponding to SEQ ID N0:354.
In one particular embodiment, both said first and second monomer
units comprise a sequence xix) ponding to SEQ ID N02360. In one
embodiment, said sequence xix) is SEQ ID N02361. In one embodiment, said
sequence xix) is SEQ ID . In one embodiment, said sequence xix) is
SEQ ID N02363. In one embodiment, said sequence xix) is SEQ ID NO:364.
In another particular embodiment, both said first and second monomer units
comprise a sequence xv) corresponding to SEQ ID N0:365. In one
embodiment, said sequence xv) is SEQ ID N02366. In one embodiment, said
sequence xv) is SEQ ID .
In a specific ment of the FcRn binding dimer, the first and
second monomer units comprise SEQ ID N021 and SEQ ID NO:1; SEQ ID
N021 and SEQ ID N0223; SEQ ID N021 and SEQ ID N0244; SEQ ID N021
and SEQ ID N0265; SEQ ID N021 and SEQ ID N0275; SEQ ID N021 and
SEQ ID N0:354; SEQ ID N021 and SEQ ID N0:357;SEQ ID N0223 and SEQ
ID N0223; SEQ ID N0223 and SEQ ID N0244; SEQ ID N0223 and SEQ ID
N0265; SEQ ID N0223 and SEQ ID N0275; SEQ ID N0223 and SEQ ID
N02354; SEQ ID N0223 and SEQ ID N02357; SEQ ID N0244 and SEQ ID
N0244; SEQ ID N0244 and SEQ ID N0265; SEQ ID N0244 and SEQ ID
N0275; SEQ ID N0244 and SEQ ID N02354; SEQ ID N0244 and SEQ ID
N02357; SEQ ID N0265 and SEQ ID N0265; SEQ ID N0265 and SEQ ID
N0275; SEQ ID N0265 and SEQ ID N02354; SEQ ID N0265 and SEQ ID
N02357; SEQ ID N0275 and SEQ ID N02354; SEQ ID N0275 and SEQ ID
N02357; SEQ ID N0:354 and SEQ ID N02354; SEQ ID N0:354 and SEQ ID
N02357; or SEQ ID N02357 and SEQ ID N02357, respectively. In one
embodiment, the first and second r units comprise SEQ ID N021 and
SEQ ID NO:1; SEQ ID N021 and SEQ ID N0223; SEQ ID N021 and SEQ ID
N0244; SEQ ID N021 and SEQ ID N02354; SEQ ID N021 and SEQ ID
N02357; SEQ ID N0223 and SEQ ID N0223; SEQ ID N0223 and SEQ ID
N0244; SEQ ID N0223 and SEQ ID N02354; SEQ ID N0223 and SEQ ID
2015/071339
NO:357; SEQ ID NO:44 and SEQ ID NO:44; SEQ ID NO:44 and SEQ ID
NO:354; SEQ ID NO:44 and SEQ ID NO:357; SEQ ID NO:354 and SEQ ID
NO:354; SEQ ID NO:354 and SEQ ID NO:357; or SEQ ID NO:357 and SEQ
ID NO:357, respectively. In another embodiment, the first and second
monomer units comprise SEQ ID NO:1 and SEQ ID NO:1; SEQ ID N023
and SEQ ID NO:23; SEQ ID NO:44 and SEQ ID NO:44; SEQ ID NO:354 and
SEQ ID NO:354; or SEQ ID NO:357 and SEQ ID , respectively. In yet
another embodiment, the first and second monomer units comprise SEQ ID
NO:44 and SEQ ID NO:44; or SEQ ID NO:357 and SEQ ID NO:357,
respectively.
In a specific embodiment of the FcRn binding dimer, the first and
second monomer units comprise SEQ ID NO:1 and SEQ ID NO:1; SEQ ID
NO:1 and SEQ ID NO:20; SEQ ID NO:1 and SEQ ID NO:23; SEQ ID NO:1
and SEQ ID NO:41; SEQ ID NO:1 and SEQ ID NO:44; SEQ ID NO:1 and
SEQ ID NO:65; SEQ ID NO:1 and SEQ ID NO:75; SEQ ID NO:1 and SEQ ID
NO:354; SEQ ID NO:1 and SEQ ID ; SEQ ID NO:1 and SEQ ID
NO:365; SEQ ID NO:1 and SEQ ID NO:366; SEQ ID NO:1 and SEQ ID
NO:367; SEQ ID NO:20 and SEQ ID NO:20; SEQ ID NO:20 and SEQ ID
NO:23; SEQ ID NO:20 and SEQ ID NO:41; SEQ ID NO:20 and SEQ ID
NO:44; SEQ ID NO:20 and SEQ ID NO:357; SEQ ID NO:20 and SEQ ID
NO:365; SEQ ID NO:20 and SEQ ID NO:366; SEQ ID NO:20 and SEQ ID
NO:367; SEQ ID N023 and SEQ ID NO:23; SEQ ID N023 and SEQ ID
NO:41; SEQ ID N023 and SEQ ID NO:44; SEQ ID N023 and SEQ ID
NO:65; SEQ ID N023 and SEQ ID NO:75; SEQ ID N023 and SEQ ID
NO:354; SEQ ID N023 and SEQ ID NO:357; SEQ ID N023 and SEQ ID
NO:365; SEQ ID N023 and SEQ ID NO:366; SEQ ID N023 and SEQ ID
NO:367; SEQ ID NO:41 and SEQ ID NO:41; SEQ ID NO:41 and SEQ ID
NO:44; SEQ ID NO:41 and SEQ ID NO:357; SEQ ID NO:41 and SEQ ID
NO:365; SEQ ID NO:41 and SEQ ID NO:366; SEQ ID NO:41 and SEQ ID
NO:367; SEQ ID NO:44 and SEQ ID NO:44; SEQ ID NO:44 and SEQ ID
NO:65; SEQ ID NO:44 and SEQ ID NO:75; SEQ ID NO:44 and SEQ ID
NO:354; SEQ ID NO:44 and SEQ ID NO:357; SEQ ID NO:44 and SEQ ID
NO:365; SEQ ID NO:44 and SEQ ID ; SEQ ID NO:44 and SEQ ID
NO:367; SEQ ID NO:65 and SEQ ID NO:65; SEQ ID NO:65 and SEQ ID
NO:75; SEQ ID NO:65 and SEQ ID NO:354; SEQ ID NO:65 and SEQ ID
NO:357; SEQ ID NO:75 and SEQ ID NO:354; SEQ ID NO:75 and SEQ ID
NO:357; SEQ ID NO:354 and SEQ ID NO:354; SEQ ID NO:354 and SEQ ID
NO:357; SEQ ID NO:357 and SEQ ID NO:357; SEQ ID NO:357 and SEQ ID
NO:365; SEQ ID NO:357 and SEQ ID NO:366; SEQ ID NO:357 and SEQ ID
NO:367; SEQ ID NO:365 and SEQ ID NO:365; SEQ ID NO:365 and SEQ ID
NO:366; SEQ ID NO:365 and SEQ ID ; SEQ ID NO:366 and SEQ ID
; SEQ ID NO:366 and SEQ ID NO:367; or SEQ ID NO:367 and SEQ
ID NO:367, respectively. In one embodiment, the first and second monomer
units comprise SEQ ID NO:1 and SEQ ID NO:1; SEQ ID NO:1 and SEQ ID
NO:20; SEQ ID NO:1 and SEQ ID NO:23; SEQ ID NO:1 and SEQ ID NO:41;
SEQ ID NO:1 and SEQ ID NO:44; SEQ ID NO:1 and SEQ ID NO:354; SEQ
ID NO:1 and SEQ ID NO:357; SEQ ID NO:1 and SEQ ID NO:365; SEQ ID
NO:1 and SEQ ID NO:366; SEQ ID NO:1 and SEQ ID NO:367; SEQ ID
N020 and SEQ ID NO:20; SEQ ID N020 and SEQ ID NO:23; SEQ ID
N020 and SEQ ID NO:41; SEQ ID N020 and SEQ ID NO:44; SEQ ID
N020 and SEQ ID NO:357; SEQ ID N020 and SEQ ID NO:365; SEQ ID
N020 and SEQ ID NO:366; SEQ ID N020 and SEQ ID NO:367; SEQ ID
N023 and SEQ ID NO:23; SEQ ID N023 and SEQ ID NO:41; SEQ ID
N023 and SEQ ID NO:44; SEQ ID N023 and SEQ ID NO:354; SEQ ID
N023 and SEQ ID NO:357; SEQ ID N023 and SEQ ID NO:365; SEQ ID
N023 and SEQ ID NO:366; SEQ ID N023 and SEQ ID NO:367; SEQ ID
NO:41 and SEQ ID NO:41; SEQ ID NO:41 and SEQ ID NO:44; SEQ ID
NO:41 and SEQ ID NO:357; SEQ ID NO:41 and SEQ ID ; SEQ ID
NO:41 and SEQ ID NO:366; SEQ ID NO:41 and SEQ ID NO:367; SEQ ID
NO:44 and SEQ ID NO:44; SEQ ID NO:44 and SEQ ID ; SEQ ID
NO:44 and SEQ ID NO:357; SEQ ID NO:44 and SEQ ID NO:365; SEQ ID
NO:44 and SEQ ID NO:366; SEQ ID NO:44 and SEQ ID NO:367; SEQ ID
NO:354 and SEQ ID ; SEQ ID NO:354 and SEQ ID NO:357; SEQ ID
NO:357 and SEQ ID NO:357; SEQ ID NO:357 and SEQ ID NO:365; SEQ ID
NO:357 and SEQ ID NO:366; SEQ ID NO:357 and SEQ ID NO:367; SEQ ID
NO:365 and SEQ ID NO:365; SEQ ID NO:365 and SEQ ID NO:366; SEQ ID
NO:365 and SEQ ID ; SEQ ID NO:366 and SEQ ID NO:366; SEQ ID
NO:366 and SEQ ID NO:367; or SEQ ID NO:367 and SEQ ID NO:367,
respectively. In another embodiment, the first and second monomer units
comprise SEQ ID NO:1 and SEQ ID NO:1; SEQ ID N020 and SEQ ID
NO:20; SEQ ID N023 and SEQ ID NO:23; SEQ ID NO:41 and SEQ ID
NO:41; SEQ ID NO:44 and SEQ ID NO:44; SEQ ID NO:354 and SEQ ID
NO:354; SEQ ID NO:357 and SEQ ID NO:357; SEQ ID NO:365 and SEQ ID
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NO:365; SEQ ID NO:366 and SEQ ID NO:366; or SEQ ID NO:367 and SEQ
ID , respectively. In yet another embodiment, the first and second
monomer units comprise SEQ ID N020 and SEQ ID NO:20; SEQ ID NO:41
and SEQ ID NO:41; SEQ ID NO:44 and SEQ ID NO:44; SEQ ID NO:357 and
SEQ ID NO:357; SEQ ID NO:365 and SEQ ID ; SEQ ID NO:366 and
SEQ ID NO:366; or SEQ ID NO:367 and SEQ ID NO:367, respectively.
In yet another ment, the first and second monomer units
comprise SEQ ID NO:365 and SEQ ID NO:365; SEQ ID NO:366 and SEQ ID
NO:366; or SEQ ID NO:367 and SEQ ID NO:367, respectively.
For the sake of clarity, the designation of first and second monomer
units as used throughout the present disclosure is made for clarity reasons to
distinguish between them, and is not intended to refer to the actual order of
the r units in the polypeptide chain of the FcRn binding dimer. Thus,
for example, said first monomer unit may appear N—terminally or C-terminally
in a polypeptide chain, with respect to said second monomer unit.
As the skilled person understands, the construction of a fusion protein
often involves using linkers between functional moieties to be fused. The
skilled person is aware of different kinds of linkers with different properties,
such as flexible amino acid linkers, rigid amino acid linkers and cleavable
amino acid linkers. Linkers have been used to for example se ity
or improve folding of fusion proteins, to se expression, improve
biological activity, enable targeting and alter pharmacokinetics of fusion
ns.
Thus, in one embodiment of the first aspect, there is provided an FcRn
binding dimer as defined herein, wherein said linker is selected from the
group ting of flexible amino acid linkers, rigid amino acid linkers and
cleavable amino acid linkers. In one embodiment of an FcRn binding dimer as
defined herein, said linker is arranged between the first monomeric unit and
the second monomeric unit. The d person will appreciate that the
presence of a linker arranged between the first monomeric unit and the
second monomeric unit does not exclude the presence of onal linkers.
Flexible linkers are often used in the art when the joined domains
require a certain degree of movement or interaction, and may be particularly
useful in some embodiments of the FcRn binding dimer. Such linkers are
generally ed of small, non-polar (for example G) or polar (for example
W0 2016;042083
S or T) amino acids. Some flexible linkers primarily consist of hes of G
and 8 residues, for e (GGGGS)p and (SSSSG)p. ing the copy
number “p” allows for optimization of the linker in order to achieve riate
separation between the functional moieties or to maintain necessary inter-
moiety interaction. Apart from G and S linkers, other flexible linkers are known
in the art, such as G and S linkers ning additional amino acid residues,
such as T, A, K and E, to maintain flexibility, as well as polar amino acid
residues to improve solubility.
Additional non-limiting examples of linkers include
GGGGSLVPRGSGGGGS, (GS)3, (GS)4, (GS)8, GGSGGHMGSGG,
GGSGGSGGSGG, GGSGG, GGSGGGGG, GGGSEGGGSEGGGSEGGG,
AAGAATAA, GGGGG, GGSSG, GSGGGTGGGSG, GSGGGTGGGSG, GT,
GSGSGSGSGGSG, GSGGSGGSGGSGGS and SGGSGGSG.
The skilled person is aware of other suitable linkers.
In one embodiment, said linker is a flexible linker comprising glycine
(G), serine (8) and/or threonine (T) residues. In one embodiment, said linker
has a general formula selected from (GnSm)p and (SnGm)p, wherein,
independently, n = 1—7, m = 0—7, n + m S 8 and p = 1-7. In one embodiment,
n = 1-5. In one embodiment, m = 0-5. In one embodiment, p = 1-5. In a more
specific embodiment, n = 4, m = 1 and p = 1-4. In one embodiment, said
linker is selected from the group consisting of 84G, (S4G)3 and (S4G)4_ In one
ment, said linker is selected from the group ting of G8, G48 and
(G4S)3. In one particular embodiment, said linker is G48 and in another
embodiment said linker is (G4S)3.
The terms “FcRn binding” and ”binding affinity for FcRn” as used in this
ication refer to a property of a polypeptide which may be tested for
example by the use of surface plasmon resonance (SPR) technology or
ELISA.
For e as described in the examples below, FcRn binding affinity
may be tested in an experiment in which FcRn, or a correctly folded fragment
thereof, is immobilized on a sensor chip of the instrument, and the sample
containing the polypeptide to be tested is passed over the chip. Alternatively,
the polypeptide to be tested is immobilized on a sensor chip of the ment,
and a sample ning FcRn, or a correctly folded fragment thereof, is
passed over the chip. The skilled person may then interpret the results
obtained by such experiments to establish at least a qualitative measure of
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the binding affinity of the polypeptide for FcRn. If a quantitative measure is
desired, for example to determine a KD value for the interaction, surface
n resonance methods may also be used. Binding values may for
example be defined in a Biacore (GE Healthcare) or ProteOn XPR 36 (Bio-
Rad) instrument. FcRn is suitably immobilized on a sensor chip of the
instrument, and samples of the polypeptide whose affinity is to be determined
are prepared by serial dilution and injected in random order. KD values may
then be calculated from the results using for example the 1:1 Langmuir
binding model of the BlAevaluation 4.1 software, or other suitable software,
provided by the instrument manufacturer.
Alternatively, as described in the examples below, FcRn g affinity
may be tested in an experiment in which samples of the polypeptide are
ed on antibody coated ELISA plates, and biotinylated FcRn is added
followed by streptavidin conjugated HRP. TMB substrate is added and the
absorbance at 450 nm is measured using a multi-well plate reader, such as
Victor3 (Perkin . The skilled person may then interpret the results
obtained by such experiments to establish at least a qualitative measure of
the binding affinity of the polypeptide for FcRn. If a quantitative measure is
desired, for example to determine the KB value (the half maximal effective
concentration) for the interaction, ELISA may also be used. The response of
the polypeptides against a dilution series of biotinylated FcRn are measured
using ELISA as described above. The skilled person may then interpret the
results obtained by such experiments and KD values may be calculated from
the results using for example GraphPad Prism 5 and non—linear regression.
Alternatively, affinity for FcRn may also be studied indirectly by looking
at the ability of an FcRn binding ptide to block binding of IgG to FcRn.
Thus, a d person would iate that the ability of an FcRn binding
ptide to block said binding correlates with the binding ty of the
FcRn binding polypeptide to FcRn, provided that the FcRn binding dimer
interacts with FcRn at the same, or an at least partially overlapping, region of
FcRn as IgG. Thus, the higher the capacity of binding of the polypeptide to
FcRn, the better the y to block IgG binding to FcRn.
The d person would also iate that interaction of an FcRn
binding polypeptide and FcRn can be evaluated by FACS (Fluorescence—
activated cell sorting) analysis, wherein the ed mean fluorescence
intensity (MFI) value is an indirect readout of the strength of binding of a
tested polypeptide ve to other tested polypeptides in the same
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experiment. Thus, a higher MFI-value correlates to a higher relative affinity
and a lower MFI-value correlates to a lower relative affinty.
As used herein, the term “higher binding capacity” in the context of
binding affinity for FcRn or binding of FcRn is to be interpreted in the context
of any one or more of the above-mentioned assays for direct or indirect
evaluation of affinity.
As defined herein, the FcRn binding dimer binds FcRn with a higher
binding capacity compared to said first or second monomer unit alone. In one
embodiment, the FcRn binding dimer may bind to FcRn with at least 2 times,
such as at least 3 times, such as at least 4 times, such as at least 5 times,
such as at least 6 times, such as at least 7 times, such as at least 8 times,
such as at least 9 times, such as at least 10 times, such as at least 25 times,
such as at least 50 times, such as at least 100 times higher capacity than the
ponding first monomer unit or second monomer unit alone. This
relationship may be true at both pH 6.0 and pH 7.4, or at pH 6.0 only, or at pH
7.4 only.
In someln some ments, explained further below, the FcRn
binding dimer inhibits binding of lgG to FcRn. In such embodiments, said
FcRn binding dimer may bind FcRn such that the ability of the FcRn binding
dimer to block lgG binding to FcRn is at least 2 times , such as at least
3 times higher, such as at least 4 times higher, such as at least 5 times
higher, such as at least 10 times, such as at least 15 times, such as at least
times, such as at least 25 times higher compared to the blocking ability of
the corresponding first or second monomer unit alone.
In some embodiments, said FcRn binding dimer may bind FcRn such
that the MFI value of the interaction between FcRn and the FcRn binding
dimer is at least 2 times higher, such as at least 3 times higher, such as at
least 4 times higher, such as at least 5 times higher, such as at least 10 times
higher compared to MFI value of the ction n FcRn and the
corresponding first or second monomer unit alone.
In some embodiments, said FcRn binding dimer may bind FcRn such
that the KB value of the ction between FcRn and the FcRn binding dimer
is at least 2 times lower, such as at least 3 times lower, such as at least 4
times lower, such as at least 5 times lower, such as at least 10 times lower,
such as at least 25 times lower, such as at least 50 times lower, such as at
least 100 times lower, such as at least 1000 times lower compared to the KB
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value of the interaction between FcRn and the corresponding first monomer
unit or second r unit alone.
In one embodiment, there is provided an FcRn binding dimer, which is
e of binding to FcRn at pH 6.0 such that the KB value of the interaction
is at most 1 X 10'7 M, such as at most 1 X 10'8 M, such as at most 1 X 10'9 M,
such as at most 1 X 10‘10 M, such as at most 1 X 10‘11 M, such as at most
1 X 10'12 M. An FcRn binding dimer according to this embodiment would bind,
or remain bound, to FcRn in acidic pH conditions, such as pH 6.0, for
example in an endosome. If such a polypeptide were to enter an increasingly
acidic ellular environment, it would be recycled to the plasma membrane
through its interaction with FcRn, and thus avoid degradation.
In one embodiment, the KB value of the interaction n an FcRn
binding dimer and FcRn at pH 7.4 is higher than the KB value of said
interaction at pH 6.0. Thus, the FcRn binding polypeptide would bind to FcRn
with higher affinity at pH 6.0 than at pH 7.4. In one embodiment, the KB value
of said interaction at pH 7.4 is at least 2 times higher, such as at least 5 times
higher, such as at least 10 times higher, such at least 25 times, such as at
least 50 times higher, such as at least 100 times, such as at least 1000 times
higher than the KB value of said interaction at pH 6.0.
As mentioned above, FACS analysis may be used to e the
interaction of between an FcRn binding dimer and FcRn. Hence, the
interaction of between an FcRn binding dimer and FcRn at pH 6.0 and pH 7.4
can be evaluated and the MFI value at pH 6.0 and pH 7.4 may be compared
as disclosed in the experimental section to follow. An obtained higher relative
MFI value corresponds to a higher affinity and a lower relative MFI value
corresponds to a lower affinity, provided that said MFI values are compared
within the same eXperimental set up. Thus, in one ment, the FcRn
binding dimer binds to FcRn with a higher affinity at pH 6.0 than at pH 7.4,
such as at least 10 % higher, such as at least 20 % higher, such as at least
35 % higher, such as at least 50 % higher, such as least 100% higher.
In one embodiment, the KB value of the interaction between FcRn
binding dimer and FcRn at pH 7.4 is at least 1 X 10'10 M, such as at least
1 x10'9 M, such as at least 1 x10'8 M, such as at least 1 X 10'7 M, such as at
least 1 X 10'6 M, such as at least 1 X 10'5 M. In some embodiments, the only
criterion for the interaction between FcRn binding dimer and FcRn at pH 7.4
is that any FcRn g dimer which has bound to FcRn during more acidic
conditions is released more rapidly from FcRn when the pH value increases.
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In an alternative embodiment, there is ed an FcRn binding dimer,
for which the KB of said ction at pH 7.4 is the same as or lower than the
KB of said interaction at pH 6.0. An FcRn binding dimer according to this
ment would bind or remain bound to FcRn in acidic pH conditions (i.e.
would have an off-rate at pH 6.0 which is sufficiently slow to avoid release),
for example in the endosome, as well as in neutral or slightly basic pH
conditions, for example on the plasma membrane. In a more specific
embodiment, the KB value of said interaction at pH 7.4 is at least 2 times
lower, such as at least 5 times lower, such as at least 10 times lower, such as
at least 50 times lower, such as at least 100 times lower than the KB value of
said interaction at pH 6.0.
In another embodiment, there is provided an FcRn binding dimer,
which is capable of binding to FcRn at pH 7.4 such that the KB value of the
interaction is at most 1 x 10'7 M, such as at most 1 x 10'8 M, such as at most
1 x10'9 M, such as at most 1 X 10'10 M, such as at most 1 x 10'11 M, such as
at most 1 x 10'12 M. An FcRn binding dimer according to this embodiment
would bind or remain bound for an extended time to FcRn in neutral or slightly
basic pH conditions, such as pH 7.4, for example on the plasma membrane.
The term “remain bound” should be understood to mean an interaction having
a slow off-rate at given conditions.
In general, the skilled person knows that the KB value of an interaction
is defined as the ratio between the off-rate (koff) and the on-rate (kon). Thus, a
high KD value may be due to either a high koff, a low kon or both, and
conversely, a low KD value may be due to either a low koff, a high kon or both.
The skilled person will understand that various modifications and/or
additions can be made to an FcRn binding dimer according to any aspect
disclosed herein in order to tailor the polypeptide to a specific ation
without departing from the scope of the present disclosure.
For example, in one embodiment there is provided an FcRn binding
dimer as described herein, wherein at least one of said first and second
monomer units comprises at least one additional amino acid at the C-terminal
and/or N-terminal end. Such a polypeptide should be tood as a
polypeptide having one or more onal amino acid residues at the very
first and/or the very last on in the polypeptide chain of at least one of
said first and second monomer units. Thus, said at least one of said monomer
units of the FcRn binding dimer as defined herein may comprise any suitable
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number of additional amino acid residues, for example at least one additional
amino acid residue. Each additional amino acid residue may individually or
collectively be added in order to, for example, improve or simplify production,
purification, stabilization in vivo or in vitro, ng, or detection of the
polypeptide. Such onal amino acid residues may comprise one or more
amino acid residues added for the purpose of chemical coupling. One
example of this is the addition of a cysteine residue. Such additional amino
acid residues may also provide a ”tag” for purification or detection of the
polypeptide, such as a Hiss tag or a ”myc” (c—myc) tag or a ”FLAG” tag for
interaction with antibodies specific to the tag or immobilized metal affinity
chromatography (IMAC) in the case of the hexahistidine tag.
The further amino acids as discussed above may be coupled to the
FcRn binding dimer or to any one or both of said first and second monomeric
units by means of chemical conjugation (using known c chemistry
methods) or by any other means, such as expression of the FcRn binding
dimer as a fusion protein orjoined in any other fashion, either directly or via a
linker, for example an amino acid linker as described above.
The further amino acids as sed above may for example
comprise one or more ptide (s). A further ptide domain
may e the FcRn g dimer with another on, such as for
example another g function, or an enzymatic function, or a toxic
function or a fluorescent signaling function, or combinations thereof.
Thus, in a second aspect of the present disclosure, there is provided a
fusion protein or a conjugate, comprising a first moiety consisting of an FcRn
binding dimer according to the first aspect, and a second moiety consisting of
a polypeptide having a desired biological activity. In another embodiment,
said fusion protein or conjugate may additionally comprise further moieties,
comprising desired ical activities that can be either the same or different
from the biological activity of the second moiety.
In one embodiment of said fusion protein or conjugate, the total size of
the molecule is below the threshold for efficient renal clearance upon
administration to a mammalian t.
In another embodiment of said fusion protein or conjugate, the total
size of the molecule is above the threshold for efficient renal clearance upon
administration to a mammalian subject.
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In one embodiment of said fusion protein or ate, the in vivo half-
life of said fusion protein or conjugate is longer than the in vivo ife of the
polypeptide having the desired biological activity per se.
Non-limiting examples of a desired ical activity comprise a
therapeutic activity, a binding activity, and an enzymatic activity.
In one embodiment, said desired biological activity is a g activity
to a selected target.
One example of such a binding ty is a binding activity, which
increases the in vivo half-life of a fusion protein or conjugate. This fusion
protein or conjugate may comprise at least one further moiety. In one
particular ment, said target is albumin, binding to which increases the
in vivo half-life of said fusion protein or conjugate. In one embodiment, said
albumin binding activity is provided by an albumin binding domain (ABD) of
streptococcal protein G or a derivative thereof. For example, said fusion
protein or conjugate, comprising at least one further , may comprise
[FcRn binding dimer] — [albumin binding moiety] — [moiety with affinity for
selected ]. rmore, it will be appreciated that said fusion protein or
conjugate may comprise an albumin g moiety or other target binding
moiety interspaced between two FcRn binding monomer units making up the
FcRn binding dimer as described herein, and may thus, as non—limiting
examples, be arranged according to [FcRn binding monomer moiety] —
in g moiety] — [FcRn binding monomer moiety] — [moiety with
affinity for selected target] or according to [FcRn binding monomer moiety] —
[moiety with affinity for selected ] — [FcRn binding monomer moiety] —
[albumin binding moiety]. It is to be tood that the moieties in the fusion
protein or conjugate may be freely arranged in any order from the N- to the C-
terminal of the polypeptide. In one embodiment, said in vivo half-life is
increased at least 10 times, such as at least 25 times, such as at least 50
times, such as at least 75 times, such as at least 100 times compared the in
vivo half-life of the fusion protein or conjugate per se.
In one embodiment, when a complex between a target and the fusion
protein or conjugate as described herein is formed (or maintained) at acidic
pH, such as pH 6.0, the target is rescued from elimination by lysosomal
degradation. Thus, target half-life is extended. Half-life extension implies that
the elimination rate of a target is lower when interacting with said fusion
protein or conjugate than the elimination rate of the target molecule in the
absence of said fusion protein or conjugate. Furthermore, it is desirable in this
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embodiment that the g of target by the fusion protein or conjugate
should not interfere ntially with the function of the target.
On the other hand, when a complex between the target and the fusion
protein or conjugate as described herein is not maintained or not formed at
acidic pH, the target is directed to the subcellular lysosomes where it is
degraded.
In one embodiment, there is provided a fusion protein or conjugate,
wherein the rate of elimination of a selected, undesirable target from the
subject is increased. Increased elimination of an undesirable target implies
increased ation rate of the target from the body of the multicellular
organism, as compared to a “normal” elimination rate of the target molecule
per se, i.e. without previous ction with the fusion protein or conjugate.
In another embodiment, binding of a selected undesirable target could
inactivate the function of the target, thereby blocking its biological activity in
situations where this is desirable. Such biological activity may for example be
tion or blocking of receptors or an enzymatic or othen/vise toxic or
undesirable activity. Such undesirable target may be an endogenous
hormone, enzyme, cytokine, chemokine or a target having some other
ical activity. By using an inactivating target binding, the biological
activity is blocked until the target is delivered for degradation and released at
a low pH value, and the target binding fusion protein is recycled to circulation.
This ing of the target binding fusion protein (via its FcRn g )
enables it to “catalyze” the removal of more than one molecule of the ed
undesirable .
Undesirable targets may for example be foreign proteins and
compounds, or lly expressed proteins that display elevated levels in
plasma following a medical condition and where a therapeutic effect may be
achieved by ation of said protein. The undesired target is not
necessarily evenly distributed in the plasma but may be concentrated in
certain regions, for example around a tumor or at sites of ation.
Non-limiting examples of targets are targets selected from the group
consisting of allergens, ds, antibodies, auto-antigens, blood clotting
factors, hormones, tumor cells, drug molecules, cytokines, chemokines,
proteases, hypersensitivity mediators, proinflammatory factors, toxins such as
bacterial toxins and snake venoms; pollutants, metals and anti-oxidants.
Under certain conditions, such as in certain cancer es, it is
desired to remove endogenous molecules, for example VEGF, PDGF, HGF
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and other growth atory hormones. Such molecules could also be
targeted by a binding function in said fusion protein or conjugate.
Under other conditions, such as in certain immunological diseases, it
may be desirable to remove endogenous les transiently, such as
selected interleukins or TNF. Such molecules could also be targeted by a
binding function in said fusion protein or conjugate.
In one embodiment, the second moiety having a d biological
activity is a therapeutically active polypeptide. Non-limiting es of
eutically active polypeptides are biomolecules, such as molecules
selected from the group consisting of s, for example algasidase d and
B, glucocerebrosidase, dase, arylsulphatase, aglucosidase-d,
ginase, Factor VII, Factor VIII, Factor IX and Factor Xa; hormones and
growth factors, for example growth hormone, transforming growth factor-62,
erythropoietin, insulin, insulin-like growth factor-1, myostatin, bone-derived
growth factor and glucagon—like peptide-1; chemokines, for example CCL17,
CCL19, CCL20, CCL21, CCL22, CCL27, XCL1 and CXCBCL1; and
cytokines, for example interleukin (lL)-2, lL—4, lL-7, lL-10, lL-12, lL-15, lL-18,
lL—22, lL-27, interferon (lFN)—d, lFN-B, lFN-y, tumor necrosis factor (TNF),
granulocyte-colony stimulating factor (G-CSF), macrophage-CSF, and
granulocyte/macrophage-CSF.
As the skilled person understands, the FcRn binding dimer according
to the first aspect may be useful in a fusion protein or as a conjugate partner
to any other moiety. Therefore, the above lists of therapeutically active
polypeptides should not be ued as limiting in any way.
Other possibilities for the creation of fusion polypeptides or conjugates
are also contemplated. Thus, an FcRn binding dimer according to the first
aspect of the invention may be covalently d to a second or further
moiety or moieties, which, in addition to or instead of target binding, exhibit
other functions. One example is a fusion between one or more FcRn binding
dimer and an enzymatically active polypeptide serving as a reporter or
effector moiety.
With regard to the description above of fusion proteins or conjugates
incorporating an FcRn g dimer according to the disclosure, it is to be
noted that the designation of first, second and further moieties is made for
clarity reasons to distinguish between FcRn binding dimer according to the
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disclosure on the one hand, and moieties exhibiting other functions on the
other hand. These designations are not intended to refer to the actual order of
the different domains in the polypeptide chain of the fusion protein or
conjugate. Thus, for example, said first moiety may without restriction appear
at the N-terminal end, in the middle, or at the C-terminal end of the fusion
protein or conjugate. Furthermore, the FcRn binding dimer as disclosed
herein may comprise a second moiety interspaced between the two FcRn
binding monomer units of the FcRn binding dimer.
The half maximal inhibitory concentration (IC50) is a measure of the
effectiveness of a substance for inhibiting a specific quantifiable biological or
biochemical function. This quantitative measure indicates how much of a
particular substance is needed to inhibit a specific ical function by 50 %
and is commonly used in the art. In one particular embodiment, there is
provided an FcRn binding dimer, fusion n or conjugate as defined herein
capable of blocking lgG binding to FcRn such that the half maximal inhibitory
concentration (IC50) of the blocking is at most 1 x 10'8 M, such as at most 6 x
'9 M, such as at most 4 x 10'9 M, such as at most 1 x10'9 M, such as at
most 1 x10'10 M, such as at most 1 x10'11 M. In one embodiment, there is
provided an FcRn g dimer, fusion protein or conjugate as defined herein
capable of ng lgG binding to FcRn such that the half maximal inhibitory
tration (IC50) of the blocking is at least 10 times lower, such as at
least 100 times lower, such as at least 1000 times lower compared to the
|C50 of the blocking by the corresponding first or second monomer unit alone.
The tion may be due to binding of the FcRn binding dimer, fusion
protein or ate to the same, or an at least partially pping, region of
FcRn as lgG. Alternatively, the FcRn binding dimer, fusion protein or
conjugate may bind to a different region of FcRn than lgG but sterically hinder
the binding of lgG to FcRn. Thus, the rate of ation or clearance of lgG
from the circulatory system would increase due to increased lysosomal
degradation of lgG, because the FcRn mediated recycling of lgG would be
wholly or partially unavailable due to the occupation of FcRn binding sites by
the FcRn g dimer according to the present disclosure. In other words,
administration of FcRn binding dimer, fusion n or conjugate according to
the present disclosure will act to increase the lism of circulating lgG
antibodies.
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In one embodiment, the KB value of the ction between the FcRn
binding dimer, fusion protein or ate and FcRn is lower than the KB of
the interaction between lgG and FcRn. This relationship may be true at both
pH 6.0 and pH 7.4, or at pH 6.0 only.
The above aspects furthermore encompass polypeptides in which the
FcRn binding dimer according to the first aspect, or the FcRn binding dimer
as comprised in a fusion protein or conjugate according to the second aspect,
further comprises a label, such as a label selected from the group consisting
of fluorescent dyes and metals, chromophoric dyes, chemiluminescent
compounds and bioluminescent proteins, enzymes, uclides and
radioactive particles. Such labels may for example be used for detection of
the polypeptide.
In other embodiments, the labeled FcRn binding dimer is present as a
moiety in a fusion protein or conjugate also comprising a second moiety
having a desired biological activity and/or comprising a binding on as
described above. The label may in some instances be coupled only to the
FcRn binding dimer (for example to one, two or both of said first and second
monomeric units), and in some instances both to the FcRn binding dimer and
to the second moiety of the conjugate or fusion protein. rmore, it is also
possible that the label may be coupled to a second moiety only and not to the
FcRn binding moiety. Hence, in yet another embodiment there is provided an
FcRn binding dimer comprising a second moiety, wherein said label is
coupled to the second moiety only.
When reference is made to a labeled ptide, this should be
understood as a reference to all s of the FcRn g dimer as
described herein, including fusion proteins and conjugates comprising an
FcRn binding dimer and a second and optionally further es. Thus, a
labeled polypeptide may contain only the FcRn binding dimer and e.g. a
therapeutic radionuclide, which may be chelated or covalently coupled to the
FcRn binding dimer, or contain the FcRn binding dimer, a therapeutic
radionuclide and a second moiety such as a small molecule having a desired
biological activity, for e resulting in a therapeutic efficacy.
ln embodiments where the FcRn binding dimer, fusion protein or
conjugate is radiolabeled, such a radiolabeled polypeptide may comprise a
radionuclide. A ty of radionuclides have a metallic nature, are used in
the ionic form, and are typically incapable of forming stable covalent bonds
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with elements presented in proteins and peptides. For this reason, labeling of
proteins and peptides with radioactive metals is performed with the use of
ors, i.e. multidentate ligands, which form non—covalent compounds,
called chelates, with the metal ions. In an embodiment of the FcRn binding
dimer, fusion protein or conjugate, the incorporation of a radionuclide is
enabled through the provision of a chelating environment, through which the
radionuclide may be nated, chelated or complexed to the polypeptide.
One example of a chelator is the inopolycarboxylate type of
chelator. Two classes of such polyaminopolycarboxylate chelators can be
distinguished: macrocyclic and acyclic chelators.
In one ment, the FcRn binding dimer, fusion protein or
conjugate comprises a ing environment provided by a
polyaminopolycarboxylate chelator coupled to the FcRn binding dimer via a
thiol group of a cysteine residue or an epsilon amine group of a lysine
residue. Alternatively, the polyaminopolycarboxylate or may be coupled
to any part of the fusion protein or ate as disclosed herein, such as to
the second or further moiety of said fusion protein or conjugate.
The most ly used macrocyclic chelators for sotopes of
indium, gallium, yttrium, bismuth, radioactinides and radiolanthanides are
different derivatives of DOTA (1 ,4,7,10-tetraazacyclododecane-1 ,4,7,10-
tetraacetic acid). In one embodiment, a chelating environment of the FcRn
binding dimer, fusion protein or ate is provided by DOTA or a derivative
thereof. More specifically, in one ment, the chelating polypeptides
encompassed by the t disclosure are obtained by reacting the DOTA
derivative 1,4,7,10-tetraazacyclododecane-1,4,7-tris-acetic acid
maleimidoethylacetamide (maleimidomonoamide-DOTA) with said
polypeptide.
Additionally, 1,4,7-triazacyclononane-1,4,7-triacetic acid (NOTA) and
derivatives thereof may be used as chelators. Hence, in one embodiment,
there is provided an FcRn binding dimer, fusion protein or conjugate, wherein
the polyaminopolycarboxylate chelator is 1,4,7-triazacyclononane-1,4,7-
triacetic acid or a derivative thereof.
The most ly used acyclic polyaminopolycarboxylate chelators
are different derivatives of DTPA (diethylenetriamine-pentaacetic acid).
Hence, polypeptides having a chelating environment provided by
diethylenetriaminepentaacetic acid or derivatives thereof are also
encompassed by the t disclosure.
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In a further embodiment, the FcRn binding dimer, produced
recombinantly h expression of a polynucleotide or synthetically, is
conjugated to one or more synthetic polymers, in order for example to
increase its hydrodynamic radius. Polyethylene glycol (PEG) is ly
used for this purpose, but other polymers have also been used in the art.
Such “PEGylation” may be used to increase the size of the FcRn binding
dimer, fusion protein or conjugate as described herein to a size above the
threshold for effective renal ion.
In one embodiment, a synthetic polymer is conjugated to one or more
chemically sized FcRn binding dimer(s). Other functionalities may also
be conjugated to the same synthetic r. If the FcRn binding dimer and
other components are chemically synthesized, none of the components will
have to be made in a biological system if this is not desired.
In a preferred embodiment, one or more synthetically or biologically
manufactured FcRn binding dimers are conjugated to a tic r, to
e a size exceeding the size associated with efficient renal clearance
and used for blocking binding of lgG to FcRn. A unique cysteine in the
monomer units of the FcRn binding dimer may be used for site specific
conjugation, for example a C-terminally located ne introduced for this
purpose. With a branched tic polymer, more than two FcRn binding
moieties may be conjugated to the same polymer, to enhance the avidity and
therefore the blocking potency.
In a third aspect of the present disclosure, there is provided a
polynucleotide encoding an FcRn binding dimer or a fusion protein as
described herein. Also encompassed by this disclosure is a method of
producing an FcRn binding dimer or fusion protein as described above
comprising expressing the polynucleotide; an expression vector comprising
the cleotide; and a host cell comprising the expression vector.
Also encompassed is a method of ing FcRn binding dimer or a
fusion protein, comprising culturing said host cell under conditions permissive
of expression of said polypeptide from its expression vector, and isolating the
polypeptide.
The FcRn binding dimer or fusion protein of the present disclosure may
alternatively be produced by non-biological peptide synthesis using amino
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acids and/or amino acid derivatives having protected reactive hains, the
non-biological peptide synthesis comprising
- step-wise coupling of the amino acids and/or the amino acid
derivatives to form an FcRn binding dimer or a fusion protein having protected
reactive side-chains,
- removal of the protecting groups from the reactive side-chains of the
FcRn binding dimer or fusion protein, and
- folding of the FcRn binding dimer orfusion n in aqueous
solution.
In a fourth aspect of the disclosure, there is provided a composition
comprising an FcRn binding dimer, fusion protein or conjugate as described
herein and at least one pharmaceutically acceptable ent or carrier. In
one embodiment thereof, said composition r comprises at least one
additional active agent, such as at least two additional active agents, such as
at least three additional active agents. Non-limiting es of additional
active agents that may prove useful in such a ation are
immunosuppressing agents, anti-inflammatory agents, icrobial agents
and enzymes.
In one embodiment of this aspect, said composition is adapted for
administration by a route selected from the group consisting of oral
administration, intranasal administration, pulmonar administration, vaginal
stration, rectal administration, intravenous ion, intraperitoneal
injection, intramuscular ion, subcutaneous injection and intradermal
injection.
As used herein, the term “systemic administration” refers to a route of
administration such that the substance of interest enters into the circulatory
system so that the entire body is affected. The skilled person is aware that
ic administration can take place via enteral administration (absorption
of the drug through the gastrointestinal tract) or parenteral administration
ally injection, infusion or implantation).
In one embodiment, said composition is adapted for administration
systemically or locally. In certain embodiments, systemic administration of
said composition may be used. In another ment, said composition is
adapted for administration by a local route. For example, local administration
may be topical in an ointment, paste, foam or cream. In another embodiment,
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said composition is adapted for administration across an endothelial or
lial layer. Here, the composition may be transcytosed across said layer.
In one embodiment, the rate of uptake of a composition comprising a
fusion protein or conjugate as described herein is higher than the rate of
uptake of polypeptides corresponding to second or further moieties per se. In
one embodiment, the rate of uptake is at least 2 times higher, such as at least
times , such as at least 10 times , such as at least 25 times
higher than the rate of uptake of the at second or further moieties per se.
It should be understood from the above disclosure that the FcRn
binding dimer, fusion protein or conjugate or the composition as described
herein may for example be useful as a therapeutic agent, and/or as a means
for ing the in vivo half-life of a fusion partner, and/or as a means for
increasing the rate of elimination of undesirable targets.
Hence, in a fifth aspect of the present disclosure, there is provided an
FcRn binding dimer, fusion protein, conjugate or composition as disclosed
herein for use as a medicament.
In a related, sixth, aspect of the present disclosure, there is provided a
method of treatment or prophylaxis of a subject in need thereof, comprising
the step of administrating a therapeutically or prophylactically active amount
of an FcRn binding dimer, fusion protein, conjugate or composition as
disclosed herein.
In one embodiment of any one of these two latter aspects, the
medicament or method is intended for reduction of an IgG level in a subject in
need thereof.
In one embodiment of any one of these two latter aspects, the
medicament or method is intended for treatment or prophylaxis in which the
capacity of the FcRn g dimer to at least partially block g of IgG to
FcRn is exploited, for e treatment or laxis in which increased
catabolism of IgG antibodies is desired.
In another embodiment wherein the IgG blocking capacity is used, the
administration of FcRn binding dimers as described herein has the effect of
improving the efficacy of a drug, by blocking antibodies that exhibit anti-drug
properties. In particular, the action of drugs that are cleared by antibodies or
for which lizing antibodies are induced may be improved in this way, by
administration of FcRn binding dimers prior to administration of the drug in
question.
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In another embodiment wherein the lgG blocking capacity is used, the
administration of FcRn binding dimers as described herein has the effect of
reducing harmful effects of antibodies by ng them or reducing their
circulation time in the bloodstream of a subject. For example, radiolabelled or
toxin-conjugated dies may be removed by the subsequent
administration of FcRn binding dimers as disclosed herein. atively, in
cases where toxic adverse effects occur as a reaction against a eutic
antibody drug, such adverse effect may be ameliorated or neutralized by the
subsequent administration of an FcRn g dimer to remove such
antibodies or limit their circulation time.
In one embodiment, a condition in which such treatment or prophylaxis
may be indicated is an auto-immune condition. As non-limiting examples of
indicated conditions, mention is made of acute disseminated
encephalomyelitis (ADEM), acute necrotizing hemorrhagic leukoencephalitis,
Addison’s e, globulinemia, alopecia , amyloidosis,
ANCA-associated vasculitis, ankylosing litis, anti-GBM/anti-TBM
nephritis, antiphospholipid syndrome (APS), autoimmune angioedema,
autoimmune aplastic anemia, mune dysautonomia, autoimmune
hepatitis, autoimmune hyperlipidemia, mune immunodeficiency,
autoimmune inner ear disease , autoimmune limbic encephalitis,
autoimmune myocarditis, autoimmune pancreatitis, autoimmune retinopathy,
autoimmune thrombocytopenic purpura (ATP), autoimmune thyroid e,
autoimmune urticarial, axonal & anal neuropathies, Balo disease, Behcet’s
e, bullous pemphigoid, cardiomyopathy, man disease, celiac
disease, Chagas disease, chronic inflammatory demyelinating
polyneuropathy (CIDP), chronic recurrent ocal ostomyelitis (CRMO),
Churg-Strauss syndrome, cicatricial pemphigoid/benign mucosal pemphigoid,
Crohn’s disease, Cogans syndrome, cold agglutinin disease, congenital heart
block, coxsackie myocarditis, CREST disease, essential mixed
cryoglobulinemia, demyelinating neuropathies, dermatitis herpetiformis,
dermatomyositis, s disease (neuromyelitis optica), dilated
cardiomyopathy, discoid lupus, Dressler’s syndrome, endometriosis,
eosinophilic angiocentric fibrosis, eosinophilic fasciitis, epidermolysis bullosa
acquisita, erythema m, experimental allergic encephalomyelitis, Evans
syndrome, fibrosing alveolitis, giant cell arteritis (temporal arteritis),
glomerulonephritis, Goodpasture’s syndrome, granulomatosis with
polyangiitis (GPA; Wegener’s), Graves’ disease, Guillain-Barré syndrome,
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Hashimoto’s encephalitis, Hashimoto’s thyroiditis, hemolytic anemia, Henoch-
Schonlein purpura, herpes gestationis, hypogammaglobulinemia, idiopathic
hypocomplementemic tubulointestitial nephritis, idiopathic membranous
nephropathy, idiopathic thrombocytopenic purpura (ITP), lgA pathy,
lgG4-related disease, lgG4-related sclerosing disease, regulatory
Iipoproteins, matory aortic aneurysm, inflammatory pseudotumor,
inclusion body myositis, insulin-dependent diabetes (type 1), interstitial
cystitis, juvenile tis, juvenile diabetes, Kawasaki syndrome, Kuttner’s
tumor, Lambert-Eaton syndrome, leukocytoclastic vasculitis, lichen planus,
lichen sclerosus, Iigneous conjunctivitis, linear lgA disease (LAD), lyme
disease, chronic mediastinal fibrosis, Meniere’s disease, microscopic
polyangiitis, Mikulicz’s syndrome, mixed connective tissue disease (MCTD),
Mooren’s ulcer, morvan syndrome, Habermann disease, mucus
membrane pemphigoid, multifocal fibrosclerosis, multiple sis,
myasthenia , myositis, narcolepsy, neuromyelitis optica (Devic’s),
yotonia ’s syndrome), neutropenia, ocular cicatricial
pemphigoid, optic neuritis, Ormond’s disease (retroperitoneal is),
palindromic rheumatism, PANDAS (pediatric autoimmune neuropsychiatric
disorders associated with streptococcus), paraneoplastic cerebellar
degeneration, paraproteinemic polyneuropathies, smal nocturnal
hemoglobinuria (PNH), Parry g syndrome, Parsonnage-Turner
syndrome, pars planitis (peripheral uveitis), pemphigoid gestationis,
pemphigus vulgaris, periaortitis, periarteritis, peripheral neuropathy,
perivenous encephalomyelitis, pernicious anemia, POEMS syndrome,
polyarteritis nodosa, thritis, Type I, ll, & lll autoimmune polyglandular
syndromes, polymyalgia rheumatic, polymyositis, postmyocardial infarction
syndrome, ricardiotomy me, progesterone dermatitis, primary
biliary cirrhosis, primary sclerosing cholangitis, psoriasis, psoriatic arthritis,
thic pulmonary fibrosis, pyoderma gangrenosum, pure red cell aplasia,
Raynaud’s phenomenon, reflex sympathetic dystrophy, Reiter’s syndrome,
ing polychondritis, restless legs syndrome, retroperitoneal fibrosis
(Ormond’s disease), rheumatic fever, rheumatoid arthritis, Riedel’s thyroiditis,
sarcoidosis, Schmidt me, scleritis, scleroderma, n’s syndrome,
sperm & testicular autoimmunity, stiff person me, subacute bacterial
endocarditis (SBE), Susac’s syndrome, sympathetic ophthalmia, Takayasu’s
arteritis, systemic lupus erythematosus (SLE), temporal arteritis/giant cell
arteritis, thrombotic thrombocytopenic purpura (TTP), -Hunt syndrome,
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erse myelitis, ulcerative colitis, undifferentiated tive tissue
disease (UCTD), s, vasculitis, vesiculobullous osis, vitiligo,
Waldenstrom macroglobulinaemia and warm thic hemolytic anemia.
In another embodiment of the fifth and sixth aspects, a condition in
which such treatment or prophylaxis may be ted is an allo-immune
condition. As non-limiting examples of indicated conditions, mention is made
of transplantation donor mismatch due to anti-HLA antibodies; foetal and
neonatal alloimmune thrombocytopenia, FNAIT (or neonatal alloimmune
thrombocytopenia, NAITP or NAIT or NAT, or foeto—maternal alloimmune
thrombocytopenia, FMAITP or FMAIT).
In another embodiment of the fifth and sixth s, a condition in
which such treatment or prophylaxis may be indicated is selected from the
group consisting of autoimmune polyendocrine syndrome types 1 (APECED
or Whitaker’s Syndrome) and 2 (Schmidt’s Syndrome); alopecia salis;
myasthenic crisis; thyroid crisis; thyroid associated eye disease; thyroid
ophthalmopathy; autoimmune diabetes; autoantibody associated encephalitis
and/or encephalopathy; pemphigus foliaceus; epidermolysis bullosa;
dermatitis herpetiformis; Sydenham’s chorea; acute motor axonal neuropathy
(AMAN); Miller-Fisher me; multifocal motor neuropathy (MMN);
onus; inflammatory myopathy; Isaac’s syndrome (autoimmune
neuromyotonia), oplastic syndromes and limbic encephalitis.
In another embodiment of the fifth and sixth aspects, a ion in
which such treatment or prophylaxis may be indicated is selected from
epilepsy and seizures.
In another embodiment, there is provided an FcRn binding dimer,
fusion n, conjugate or composition as described herein for use in
blocking or removal of an undesirable target from the circulation. In one
embodiment, said undesirable target is selected from the group comprising
allergens, amyloids, antibodies, auto-antigens, blood clotting factors,
hormones, tumor cells, drug les, cytokines, chemokines,
hypersensitivity mediators, pro-inflammatory factors, toxins such as bacterial
toxins and snake venoms, pollutants, metals and anti-oxidants.
While the invention has been bed with reference to various
ary aspects and embodiments, it will be understood by those skilled in
the art that various changes may be made and equivalents may be
substituted for elements f without departing from the scope of the
invention. In addition, many modifications may be made to adapt a particular
situation or molecule to the ngs of the invention without departing from
the essential scope thereof. ore, it is intended that the invention not be
limited to any particular embodiment contemplated, but that the invention will
include all embodiments falling within the scope of the appended claims.
Brief description of the figures
Figure 1 is a listing of the amino acid sequences of examples of FcRn
binding polypeptides in monomeric form (SEQ ID NO:1-367) and FcRn
binding ptides in dimeric form (SEQ ID NO:368—376), as well as the
amino acid sequences of the albumin binding polypeptide variant PP013
(SEQ ID NO:377), Taq polymerase binding Z variant 203638 (SEQ ID
NO:378), human chRn (SEQ ID NO:379), murine chRn (SEQ ID NO:384),
human BZ-microglobulin (SEQ ID ), murine BZ-microglobulin (SEQ ID
NO:381), human chRn (SEQ ID NO:382) when in human FcRn-eGFP and
murine chRn (SEQ ID NO:383) when in murine FcRn-eGFP. The deduced
FcRn binding motifs (BMs) of the FcRn g polypeptides disclosed herein
extend from e 8 to residue 36 in sequences with SEQ ID NO:1-367.
The amino acid sequences of the 49 amino acid residues long polypeptides
(BMod) predicted to constitute the complete three-helix bundle within each of
these Z ts extend from residue 7 to residue 55.
Figures 2A-2E show the binding to human FcRn at pH 6.0 and
dissociations at pH 6.0 and 7.4 for agged Z variants and for lgG as
described in Example 3. Overlays of grams obtained from a Biacore
instrument representing injection at pH 6.0 followed by dissociation at pH 6.0
(solid line) and injection at pH 6.0 followed by dissociation at pH 7.4 (dashed
line) are yed for (A) 207918 (SEQ ID NO:1), (B) ZO7960 (SEQ ID
NO:4), (C) Z10109 (SEQ ID NO:3), (D) Z10193 (SEQ ID N02) and (E) lgG.
Figure 3 shows dot plots from a flow cytometry analysis of binding of
FcRn binding Z variant to human (upper panel) and mouse (lower panel)
FcRn-eGFP HeLa cells, as described in Example 4. Due to heterogeneous
expression of FcRn-eGFP by HeLa cells, cells were gated according to FcRn-
eGFP expression level. Cells in gate H are considered to be FcRn—eGFP
negative and cells in gate l are considered to be positive. Incubation with
Alexa Fluor® 647 labeled Z variants ed in a population positive both for
Alexa Fluor® 647 and eGFP, whereas incubation with buffer (buffer control)
did not. The figure shows that the three variants 207960 (SEQ ID NO:4),
207930 (SEQ ID NO:6) and 207918 (SEQ ID NO:1) bind to human FcRn and
mouse FcRn. The y-axis shows Alexa Fluor® 647 intensity and the x-axis
shows eGFP activity.
Figure 4 shows mean scence intensity (MFI) values of Alexa
Fluor® 647 labeled 207960 (SEQ ID NO:4), 207930 (SEQ ID N026) and
207918 (SEQ ID NO:1), measured in the cell binding assay described in
Example 4. Diagram (A) shows MFI from HeLa cells transduced with human
FcRn-eGFP and diagram (B) shows MFI from HeLa cells transduced with
mouse FcRn-eGFP.
Figure 5 shows dot plots from flow cytometry is of human or
mouse lgG Alexa Fluor® 647 g to human (upper panel) and mouse
(lower panel) FcRn-eGFP HeLa cells, as described in Example 5. Due to
heterogeneous expression of FcRn—eGFP by HeLa cells, cells were gated
ing to the abundance of FcRn-eGFP on the cell surface. Cells in gate
M are considered to be FcRn—eGFP negative and cells in gate N are
considered to be positive. Binding of 100 nM human or mouse lgG-Alexa
Fluor® 647 to FcRn transduced HeLa cells are shown in the left panel (0 nM).
The figure shows that lgG binding was blocked by Hiss-tagged 207918 (SEQ
ID NO:1) in a dose dependent manner (1, 10, 100 and 1000 nM). The y-axis
shows Alexa Fluor® 647 intensity and the x-axis shows eGFP activity.
Figure 6 shows mean scence intensity (MFI) values resulting
from FcRn binding of IgG Alexa Fluor® 647 in the presence of different
concentrations of Hise-tagged 207918 (SEQ ID NO:1) on (A) human FcRn-
eGFP transduced HeLa cells and (B) mouse FcRn-eGFP transduced HeLa
cells, as described in Example 5. The figure shows dose dependent blocking
of the lgG-FcRn binding by the 2 variant.
Figures 7A-7C show kinetics of binding of three 2 variants to human
FcRn at pH 6.0, as described in e 6, using a Biacore instrument.
Sensorgrams for a tration series of (A) 211948 (SEQ ID ), (B)
211946 (SEQ ID NO:355) and (C) 211947 (SEQ ID NO:356), respectively, in
fusion with the albumin binding polypeptide PP013 (SEQ ID NO:377) and the
control 2 variant molecule 203638 (SEQ ID NO:378; not specific for FcRn),
are displayed. Curves from 640 nM (dashed line), 160 nM (dotted line) and 40
nM (solid grey line) were subjected to kinetic analysis using the Langmuir 1:1
binding model. Kinetic parameters and ties were calculated from fitted
curves (solid black lines) and are shown in Table 6.
Figure 8 shows the pharmacokinetic profiles for three FcRn binding Z
variants fused to the albumin g polypeptide PP013 obtained as
described in Example 6. The Z ts Z11947 (SEQ ID NO:356, open
squares), 211946 (SEQ ID NO:355, open les) and 211948 (SEQ ID
NO:354, open diamonds) all displayed prolonged ife compared to the
negative control ZO3638-PP013 (open circles).
Figure 9 shows the blocking of human IgG to human FcRn by His;-
ZO7918 (SEQ ID NO:1; black circles), IVIg (grey squares) and SCIg (grey
triangles), respectively, assayed as described in Example 10.
Figure 10 shows that blocking of the IgG-FcRn interactions with FcRn
specific Z variants in mice results in reduced levels of IgG. As further
described in Example 11, mice were treated with five daily injections of
Vehicle (+), the ABD fused Z variant ZO7918-PP013 (open square) and
211948 (SEQ ID NO:354; closed circle). The concentration of endogenous
IgG was measured by ELISA. The tration of IgG in individual mice at
24, 72, 120 and 168 h was related to the level at 0 h and the results are
therefore presented as percentage of IgG at 0 h.
Figure 11 shows mean fluorescence intensity (MFI) values of Alexa
Fluor® 647 labeled dimeric and ric polypeptides binding to human
FcRn-eGFP transfected HeLa cells measured as described in Example 13.
(A) Dimers Z11948-(G4S)3-Z11948 (SEQ ID NO:369) and Z11948-(G4S)—
Z11948 (SEQ ID NO:368), and a corresponding monomer Z variant, ZO7918
(SEQ ID NO:1), g to FcRn at pH 6 (black) and pH 7.4 (white). (B)
Monomer primary Z variant ZO7918 (SEQ ID NO:1) and monomer maturated
Z variants Z13583 (SEQ ID NO:23), Z13621 (SEQ ID NO:44), Z13654 (SEQ
ID NO:65) and 213674 (SEQ ID NO:75), binding to FcRn at pH 6 (black) and
pH 7.4 (white).
Figure 12 shows the blocking of human IgG binding to human FcRn by
dimeric and monomeric polypeptides assayed as described in Example 14.
(A) Dimers Z11948-(G4S)3-Z11948 (SEQ ID NO:369) and Z11948-(G4S)-
Z11948 (SEQ ID NO:368); a corresponding monomer Z variant, ZO7918
(SEQ ID NO:1), SCIg and Mg. B) Monomer primary Z variant ZO7918 (SEQ
ID NO:1) and r maturated Z variants Z13583 (SEQ ID N023) and
213621 (SEQ ID NO:44).
Figure 13 shows pH dependent binding of ptides to hFcRn
ed by ELISA as described in Example 17. (A) Binding of the indicated
polypeptides at pH 6. (B) g of the indicated polypeptides at pH 7.4. At
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both pH , more efficient binding was seen for the dimeric polypeptides
(ZAZ####) than for the monomeric Z variant (Z13621).
Figure 14 shows reduction of hlgG levels in FcRn transgenic mice
treated with dimeric polypeptides as described in Example 20. (A) Reduction
of hlgG levels was equally efficient with the albumin binding domain PP013
(SEQ ID ) situated between the two 2 moieties (ZAZ3715; SEQ ID
NO:371) as with PP013 situated at the C-terminus of the polypeptide
(ZZA3716; SEQ ID NO:372). (B) Equal ion of hlgG levels was obtained
with the polypeptides ZAZ3869 (SEQ ID NO:374), ZAZ3870 (SEQ ID
NO:375) and ZAZ3871 (SEQ ID NO:376).
Figure 15 shows dose dependent reduction of hlgG levels in NMRI
mice d with dimeric polypeptides ZAZ3715 (SEQ ID NO:371) and
ZAZ3824 (SEQ ID NO:373) as described in Example 21.
Figure 16 shows the serum concentrations of ZAZ3715 (SEQ ID
NO:371) and ZAZ3824 (SEQ ID NO:373), respectively, measured in the same
lgG catabolism study as that presented in Figure 15.
Figure 17 is an image of an SDS-PAGE gel showing al and
d FcRn binding Z variants before (0) and after a 2 week (2w) stability
test. Lane 1: Z11948 (0), lane 2: Z11948 (2w), lane 3: Mw, lane 4: Z17347
(0), lane 5: 217347 (2w), lane 6: Z17348 (0), lane 7: 217348 (2w). The
molecular size marker (Mw) was Novex® Sharp Pre-stained Protein Standard
(216, 160, 110, 80, 60, 50, 40, 30, 20, 15, 10, 3.5 kDa). The diagonal bands
seen in the figure are an artifact resulting from an t from a second gel
stained in the same ner.
Figure 18 shows the binding to human and cynomolgus FcRn at pH 6.0
as described in Example 25. Overlays of sensorgrams ed from a
Biacore instrument representing responses from injection of 90 nM Hise-
tagged Z variant over hFcRn ) and chRn (grey) are displayed for (A)
Z13578 (solid line) and 218632 (dashed line), (B) Z13616 (solid line) and
Z18633 (dashed line), and (C) Z13621 (solid line) and Z18634 (dashed line).
Examples
Summary
The following Examples disclose the development of novel Z variant
molecules targeting the al Fc receptor (FcRn). The Z variants were
obtained using phage display technology. The genes encoding FcRn g
polypeptides described herein were sequenced, and the corresponding amino
acid sequences are listed in Figure 1, and denoted by the fiers SEQ ID
NO:1-353. The deduced FcRn binding motifs (BMs) of the FcRn binding
polypeptides disclosed herein extend from residue 8 to residue 36 in
sequences with SEQ ID NO:1—353. Furthermore, the FcRn binding properties
and ability to block lgG binding to FcRn of said polypeptides in dimeric form
were investigated.
Example 1
tion of human chRn and human roglobulin (82M)
In this Example, the extracellular domain (ECD) of human chRn (SEQ
ID ) in complex with human BZ-microglobulin (SEQ ID NO:380)
(complex denoted FcRn) and human BZ-microglobulin in non-complexed form
(denoted BZM) were produced as soluble ns. Human FcRn and BZM
produced in this Example were used for phage selection, ELISA and Biacore
assays in Examples 2 and 3.
Materials and methods
Construction of plasmids containing the genes for human chRn and
human fi2-microglobulin to be used for co-expression: The genes encoding
human chRn (Genbank BC008734.2) and human BZ-microglobulin (82M)
(Genbank 89.1) were obtained from OpenBiosystems. Using PCR
overlap extension, a gene fragment encoding amino acids 24-290 of human
chRn (chRnECD) (SEQ ID ) was amplified to a construct ting
of attB1-site/Kozak sequence followed by a gene encoding: an lg kappa chain
leader sequence, hFcRnECD, a GS-linker and a flag tag, followed by an attBZ
site. A similar construct was made containing a gene fragment encoding
amino acids 21-119 of human 82M (SEQ ID NO:380), except that a Hise tag
replaced the flag tag. The constructs were inserted into the plasmid
pDONOR221 rogen, cat. no. 12536-017) by recombination using the
Gateway system (Invitrogen, cat. no. 11789020, y® BP Clonase® II
Enzyme mix), according to the manufacturer’s recommendations. After
verification of correct sequences, the human chRnECD construct was
inserted into 2K7bsd (Suter et al. (2006) Stem Cells 24:615—623) using multi-
site gateway cloning together with the promoter-containing plasmid pENTR-
CMV (Tai et al. (2012) PLoS One 7(9):e46269), resulting in the vector 2K7bsd-
CMV-hFcRnECD. The human 82M gene uct was similarly inserted into
2K7neo (Suter et al., supra), giving the vector 2K7neo—CMV-h 82M.
Cell culture, preparation of recombinant lentiviral vectors and gene
insertions into SKOV-3 cell line: The HEK293T and SKOV—3 cell lines were
obtained from ATCC. Cells were grown at 37 °C in a humidified incubator in
the presence of 5 % C02. Complete medium for the HEK293T cell line was
Dulbeccos modified eagle medium (DMEM) supplemented with 10 % fetal
bovine serum (FBS), 1 % Antibiotic Antimycotic Solution (AA) and 1 % MEM
sential Amino Acid Solution (NEAA). Complete medium for the SKOV-
3 cell line was McCoy’s 5A medium mented with 10 % FBS and 1 %
The plasmids 2K7bsd-CMV-hFcRnECD and 2K7neo-CMV-hBZM were
separately co-transfected together with VSV-G envelope and gag/pol
packaging plasmid into HEK293T cells using calcium chloride transfection
(Zufferey etal. (1997) Nat Biotechnol 15(9):871-5; Jakobsson etal. (2006) J
Neurosci Res 84:58-67). HEK293 culture atants containing formed
lentiviral particles with human chRnECD and human BZM transgenes,
respectively, were cleared from cell debris by centrifugation and filtration. The
two types of lentiviral particles were used to sequentially transduce SKOV-3
cells. Successful double integrants ning both the human chRnECD and
the BZM genes were selected for by the addition of blasticidin (lnvitrogen) and
G418 sulfate (lnvitrogen) to culture medium while passaging the cells for two
weeks. The resulting, stably transduced SKOV-3 cell line was denoted SKOV—
3 hFcRnECD/hBZM.
sion of recombinant human FcRn: SKOV-3 cells, ressing
human chRnECD and BZM resulting in human FcRn, were ed and
1.5 x 107 cells were seeded in a HYPERFlask (Coming) in 560 ml complete
growth medium. After five days, when the cells had settled and multiplied, the
medium was d to complete growth medium without FBS. After five
days, the e was terminated and the supernatant was ted, passed
through a 45 pm filter and frozen at -80 °C.
Purification of recombinant human FcRn using human lgG
chromatography: Protein purification was carried out in an AKTA Explorer
system (GE Healthcare). Human lgG (Pharmacia), 1 ml in 0.2 M NaHC03, 0.5
M NaCl pH 8.3 at a concentration of 10 mg/ml, was coupled to a 1 ml HiTrap
NHS-activated HP column (GE Healthcare) according to the manufacturer’s
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instruction. The supernatant containing inant human FcRn from
SKOV-3 cells was thawed and the pH was ed to 5.8 with HCI. The
supernatant was subsequently loaded in batches of 100 ml onto the column
previously equilibrated with 20 mM Bis-Tris pH 5.8. The column was washed
with 20 ml of 20 mM Bis-Tris pH 5.8 and eluted in fractions of 1 ml using 50
mM Tris, pH 8.1. Buffer exchange to PBS (phosphate buffered saline, 10 mM
phosphate, 137 mM NaCl, 2.68 mM KCI, pH 7.4) was performed using
dialysis.
GE and Western blot: The purity of the eluted fractions from
the protein purification was analyzed by SDS-PAGE and staining with
e Blue Stain Reagent (Pierce) and SilverXpress® Silver Staining Kit
(lnvitrogen). Western blotting was carried out using an Amersham HybondTM-
C Extra nitrocellulose membrane (GE Healthcare). The membrane was
blocked with 5 % non—fat dry milk (Semper) in TBS+T (50 mM Trizma base,
150 mM NaCl, 0.05 % Tween-20, pH 8) for 1 hour, then probed with a mixture
of rabbit anti-FCGRT polyclonal antibody (Atlas Antibodies) at a concentration
of 0.15 ug/ml and rabbit anti-B2M onal antibody (Atlas Antibodies) at a
concentration of 0.23 ug/ml in TBS+T. The ne was subsequently
ted with stabilized goat anti-rabbit antibody conjugated with horse
radish peroxidase (Pierce) diluted 1:10,000 in TBS+T. After addition of TMB
Substrate (Pierce), an image of the membrane was ed on Amersham
Hyperfilm ECL (GE Healthcare). The Hyperfilm was processed using GBX
developer and GBX fixer (Sigma-Aldrich).
Production of a non-complexed form of human B2M: Human B2M was
produced in E. coli. The expression and purification was performed
essentially as described in Sandalova et al. (2005) Acta Chryst F61 :1090-
1093 and lsson et al. (2001) J Immunol 27-7334. The purified
protein, consisting of amino acids 21-119 of human B2M, in urea was
subjected to arginine refolding as follows; 0.5 mg of B2M was rapidly added
to 2 ml refolding buffer (20 ml 1 M Tris-HCI pH 8.0, 16.87 g L-Arginine
(buffered with HCI), 0.8 ml 0.5 M EDTA, 61 mg GSSG, 307 mg GSH and milli-
Q water to a final volume of 200 ml, pH 8.0, and supplemented with protease
tor (Roche, cat. no. 11 873 580 001)). The refolding procedure was
performed at 4 °C during 4 hours. Refolded B2M protein was buffer
exchanged to PBS using a PD-10 column (GE Healthcare).
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Results
Construction of plasmids containing the genes for human chRn and
human fi2—microglobulin to be used for co-expression: Genes encoding the
extracellular domain of the q—chain of human FcRn (chRnECD) and human
82M were inserted into the lentiviral transfer plasmids 2K7bsd and 2K7neo,
respectively. In both cases, the inserted gene is under the control of a CMV
er. The genes were extended so that the resulting proteins would have
an lg kappa chain leader sequence in the N-terminus to target the protein for
export through the endoplasmic reticulum to the culture medium (the signal
sequence was cleaved upon secretion). In addition, chRnECD had a C-
terminal spacer sequence followed by a FLAG-tag for potential detection.
Human 82M had a inal spacer ce followed by a Hise tag for
potential detection. The spacer sequence was added to enhance accessibility
of the tag. The lentiviral transfer plasmids also contained two different
antibiotic resistance genes to allow ion of cells where both constructs
had been inserted.
Expression and purification of recombinant human FcRn: The genes
encoding chRnECD and BZM were ed into the genome of SKOV—3 by
lentiviruses, and the resulting FcRn protein was secreted into the culture
medium. To capture only FcRn having retained pH-dependent lgG binding,
affinity chromatography using immobilized lgG was used where the or
was captured at pH 5.8 and eluted at pH 8.1. ed protein was eluted in
three fractions.
SDS-PAGE and Western blot: To investigate the presence of two
peptide chains (chRnECD and 82M) of the produced FcRn protein, and to
analyze the purity of the eluted material, an SDS—PAGE analysis was
performed on the eluted ons. For the gel d with GelCode Blue
Stain, two bands were detected with molecular weights of 12 and 36 kDa,
respectively. This corresponds approximately to the tical molecular
weights of the non-glycosylated peptide chains of 12 kDa for 82M and 31 kDa
for chRnECD. The chRnECD part of the protein contains one glycosylation
site and it was therefore expected that its molecular mass would be higher
than 31 kDa. The gel was also silver stained to increase sensitivity and
possibly detect impurities. A band of approximately 66 kDa was detected in
the first eluted fraction, which could correspond to BSA (bovine serum
n) originating from cell attachment. The total amount of protein
recovered in fraction 2 and 3 corresponded to 1.4 mg/l e medium. A
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western blot analysis on the pooled material was carried out, which showed
essentially only the two major bands and in addition a very weak band below
12 kDa which might correspond to a degradation product.
Example 2
Selection and ELISA binding of FcRn binding Z variants
In this Example, human FcRn was used as target in phage y
selections using a phage library of Z variants. Selected clones were DNA
sequenced, produced in E. coli periplasmic fractions and d against
FcRn in ELISA (enzyme-linked immunosorbent assay).
Materials and s
ylation of target protein FcRn and of B2M: Human FcRn and
human B2M, produced as described in Example 1, were ylated using
No-Weigh EZ-Link Sulfo-NHS—LC-Biotin (Pierce, cat. no. 21327) at a
31 x (FcRn) and 10 x (B2M) molar , respectively, according to the
manufacturer’s recommendations. The reactions were performed at room
temperature (RT) for 30 min. Subsequent buffer exchange to PBS was
performed using Slide-a-lyzer dialysis cassettes (FcRn; Pierce, cat. no.
66380, 10,000 MWCO and B2M; Pierce, cat. no. 66333, 3,500 MWCO),
according to the manufacturer’s instructions.
Phage display selection of FcRn binding Z variants: A library of random
variants of n Z displayed on bacteriophage, constructed in phagemid
pAY02592 essentially as bed in Grénwall et al. (2007) J Biotechnol,
128:162-183, was used to select FcRn binding Z variants. In this library, an
albumin binding domain (ABD, GA3 of protein G from ococcus strain
G148) is used as fusion partner to the Z variants. The library is denoted
Zlib006Naive.l| and has a size of 1.5 x 1010 library members (Z variants).
E. coli RRIAM15 cells (RUther et al., (1982) c Acids Res 10:5765-5772)
from a glycerol stock containing the phagemid library Zlib006Naive.l|, were
inoculated in 20 l of a defined proline free medium [dipotassium
hydrogenphosphate 7 g/l, trisodium citrate dihydrate 1 g/l, uracil 0.02 g/l, YNB
(DifcoTM Yeast Nitrogen Base w/o amino acids, Becton Dickinson) 6.7 g/l,
glucose monohydrate 5.5 g/I, L—alanine 0.3 g/l, L-arginine monohydrochloride
0.24 g/l, L-asparagine monohydrate 0.11 g/l, L-cysteine 0.1 g/l, L-glutamic
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acid 0.3 g/l, L-glutamine 0.1 g/l, glycine 0.2 g/l, L-histidine 0.05 g/l, L-
isoleucine 0.1 g/l, L-leucine 0.1 g/l, L-lysine monohydrochloride 0.25 g/l, L-
methionine 0.1 g/l, L-phenylalanine 0.2 g/l, L—serine 0.3 g/l, L-threonine 0.2
g/l, L-tryptophane 0.1 g/l, L-tyrosine 0.05 g/l, L-valine 0.1 g/l], supplemented
with 100 ug/ml llin. The cultivations were grown at 37 °C in a fermenter
(Belach Bioteknik, BR20). When the cells d an optical density at 600
nm (ODsoo) of 0.75, approximately 2.6 l of the cultivation was infected using a
x molar excess of M13K07 helper phage (New England Biolabs, cat. no.
N0315S). The cells were incubated for 30 minutes, whereupon the fermenter
was filled up to 20 | with TSB-YE (Tryptic Soy Broth-Yeast Extract; 30 g/l
TSB, 5 g/l yeast extract) supplemented with 100 uM isopropyl-B-D
thiogalactopyranoside (IPTG) for ion of expression and with 25 ug/ml
kanamycin and 12.5 ug/ml icillin and grown at 30 °C for 22 h. The cells
in the cultivation were pelleted by centrifugation at 15,900 g. The phage
particles were precipitated from the supernatant twice in PEG/NaCl
(polyethylene glycol/sodium chloride), filtered and ved in PBS and
glycerol as described in Gronwall et al., supra. Phage stocks were stored at -
80 °C before use.
ions against biotinylated human FcRn were performed in four
cycles d in two different tracks. Phage stock preparation and selection
procedure were performed essentially as described for selection against
another biotinylated target in WO2009/077175. The amplification of phage
between the ion cycles was med by infecting E. coli RRIAM15
with phage, then performing cultivation in solution as follows. Eluted phage
and 10 x excess of M13K07 helper phage compared to bacteria were d
to simultaneously infect log phase bacteria at 37 °C for 30 min without
rotation, followed by 30 min with slow rotation. Prior to infection, bacteria were
grown to log phase in the defined proline free medium described above.
Infected bacteria were pelleted by centrifugation at 4,300 g for 10 min and
resuspended in 200 ml TSB+YE medium mented with 0.1 mM lPTG,
ug/ml kanamycin and 100 ug/ml llin and cultivated at 30 °C
overnight for phage production.
The selection buffer consisted of 100 mM sodium phosphate and 150
mM sodium chloride adjusted to pH 5.5 with hydrogen chloride and
supplemented with 0.1 % gelatin and 0.1 % Tween-20. At selection, human
serum albumin (HSA, Albucult, Novozymes) was added to the ion buffer
to a final concentration of 1.5 uM. In order to reduce the amount of
background binders, pre-selection was performed by incubation of phage
stock with Dynabeads® M-280 Streptavidin ads, Dynal, cat. no.
112.06) for 1 hour at RT. A second pre-selection was performed during 30
min at RT against human B2M immobilized in immunotubes (Nunc, cat. no.
444474). 5 pg/ml of human B2M in carbonate buffer (Sigma, cat. no.
068K8214) was lized in the tube at 7 °C for >1 h. After washing twice
with tap water, the tubes were blocked with PBS + 0.5 % casein (Sigma, cat.
no. C8654) for 30 min at RT before use. All tubes and beads used in the
selection were pre-blocked with PBS + 0.1 % gelatin. Selection was
performed in solution at RT, followed by capture of target—phage complexes
on SA-beads where 1 mg beads per 2.9 pg biotinylated FcRn were used. In
cycle 1 of the selections, 100 nM biotinylated FcRn was used and two washes
of two min each were performed using selection buffer. An increased
stringency, using a lowered target concentration and an increased number of
washes, was d in the subsequent cycles: 50 nM/5 washes, 25 nM/8
washes and 10 nM/12 washes were applied in cycle 2, 3 and 4, respectively.
After the washes, bound phage was eluted from the two ion tracks
using two different ures; 1) 500 pl 0.1 M glycine-HCI, pH 2.2, followed
by immediate neutralization with 50 pl 1 M Tris-HCI, pH 8.0, and 450 pl PBS,
or; 2) 500 pl of 100 mM sodium phosphate and 150 mM sodium chloride, pH
8.0 and neutralization with 500 pl PBS.
Seguencing: PCR fragments were amplified from single colonies using
a standard PCR program and the primers AFFI-21 (5’-tgcttccggctcgtatgttgtgtg
(SEQ ID NO:385)) and AFFI—22 (5’—cggaaccagagccaccaccgg (SEQ ID
NO:386)). Sequencing of amplified fragments was performed using the
biotinylated oligonucleotide AFFI-72 (5’-biotin-cggaaccagagccaccaccgg (SEQ
ID NO:387)) and a BigDye® Terminator v3.1 Cycle Sequencing Kit (Applied
Biosystems), used in accordance with the manufacturer’s protocol. The
sequencing ons were purified by binding to magnetic streptavidin coated
beads (Detach Streptavidin Beads, g, cat. no. 2012-01) using a
Magnatrix 8000 (Magnetic Biosolution), and analyzed on ABI PRISM® 3130xl
Genetic Analyzer (PE Applied tems).
Production of Z variants for ELISA: Sequenced Z variants were
produced by inoculating single colonies from the selections into 10 ml TSB-
YE medium supplemented with 100 pg/ml llin and 0.1 mM IPTG and
incubating for 24 h at 37 °C. Cells were pelleted by fugation, re-
suspended in 2 ml PBST (PBS mented with 0.05 % Tween-20), frozen
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at —80 °C and thawed in a water bath, to release the periplasmic fraction of
the cells. The freeze-thawing procedure was repeated seven times and cells
were then pelleted by fugation. The supernatant of the periplasmic
extract contained the Z variants as fusions to ABD, expressed as
AQHDEALE-[Z#####]—VDYV-[ABD]—YVPG (Gronwall et a/., supra). Z#####
refers to dual, 58 amino acid residue Z variants.
ELISA KD analysis of Z variants: The binding of Z variants to FcRn was
ed in ELISA assays. Half-area 96-well ELISA plates were coated with 2
ug/ml of an anti-ABD goat antibody (produced in-house) diluted in coating
buffer (50 mM sodium carbonate, pH 9.6) at 4 °C overnight. The dy
solution was poured off and the wells were blocked with 100 pl of PBSC (PBS
supplemented with 0.5 % casein) for 1.5 h at RT. The blocking solution was
discarded and 50 pl periplasmic solution, diluted 1:4, was added to the wells
and incubated for 1.5 h at RT under slow shaking. The ons were poured
off and the wells were washed four times with either 0.05% PCT buffer, pH
6.0 (Mcllvaines phosphate-citrate buffer, pH 6.0, supplemented with 0.05 %
Tween-20) or 0.05% PCT buffer, pH 7.4 (Mcllvaines phosphate-citrate buffer,
pH 7.4, supplemented with 0.05 % Tween—20). The target protein, biotinylated
human FcRn, was added to the wells in a 1:3 diluted concentration series
from 2 pg/ml (45 nM) to 0.3 ng/ml (6.9 pM) diluted in PCC buffer, pH 6.0 or
pH 7.4, (Mcllvaines phosphate-citrate buffer, pH 6.0 or pH 7.4, supplemented
with 0.5 % casein), tively. The plates were incubated for 1.5 h at RT
followed by washes as described above. Streptavidin conjugated HRP
o Scientific, cat. no. N100) was diluted 1:30 000 in PCC buffer, pH 6.0
or pH 7.4, respectively, and added to the wells followed by 45 min incubation.
After washing as described above, 50 pl lmmunoPure TMB substrate
(Thermo Scientific, cat. no. 34021 ) was added to the wells and the plates
were treated according to the manufacturer’s recommendations. Absorbance
was measured at 450 nm using a multi-well plate reader, Victor3 (Perkin
Elmer). A Z variant binding an irrelevant protein was used as negative control
and a blank was created by omitting the asmic step. A Z variant which
bound to FcRn in a pre-experiment (Z07918, SEQ ID NO:1) was used as
positive control. Measured values were ed using GraphPad Prism 5
(GraphPad Software, Inc.) and non-linear regression in order to determine the
affinities (KB) of the ctions.
ELISA specificity analysis of Z variants: In another ELISA ment,
the specificities of the Z variants were tested by ng them against 2
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pg/ml biotinylated human proteins BZM, PSMA (produced in-house) and lgG
(polyclonal, Pharmacia) and against PCC buffer pH 6.0 or pH 7.4,
respectively. The assay was performed at pH 6.0 and at pH 7.4, respectively,
as described above. The biotinylated proteins or buffer were added to the
wells instead of FcRn in the target protein step.
Results
Phage display selection of FcRn binding Z variants: Individual clones
were obtained after four cycles of phage display selections against
biotinylated human FcRn.
Seguencing: Sequencing was performed on clones picked at random
from ion round four. Each Z variant was given a unique fication
number ##### and individual variants are referred to as 2#####. The amino
acid sequences of the 58 amino acid residues long Z variants are listed in
Figure 1 as SEQ ID NO:1-16 and SEQ ID .
The deduced FcRn binding motifs of these Z variants extend from
residue 8 to e 36 in sequences with SEQ ID 6 and SEQ ID
NO:353 in Figure 1. The amino acid sequences of the 49 amino acid residues
long polypeptides (BMod) predicted to constitute the te three-helix
bundle within each of these Z variants extend from residue 7 to residue 55.
ELISA assays with Z variants: Sixteen clones were produced as ABD
fusion proteins in E. coli. The periplasmic fractions were used in an ELISA
against a dilution series of human FcRn. The clones were: 207909 (SEQ ID
NO:13), 207918 (SEQ ID NO:1), 207930 (SEQ ID NO:6), 207960 (SEQ ID
N024), 210109 (SEQ ID NO:3), 210111 (SEQ ID N028), 210127 (SEQ ID
NO:12), 210129 (SEQ ID NO:9), 210140 (SEQ ID NO:5), 210141 (SEQ ID
NO:10), 210145 (SEQ ID NO:15), 210152 (SEQ ID NO:14), 210156 (SEQ ID
NO:11), 210161 (SEQ ID NO:16), 210183 (SEQ ID NO:7) and 210193 (SEQ
ID NO:2). KD values were ined for all variants at pH 6.0 and for three
variants at pH 7.4 (Table 2). For thirteen variants, data was not obtained for a
KD is at pH 7.4. None of the sixteen variants displayed non—specific
binding when assayed against human B2M, lgG or PSMA.
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Table 2. ELISA KD is of Z-ABD variants in E. coli periplasmic fractions.
z variant SEQ ID NO: KD pH 5.0 (M) KD pH 7.4 (M)
207909 13 24.5 x10'9 n.d.
207918 1 2.0 x10'9 10.9 x10'9
207930 5 10.4 x10'9 n.d.
207950 4 5.0 x 10'9 n.d.
210109 3 3.9 x 10'9 23.9 x 10'9
210111 8 11.4x10'9 n.d.
210127 12 21.3 x10'9 n.d.
210129 9 17.5 x10'g n.d.
210140 5 8.8 x 10'9 n.d.
210141 10 21.2 x10'9 n.d.
210145 15 42.0 x10'9 n.d.
210152 14 24.5 x10'9 n.d.
210155 11 21.3 x10'9 n.d.
210151 15 153.0 x10'9 n.d.
210183 7 10.9 x10'9 n.d.
210193 2 2.3 x10'9 25.9 x10"g
n.d.= not determinable
Example 3
Production and characterization of FcRn binding Z variants
In this e, seventeen Z variants were produced in E. coli, purified
and assayed t human FcRn in Biacore. A subset of said ts was
also assayed against mouse FcRn. Circular dichroism (CD) spectroscopy was
performed for a subset of Z variants for investigation of their ary
structure.
Materials and methods
Subcloning of Z variants: The DNA of seventeen FcRn binding Z
variants (SEQ ID NO:1-16 and SEQ ID NO:353) was amplified from the
library vector pAY02592. A subcloning strategy for construction of ric
Z variant molecules with N-terminal Hise tag was applied using standard
molecular biology techniques (essentially as described in detail in
W02009/077175 for Z variants binding another target). The Z gene fragments
were subcloned into the expression vector pAY01448 resulting in the
encoded sequence MGSSHHHHHHLQ-[Z#####]—VD.
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In addition, the FcRn binding variant 207918 (SEQ ID NO:1), but
starting with the amino acids AE instead of VD and denoted 211948 (SEQ ID
NO:354), was cloned as homodimeric constructs with two different s
between the Z variants and followed by a inal Hise tag. This was
performed using conventional molecular biology methods including DNA
ication, restriction with suitable restriction enzymes and ligation of the
DNA. The two s were obtained from Thermo Fisher Scientific. The Z
gene fragments were subcloned into the expression vector (pET-26 origin,
Novagen) resulting in the encoded sequence [Z#####]—GT—(G4S)—PR-
#]-LEHHHHHH and [Z#####]-GT-(G4S)3-[Z#####]—LEHHHHHH,
respectively.
Cultivation and cation: E. coli BL21(DE3) cells (Novagen) were
transformed with plasmids containing the gene fragment of each respective
FcRn binding Z variant and cultivated at 37 °C in 800 or 1000 ml of TSB—YE
medium supplemented with 50 ug/ml kanamycin. At ODBOO = 2, IPTG was
added to induce expression at a final concentration of 0.17 or 0.2 mM and the
culture was incubated at 37 °C for another 5 h. The cells were ted by
centrifugation.
Approximately 2-5 g of each cell pellet was resuspended in 10-25 ml
binding buffer (20 mM sodium phosphate, 0.5 M NaCl, 20 mM imidazole, pH
7.4) supplemented with ase® (Merck, cat. no. 1016540001) to a
concentration of 15 U/ml and me (Sigma, cat. no. L-7651) to a
concentration of 0.5 mg/ml. After cell disruption by three freeze-thawing
cycles or sonication, cell debris was removed by centrifugation and each
atant was applied on a 1 ml His GraviTrap IMAC column (GE
Healthcare, cat. no. 1199). Contaminants were removed by washing
with wash buffer (20 mM sodium phosphate, 0.5 M NaCl, 20 or 60 mM
imidazole, pH 7.4), and the FcRn binding Z variants were subsequently eluted
with elution buffer 1 (20 mM sodium phosphate, 0.5 M sodium chloride, 250
mM imidazole, pH 7.4) or elution buffer 2 (0.1 M acetic acid, 0.5 M sodium
chloride, pH 4.5). ed Z variants were buffer exchanged to PBS using PD-
columns (GE Healthcare), ing to the manufacturer’s protocol.
Protein concentrations were determined by measuring the absorbance at 280
nm, using a NanoDrop® ND-1000 spectrophotometer, and using the
extinction coefficient of the respective protein. The purity of the FcRn binding
Z variants was analyzed by SDS-PAGE stained with Coomassie Blue. The
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identity of each purified FcRn binding Z variant was confirmed using LC/MS
analysis.
CD analysis: Purified Hise-tagged Z variants were diluted to 0.5 mg/ml
in PBS. For each diluted Z variant, a CD spectrum at 250—195 nm or 250-190
nm was ed at 20 °C. In addition, a variable temperature measurement
(VTM) was med to determine the melting temperature (Tm). In the VTM,
the absorbance was measured at 221 nm while the temperature was raised
from 20 to 90 °C, with a temperature slope of 5 °C/min. A new CD spectrum
was obtained at 20 °C after the heating procedure in order to study the
refolding ability of the Z variants. The CD measurements were performed on
a Jasco J-810 spectropolarimeter (Jasco Scandinavia AB) using a cell with an
optical path-length of1 mm.
Biacore binding and c analysis: The ction of FcRn binding
Hise-tagged Z variants with human FcRn was analyzed in a Biacore 2000
instrument (GE Healthcare). Human FcRn was immobilized in a flow cell on
the carboxylated dextran layer of a CM5 chip surface (GE care). The
lization was performed using amine coupling chemistry ing to
the manufacturer’s protocol and using HBS—EP (GE Healthcare) as running
buffer. One flow cell surface on the chip was ted and deactivated for
use as blank during analyte injections. In the two binding experiments
presented below, Mcllvaines phosphate-citrate buffer pH 6.0 mented
with 0.005 % Tween—20 (0.005 % PCT) was used as running buffer. In all
experiments, a flow rate of 50 ul/min was used.
In one experiment, the dissociation at pH 6.0 was compared to the
dissociation at pH 7.4. Hiss-tagged Z variants and a human monoclonal IgG1
were d in g buffer to a final concentration of 250 nM or 2.5 nM,
respectively, and injected over the FcRn chip for 1 minute using the co-inject
procedure. The second injection of the co-inject procedure, representing the
dissociation phase of the interactions, contained either running buffer (pH 6.0)
or 0.005% PCT pH 7.4. The Z variants were allowed to dissociate for 1
minute, except for 207918 and 210193, which were allowed to dissociate for
4 minutes, before a e equilibration during 5 minutes in g buffer.
IgG was allowed to dissociate for 4 minutes before equilibration. Buffer
injections were performed in a similar way; ection of buffer pH 6.0
followed by pH 6.0 or co-injection of buffer pH 6.0 followed by pH 7.4. The
results were analyzed in BiaEvaluation software 4.1 (GE Healthcare). Curves
of the blank surface were subtracted from the curves of the ligand surface. In
on, curves of buffer injections were subtracted from the Z variant curves
and from the IgG curves to adjust for the buffer s.
In r ment, approximate kinetic constants (kon and koff) and
affinities (KD) were determined for a subset of Hise-tagged 2 variants. Three
concentrations of the Z ts were injected for 1 minute followed by
dissociation in running buffer for 1 minute. The surfaces were equilibrated
with running buffer during 7.5 minutes before the start of next cycle. Injected
concentrations were either 675 nM, 225 nM and 75 nM (210140, 210156 and
210183) or 225 nM, 75 nM and 25 nM (207918 and 210193). Kinetic
constants were calculated from the sensorgrams using the Langmuir 1:1
model of BiaEvaluation software 4.1 (GE Healthcare).
In a separate experiment, the affinity of the interactions of 2 variants to
hFcRn (SEQ ID NO:379) and chRn (SEQ ID NO:384), respectively, was
measured at both pH 6.0 and pH 7.4 on a Biacore 3000 ment (GE
care). hFcRn and chRn were produced essentially as described in
Example 1 but using mouse 3T3 cells instead of human SKOV—3 cells for
production of chRn, and immobilized on separate flow cells on a CM5 chip
in e buffer at pH 4.65. The immobilization level was approximately 1000
RU for both receptors. A nce flow cell was created by activation and
deactivation. 0.005% PCT pH 6.0 or 7.4 was used as running buffer and for
dilution of the analytes. All es were performed at 25 °C. The affinity
nts for the His6—tagged 2 variants 207918 (SEQ ID NO:1), 207960
(SEQ ID NO:4) and 210193 (SEQ ID NO:2) were determined by injecting a
dilution series from 1024 nM to 0.5 nM (pH 6.0) or from 10240 nM to 5 nM
(pH 7.4). The affinities were derived using GraphPad Prism 5 software, using
a one site binding saturation model.
AlphaLlSA blocking assay: The potential of 2 variants to inhibit binding
of IgG to FcRn was analyzed in an AlphaLlSA assay with an EnSpire
multiplate reader 2300 (Perkin Elmer). Human IgG (Roactemra) was
immobilized on AlphaLlSA acceptor beads (Perkin Elmer, cat. no. 6772002)
according to the manufacturer’s recommendations. Stepwise serial dilutions
1:3 of His-tagged 2 variants to final concentrations of 250 nM to 38 pM were
made in a 384-well plate n Elmer, cat. no. G6005350) and incubated for
45 min with 10 nM biotinylated human FcRn (Biorbyt, cat. no. orb84388;
biotinylated essentially as described in Example 2) in AlphaLlSA buffer
(Perkin Elmer, cat. no. ALOOOF) adjusted to pH 6.0 using HCI. IgG—coated
Acceptor beads were added to a final concentration of 10 uM and incubated
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for 45 min. Finally, streptavidin coated Donor beads (Perkin Elmer, cat. no.
2) were added to a final concentration of 40 ug/ml and incubated for
min. All incubations were performed at RT in the dark. The plate was
analyzed in the EnSpire instrument and the |C50 values were calculated
using GraphPad Prism 5.
Results
Cultivation and purification: The seventeen FcRn binding Z variants
(SEQ ID NO:1-16 and SEQ ID NO:353), constructed with an N-terminal Hise
tag, were produced in E. coli. The amount of lMAC-purified protein from
approximately 2—5 g ial pellets, determined spectrophotometrically by
measuring the ance at 280 nm, ranged from approximately 10 mg to
mg for the different FcRn binding Z variants. GE analysis of each
final protein preparation showed that these predominantly contained the FcRn
binding Z variant. The correct identity and molecular weight of each FcRn
binding Z variant was confirmed by HPLC—MS analysis.
CD analysis: The CD spectra determined for six Z ts showed that
each had an d—helical structure at 20 °C. This result was also verified in the
variable temperature measurements, wherein g temperatures (Tm)
were determined (Table 3). A reversible folding was seen for the six Z
variants when overlaying spectra measured before and after g to 90 °C.
Table 3. Melting temperatures for a selection of Z ts.
Zvariant SEQ ID NO: Tm °C)
207909 13 56
207918 1 49
207930 6 56
207960 4 58
210109 3 61
210193 2 59
Biacore binding and c analyses: The binding of seventeen Hise-
tagged 2 variants to human FcRn and the dissociation at different pH were
tested in a Biacore instrument by sequentially injecting each of the 2 variants
at pH 6.0 and either buffer pH 6.0 or pH 7.4 over a chip surface containing
FcRn. The ligand immobilization level of the surface was 1668 RU human
FcRn. The seventeen 2 variants showed binding to FcRn at pH 6.0, and for
WO 2016042083
all variants, faster tes were seen at pH 7.4 compared to pH 6.0. The
result for IgG was similar, ying a faster off-rate at pH 7.4. The variants
207918 and 210193 showed the slowest dissociation curves. Sensorgrams
for a subset of variants and IgG are displayed in Figure 2 A-E.
Table 4. Biacore kinetic constants and affinities for hFcRn binding at pH 6.0.
2 variant SEQ ID NO: kon (M'1s'1) km:f (s'1) KD (M)
207918 1 1.4 x106 0.022 1.6 x10'8
210140 5 1.4 x106 0.12 8.6 x10'8
210156 11 7.6 x105 0.28 3.7 x10'7
210183 7 1.0x106 0.13 1.3x10'7
210193 2 1.5 x106 0.033 2.2 x10"8
The kinetic nts of five Z variants interacting with FcRn at pH 6.0
were determined (see Table 4). The immobilization level of the surface was
2015 RU human FcRn. For each Z variant, kinetic constants were calculated
using a curve set of three injected concentrations.
Affinity (KD) constants were also determined for Hise-tagged Z variants
207918 (SEQ ID NO:1), 207960 (SEQ ID N024) and 210193 (SEQ ID N022)
interacting with human and mouse FcRn at pH 6.0 and pH 7.4 (Table 5). For
all three ts, KD values were lower at pH 6.0 compared to pH 7.4.
Table 5. Biacore ties for hFcRn and chRn at pH 6.0 and pH 7.4.
SEQ ID KD (M) hFcRn KD (M) chRn
Z variant_
NO: pH 6.0 pH 7.4 pH 6.0 pH 7.4
207918 1 1.2 x10'8 >5 x10'7 9.0 x10'8 >5 x10'7
207960 4 5.0 x10'8 >1 x10'6 3.5 x107 >5 x10'6
210193 2 1.4x10'8 >5x10'7 9.5x10'8 >5x10'7
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Table 6: Calculated I050 values from AlphaLlSA blockino assa .
z variant SEQ ID NO I050 (M)
207909 _\ 00 4.6 x 10'8
207918 A 2.1 x10'9
|207930 4.2 x 10'8
207960 A 4.2 x 10'8
210109 5.7 x 10'8
210111 4.6x10'8
210140 5.6 x 10'8
210183 3.9 x10'8
210193 1.2x10'8
213993 1.3 x 10'7
211948-(G4S)-211948 3.8 x 10'10
21 1948-(G4S)3-Zi 1948 4.1 x 10'10
AlphaLlSA blocking assay: The y of seventeen Hise-tagged
monomeric Z variants (SEQ ID NO:1-16 and SEQ ID NO:353) and two
dimeric variant, 211948-G4S-211948 and Z11948-(G4S)3-211948 to inhibit
lgG binding to FcRn was tested in an AlphaLlSA blocking assay. Serial
dilutions of the Z variants were incubated with biotinylated human FcRn and
the blocking ability of each respective variant was measured after addition of
IgG coated Acceptor beads and subsequently streptavidin coated Donor
beads. Inhibition could be measured as a decrease in AlphaLlSA counts for
positive Z variants. The calculated IC50 values for the ten monomeric variants
and the two dimeric variants that were shown to block IgG binding to FcRn in
this assay are shown in Table 6.
Binding of FcRn binding Z variants to human or mouse FcRn/eGFP
transfected HeLa cells
In this Example, the binding ability of FcRn g Z variants was
investigated. The production of HeLa cells expressing human and murine
GFP gene ene and the use of these cells for flow cytometry
analysis with Alexa Fluor® 647 d Z variants is described.
Materials and methods
Cloning of FcRn-eGFP and 82M viral vectors: The genes encoding
murine FcRn (chRn, Genbank BC003786.1, OpenBiosystems) and murine
B2M (mB2M, Genbank BC085164.1, OpenBiosystems) were amplified in a
similar way as the genes for human FcRn and human B2M as bed in
Example 1. Human and murine FcRn and B2M genes were amplified as
follows: for hFcRn, the sequence encoding amino acids 1-365 (SEQ ID
NO:382) was amplified; for hBZM, the sequence encoding amino acids 21-
119 (SEQ ID NO:380) was ied; for chRn, the sequence encoding
amino acids 1—369 (SEQ ID NO:383) was amplified; and for mB2M, the
sequence encoding amino acids 21-119 (SEQ ID NO:381) was ied. The
vector pHR-cPPT-CMV-EGFP (Jakobsson etal. (2003) J Neurosci Res
73:876-85) and FcRn PCR amplicons (human and murine) were cut using the
restriction s BamHl (human) or Bcll (murine) and Mlul (New England
Biolabs, cat. nos. R0136M, R0160L and , respectively), and ligated
using T4 DNA Ligase (New England Biolabs, cat. no. M0202M). The ligation
mix was chemically ormed into E. coli RRIAM15 and spread on
ampicillin plates. Colonies were picked and screened with suitable primer
pairs. The construct encoding the al signal peptide, human or murine
FcRn and eGFP at the cytoplasmic tail were verified by cing and
denoted pHR-cPPT-CMV-hFcRn-eGFP and pHR-cPPT-CMV-chRn-eGFP,
respectively.
The human and murine B2M PCR amplicons were inserted into the
d pDONOR221 (Invitrogen, cat. no. 12536—017) by recombination using
the y system (Invitrogen, cat. no. 11789020, Gateway® BP Clonase®
II Enzyme mix) according to the manufacturer’s recommendations. After
verification of correct sequences, human or murine B2M was inserted into
tc (Suter et al., supra) using a multi-site gateway cloning system
(Invitrogen, cat. no. 11791020, Gateway® LR Clonase® II Enzyme mix)
er with the promoter containing d pENTR-CMV (Tai et al. supra),
resulting in the vectors 2k7neo—CMV-hB2M and 2k7neo-CMV-mB2M,
respectively.
Lentiviral transduction of HeLa cells: The vector pairs 2k7neo-CMV-
hB2M and pHR-cPPT-CMV-hFcRn-eGFP or 2k7neo-CMV-mB2M and pHR-
cPPT-CMV-chRn-eGFP were co-transfected together with VSV-G envelope
and gag/pol packaging plasmid into HEK293T cells using calcium chloride
transfection (Zufferey et al., supra; Jakobsson et al. (2006) supra). HEK293T
culture atants containing formed lentiviral particles with FcRn and 82M
transgenes respectively were used to sequentially transduce HeLa Cervix
adenocarcinoma cells (Cell Line e) at low passage number. The
ing two stably transduced HeLa cell lines are in the following d
hFcRn-eGFP (transduced with genes for human FcRn-eGFP and hB2M) and
chRn—eGFP (transduced with genes for mouse FcRn-eGFP and mB2M).
Alexa Fluor® 647 ng of FcRn binding Z variants: The three Hise-
tagged Z variants 207918, 207930 and 207960 were labeled with Alexa
Fluor® 647 Carboxylic Acid Succinimidyl Ester (lnvitrogen cat. no. A20106).
Before labeling, buffer was exchanged to 0.2 M carbonate , pH 8.3,
using Vivaspin500 centrifugal filter units (10 kDa MWCO, Vivaproducts cat.
no. 512—2838) spun at 10,000 g. The labeling was performed in the
in500 and 1 pl of Alexa Fluor® 647 Succinimidyl Ester dye (40 pg/pl in
DMSO corresponding to 1.3 x molar excess) was added to 200 pg/25 pl Z
variant. The mixes were incubated at RT in the dark for 40 minutes in a
wiggling rota mixer. The reaction mixes were subsequently put on ice for 3.5
hours and free dye was removed by washing with 15 x 100 pl PBS in the
Vivaspin500.
lmmunofluorescence staining of human and mouse FcRn-eGFP
transfected HeLa-cells with FcRn binding Z variants: hFcRn-eGFP and
chRn-eGFP HeLa cells were harvested by trypsination and washed twice in
PBS at pH 6.0 before counting. 100,000 cells were ed per well of a v-
ed 96 well plate (Nunc, cat no 277143) and the cells in the plate were
subsequently pelleted at 1,700 rpm for 4 min at 4 °C. The supernatants were
removed and the cells were fixed with 50 pl of 2 % formaldehyde (Sigma
Aldrich, cat. no. F8775) in PBS at pH 6.0 for 10 min at RT. Cells were
thereafter washed with 2 x 100 pl PBS, pH 6.0, saturated with casein (PBSC),
and resuspended in PBSC with 0.1 % saponin (AppliChem, cat no
A4518.0100) containing 620 nM of Alexa Fluor® 647 labeled Hiss-tagged Z
variants; 207960, 207930 and 207918. Transduced HeLa cells, incubated
with buffer alone, were used as l. The cells were incubated for 1 h at 8
°C on a shaker in the dark, washed with 2 x 100 pl PBSC and resuspended in
180 pl of PBS, pH 6.0, containing 1 % BSA (fraction V, Merck, cat. no.
1.12018.0100). 10,000 cells/well were analyzed in a Gallios Flow Cytometer
(Beckman Coulter) and the data was analyzed using Kaluza software
an Coulter).
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Results
Flow cytometry analysis was utilized to determine whether the FcRn
binding Z variants could bind to human and/or mouse FcRn on human or
mouse FcRn/eGFP transduced HeLa cells. The experiment was performed at
pH 6.0 with Alexa Fluor® 647 labeled 207960, 207930 and 207918 (SEQ ID
N04, 6 and 1, respectively). Dot plot is (y-axis: Alexa Fluor® 647, x-
axis: eGFP) showed that the transduced cell tion could be divided into
FcRn-eGFP negative and positive population (Figure 3, gate H and l,
respectively) indicating heterogeneous expression of the FcRn-eGFP fusion
protein by HeLa cells (Figure 3). Accordingly, the mean fluorescence intensity
(MFI) values for Alexa Fluor® 647 in gate l were subtracted by background
MFI values of Alexa Fluor® 647 in gate H. The calculated MFI values are
ted in Figure 4. The results show that 207960, 207930 and 207918 are
capable of binding HeLa cells displaying human (Figure 4A) or murine (Figure
4B) FcRn-eGFP.
Blocking of lgG binding to FcRn with the FcRn binding 2 variant 207918
In this Example, the potential competition of FcRn g 2 variants
with lgG for binding to FcRn was igated in a cell based assay. Such
binding will result in blocking of the lgG-FcRn interaction.
Materials and methods
Blocking of lgG-FcRn immunofluorescence ng: Human or murine
FcRn-eGFP transduced HeLa cells were prepared as described in Example
4. Fixed cells were resuspended in 50 pl of a mix of either 100 nM Alexa
Fluor® 647-conjugated human or mouse lgG (Jackson laboratories, cat. no.
009003 and 0-003, respectively) and 1000, 100, 10, 1 or 0 (buffer
control) nM Hise-tagged 207918 d in PBS-casein, pH 6.0, ning 0.1
% saponin (AppliChem). The cells were incubated for 1 h at 37 °C on a
shaker in the dark, washed with 2 x 100 pl PBS-casein pH 6.0 and re-
suspended in 180 pl of PBS, pH 6.0, containing 1 % BSA. Data from 10,000
cells/well (except somewhat fewer cells for mouse 100 nM mlgG-Alexa
Fluor® 647) were obtained using a Gallios Flow Cytometer (Beckman
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r) and the data was analyzed using Kaluza software (Beckman
Coulter).
Results
The experiment was performed to ine if the FcRn binding Z
variant 207918 (SEQ ID NO:1) blocks the IgG-FcRn interaction. Human or
murine FcRn-eGFP transduced HeLa cells were incubated with human or
mouse Alexa Fluor® 647-conjugated lgG. The binding was blocked with
unlabeled 207918 at different concentrations. Due to the heterogeneous
expression of FcRn by the transduced HeLa cells (described in Example 4),
the MFI values for Alexa Fluor® 647 in gate N of each sample was cted
by the corresponding MFI values in gate M (Figure 5). The t lgG Alexa
Fluor® 647 binding was calculated by dividing the different MFI values with
the MFI for the blank control. The results showed that 207918 effectively
blocked hlgG g to hFcRn (Figure 6A) in a dose dependent manner.
rmore, 207918 also blocked mlgG binding to chRn (Figure 6B)
although less efficiently ed to hIgG-binding.
e 6
Pharmacokinetic study of three FcRn binding 2 variants
In this Example, the ability of FcRn binding 2 variants to g serum
half-life of a non-specific 2 variant was investigated by a pharmacokinetic
study performed in mice.
Materials and methods
Subcloning of 2 variants: A subset of 2 variants (207918, 207960 and
210193) was submitted to a second ning. DNA from the subcloned
Hise-tagged variants in Example 3 was used as template. First, PCR
amplification using suitable primer pairs was performed to create genes
encoding 2 variants starting with the amino acids AE instead of VD. The
mutated 2 variants are listed in Figure 1 and were denoted 211948 (SEQ ID
NO:354), 211946 (SEQ ID NO:355) and 211947 (SEQ ID NO:356),
corresponding to mutated 207918, 207960 and 210193, respectively. Genes
ng the new 2 variants were restriction cleaved and ligated into a vector
harboring the genes encoding albumin binding variant PP013 (SEQ ID
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) and 203638 (SEQ ID NO:378) with spacer sequences resulting in a
gene fusion encoding [2#####]-GAP(G4S)4TS—[PP013]—GT(G4S)4PR-[ZO3638]
(also denoted “Z#####—PP013—203638” or “Z variant in fusion with PP013-
203638”). The negative control molecule [203638]—GAP(G4S)4TS—[PP013]
was subcloned in a similar way by ligating 203638 into a vector containing a
(G4S)4 linker and the sequence for PP013. The subsequent steps for vector
transformation into E. coli were performed as in Example 3.
ation and purification: Z variants in fusion with 203638
were produced in E. coli as described in Example 3. Approximately 3 g of
each cell pellet was re—suspended in 30 ml TST-buffer (25 mM Tris-HCl, 1
mM EDTA, 200 mM NaCl, 0.05 % Tween20, pH 8.0) supplemented with
ase®(Merck). After cell disruption by sonication and clarification by
centrifugation, each supernatant was applied on a gravity flow column with 5
ml agarose immobilized with an anti—ABD ligand (see WO2014/064237). After
washing with TST-buffer and 5 mM NH4Ac buffer, pH 5.5, the Z variants were
eluted with 0.1 M HAc. Acetonitrile (ACN) was added to a final concentration
of 10 % to the eluted fractions from the anti-ABD e affinity
chromatography cation step and the samples were loaded on a 3 ml
ce 15RPC column (GE Healthcare), previously equilibrated with RPC
solvent A (0.1 % trifluoroacetic acid (TFA), 10 % ACN, 90 % water). After
column wash with RPC solvent A, bound protein was eluted with a linear
gradient 0-50 % RPC solvent B (0.1 % TFA, 80 % ACN, 20 % water) during
60 ml. Fractions containing pure Z variant were identified by SDS—PAGE
analysis and pooled. After the RPC purification, the buffer of the pools was
exchanged to PBS using a HiPrep 26/10 Desalting column (GE Healthcare).
Finally, the Z variants were ed on 1 ml EndoTrap red columns (Hyglos,
cat. no. 321063) to ensure low endotoxin content.
Protein concentrations, purities and the identity of each purified Z
variant were analyzed as described in Example 3.
Biacore analysis: Expressed and purified Z variants fused to PP013-
203638 were assayed against human FcRn at pH 6.0 essentially as
described for the kinetic analysis in Example 3. The 2 variants and the
ve control 203638-PP013 were injected at 40 nM, 160 nM and 640 nM
during 1 minute ed by dissociation for 2.5 minutes and equilibration for 1
minute. Kinetic nts and affinities were determined for the 2 variants
using the luation software.
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Pharmacokinetic study: 211947, 211946 and 211948 fused to PP013-
203638 were administered intravenously (i.v.) to male NMRI mice (Charles
River, Germany) at a dose of 92 nmol/kg body weight. Sera from groups of
three mice were obtained at 0.08, 6, 18, 78, 120, 168 and 240 hours. The
concentration of respective Z variant was determined by ELISA.
ELISA: Half-area 96-well ELISA plates were coated at 4 °C overnight
with 50 ul/well of an Z specific goat dy (produced in-house) diluted to 4
ug/ml in coating buffer (50 mM sodium carbonate, pH 9.6). The antibody
on was poured off and the wells were blocked with 100 pl of PBSC for
1.5 h at RT. The sera were diluted in PBSC containing 1 % mouse serum
(matrix) from 1:100 to 1:51 ,200 in a two-fold dilution series in a dilutions plate.
A standard ion for respective Z variant and four quality controls (very low,
low, medium and high control) diluted in matrix were included on each plate.
50 ul of the dilutions were transferred per well and the ELISA plates were
incubated for 1.5 h at RT. The plates were washed four times with PBST.
Bound Z variants were detected with 50 ul/well of rabbit anti-PPO13 lg
(produced in-house) diluted to 4 ug/ml in PBSC. The plates were
subsequently incubated for 1.5 h at RT followed by washes as described
above. HRP conjugated donkey abbit HRP obtained from Jackson
laboratories (cat. no. 711152), d 120,000 in PBSC, was added and
the plates were incubated for 1 hour. After washing as described above, 50 ul
of ImmunoPure TMB substrate was added to the wells and the plates were
developed according to the manufacturer’s recommendations. After 15
minutes of development, the absorbance was ed at 450 nm using a
multi-well plate reader (Victor3). The ance values were analyzed using
GraphPad Prism 5 to determine the concentrations -spline curve fit) and
area under curve (AUC). The concentrations were then plotted as their
natural logarithms t time. The resulting curves followed a two
compartment model and the terminal half-life was ated as ln2 divided by
the slope based on the last three time points.
Results
Cultivation and cation: The three FcRn binding Z variants 211947,
211946 and 211948 (SEQ ID NO:356, 355 and 354), constructed as Z#####-
PP013-ZO3638, and the negative l ZO3638-PP013, were produced in E.
coli. The amount of purified protein from approximately 3 g bacterial pellets,
determined spectrophotometrically by measuring the absorbance at 280 nm,
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ranged from approximately 10 to 25 mg for the ent FcRn binding Z
variants. SDS—PAGE analysis of each final protein ation showed that
they predominantly ned respective FcRn binding Z variant. The correct
molecular weight of each FcRn binding Z variant was med by LC/MS
analysis.
Table 7. Kinetic constants and affinities for FcRn at pH 6.0 of Z variants
produced as fusions to PPO13-ZO3638.
z t SEQ ID NO: k0,,(M'1s'1) k0,.f (5") K5 (M)
211948 354 7.73 x105 0.047 6.2 x108
211946 355 3_35 X105 0.275 82 )(10'7
211947 356 5,54 X105 0.064 9_8 x1o'8
Biacore analysis: The binding to FcRn was analyzed for the three
PP013-ZO3638 fused Z variants. The immobilization level of the surface was
548 RU of human FcRn. The resulting rough kinetic constants and affinities
for the target binding at pH 6.0 are displayed in Table 7. Fitted curves are
displayed in Figure 7A-C. The negative control ZO3638—PP013 was ve
against FcRn.
cokinetic study: The pharmacokinetic profiles of the above-
mentioned constructs of Z variants fused to ZO3638 were compared to
the negative control ZO3638—PP013 in a mouse pharmacokinetic study. In
previous work, e.g. as described in PCT application WO2009/016043, it is
shown that ABD fusion proteins have a long half-life in serum, caused by ABD
binding to serum albumin. In accordance with the previous results, terminal
half-life of ABD-fused Z variant molecule (ZO3638—PP013) was approximately
43 hours, which is comparable to half—life of mouse albumin (35 hours). The
terminal half-lives of the constructs ning FcRn g Z variant
molecule in addition to ABD were two— to three-fold longer (Figure 8). The
calculated terminal half-lives were 99 hours (211947), 69 hours (211946) and
58 hours (Z11948), suggesting that FcRn binding of the Z variants contributed
to the prolonged half-life.
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Example 7
Design and construction of a maturation library of FcRn binding Z variants
In this Example, a maturated library was constructed. The library was
used for selections of FcRn binding Z variants. Selections from maturated
libraries are usually expected to result in binders with increased affinity
(Orlova et al., (2006) Cancer Res 66(8):4339-48). In this study, randomized
single stranded linkers were generated using split-pool synthesis enabling
incorporation of defined codons in desired ons in the sis.
Materials and methods
Library design: The library was based on the sixteen sequences of the
human FcRn binding Z variants in Table 1 and further described in es
2-6. In the new library, 13 variable positions in the Z molecule ld were
biased towards certain amino acid residues, according to a strategy mainly
based on the binding motifs of the Z variants defined in SEQ ID NO:1-16. A
DNA linker was generated using split—pool synthesis containing the 147 bp
lly randomized helix 1 and 2 of the amino acid sequence: 5’- AA ATA
AAT CTC GAG GTA GAT GCC AAA TAC GCC AAA GAA NNN NNN NNN
GCG NNN NNN GAG ATC NNN NNN TTA CCT AAC TTA ACC NNN NNN
CAA NNN NNN GCC TTC ATC NNN AAA TTA NNN GAT GAC CCA AGC
CAG AGC TCA TTA TTT A -3’ (SEQ ID NO:388; randomized codons are
illustrated as NNN) flanked by restriction sites Xhol and Sacl, was d
from DNA 2.0 (Menlo Park, CA, USA). The theoretical butions of amino
acid residues in the new library, including eight variable amino acid positions
(9, 10, 11, 13, 14, 24, 32 and 35) and five constant amino acid positions (17,
18, 25, 27 and 28) in the Z le scaffold are given in Table 8. The
resulting theoretical library size is 5.3 x 108 variants.
2015/071339
Table 8: Desion of librar for maturation.
Amino acid Randomization (amino acid
Proportion
position in the abbreviations)
Z variant
9 A,D,E,F,H,|,K,L,N,Q,R,S,T,V,W,Y 1/16
_AF,H 25% ,|,K,,,LNQR,,,,,STVWY
17 ___
—_-—
—_-—
Library construction: The library was amplified using AmpliTaq Gold
polymerase (Applied Biosystems, cat. no. 4311816) during 12 cycles of PCR
and pooled products were purified with ck PCR Purification Kit
(QIAGEN, cat. no. 28106) according to the supplier’s recommendations. The
purified pool of randomized library fragments was ed with restriction
enzymes Xhol and Sacl-HF (New England Biolabs, cat. no. R0146L, and cat.
no. R3156M) and concentrated using a PCR Purification Kit. uently,
the product was subjected to preparative 2.5 % agarose (Nuisieve GTC
agarose, Cambrex, lnvitrogen) gel electrophoresis and purified using
QIAGEN gel tion Kit N, cat. no. 28706) according to the
supplier’s recommendations.
The phagemid vector pAY02592 (essentially as pAffi1 described in
ll et a/., supra) was cted with the same enzymes, purified using
phenol/chloroform extraction and ethanol precipitation. The restricted
fragments and the restricted vector were ligated in a molar ratio of 5:1 with T4
DNA ligase (Fermentas, cat. no. EL0011) for 2 hours at RT, followed by
overnight incubation at 4 °C. The ligated DNA was recovered by
phenol/chloroform extraction and ethanol precipitation, followed by dissolution
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in 10 mM Tris-HCI, pH 8.5. Thus, the resulting library in vector pAY02592
encoded Z variants, each fused to an albumin binding domain (ABD) derived
from streptococcal protein G.
The ligation ons (approximately 160 ng DNA/transformation) were
oporated into electrocompetent E. coli ER2738 cells (50 pl, Lucigen,
Middleton, WI, USA). Immediately after oporation, approximately 1 ml of
recovery medium (supplied with the ER2738 cells) was added. The
transformed cells were incubated at 37 °C for 60 min. Samples were taken for
titration and for determination of the number of transformants. The cells were
thereafter pooled and cultivated overnight at 37 °C in 1 l of TSB-YE medium,
supplemented with 2 % glucose, 10 pg/ml tetracycline and 100 ug/ml
ampicillin. The cells were pelleted for 7 min at 4,000 g and resuspended in a
PBS/glycerol on (approximately 40 % glycerol). The cells were aliquoted
and stored at —80 °C. Clones from the library of Z variants were sequenced in
order to verify the content and to evaluate the outcome of the constructed
library vis-a-vis the library . Sequencing was performed as described in
Example 1 and the amino acid distribution was verified.
Preparation of phage stock: Phage stock containing the phagemid
library was prepared in a 20 l fermenter (Belach Bioteknik). Cells from a
ol stock containing the phagemid library were inoculated in 10 l of TSB—
YE (Tryptic Soy Broth-Yeast Extract; 30 g/l TSB, 5 g/l yeast extract)
mented with 1 gil glucose, 100 mg/l ampicillin and 10 mg/l tetracycline.
When the cells reached an optical density at 600 nm (OD600) of 0.6,
approximately 1.5 l of the cultivation was infected using a 5 x molar excess of
M13K07 helper phage. The cells were ted for 30 min, whereupon the
fermenter was filled up to 10 l with x fermentation medium [2.5 g/l
(NH4)2SO4; 5.0 g/l yeast extract; 30 g/l tryptone, 2 g/l K2HPO4; 3 g/l KH2PO4,
1.25 g/l; Na3C6H507 - 2 H20; Breox FMT30 antifoaming agent 0.1 mill]. The
following components were added: 10 ml carbenicillin 25 mg/ml; 5 ml
kanamycin 50 mg/ml; 1 ml 1 M isopropyl-B-Dthiogalactopyranoside (IPTG);
17.5 ml/l of 300 g/l MgSO4, and 5 ml of a trace t solution [35 g/l FeCI3 -
6 H20; 10.56 9/] ZnSO4 - 7 H20; 2.64 g/l CuSO4 - 5 H20; 13.2 g/l MnSO4 -
H20; 13.84 g/l CaClz - 2 H20, dissolved in 1.2 M HCI]. A glucose limited fed-
batch cultivation was started where a 600 g/l glucose solution was fed to the
reactor (3.5 g/h in the start, 37.5 g/h after 20 h and until the end of the
ation). pH was controlled at pH 7 through the automatic addition of 25 %
NH4OH, air was supplemented (5 l/min), and the stirrer was set at 500 rpm.
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After 24 h of fed—batch cultivation the OD600 was 33.2. The cells in the
cultivation were pelleted by centrifugation at 15,900 g. The phage particles
were precipitated from the supernatant twice in PEG/NaCl, filtered and
dissolved in PBS and glycerol as in e 2. Phage stocks were stored at
-80 °C until use in selection.
Results
Library construction: The new library was designed based on a set of
16 FcRn binding Z variants with verified binding properties (Example 2-6).
The theoretical size of the ed library was 5.3 x 108 Z variants. The
actual size of the library, determined by titration after ormation to E. coli
ER2738 cells, was 4.5 x 109 transformants.
The library quality was tested by sequencing of 96 transformants and
by comparing their actual sequences with the theoretical design. The contents
of the actual library compared to the designed library were shown to be
satisfying. A maturated library of potential binders to FcRn was thus
successfully constructed.
e 8
Selection and screening of Z ts from a ted library
Materials and s
Phage display selection of matured FcRn binding Z variants: The target
proteins human FcRn (Biorbyt, cat. no. orb84388) and murine FcRn (Biorbyt,
cat. no. orb99076) were biotinylated essentially as described in Example 2
using biotin at 10x molar . Phage display selections, using the new
y of Z variant molecules bed in Example 7, were performed in four
cycles against human FcRn or murine FcRn essentially as in Example 2 but
with the following exceptions. Selection buffers were 0.1% PCTG buffer, pH
.5 (Mcllvaines ate-citrate buffer, pH 5.5, supplemented with 0.1 %
Tween-20 and 0.1% n) or 0.1% PCTG buffer, pH 7.4, (Mcllvaines
phosphate-citrate buffer, pH 7.4, supplemented with 0.1 % Tween-20 and
0.1% gelatin) respectively. Prior to selection, HSA was added to the selection
buffers to a final concentration of 1.5 uM. All tubes and beads used in the
selection were pre—blocked with either of the two different selections buffers.
A pre-selection step, by incubation of phage stock with SA—beads for 45 min,
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was performed in cycle 1. For capture of target complexes, 1 mg
beads per 1.1 pg biotinylated human FcRn or 1.6 pg biotinylated murine FcRn
was used. Washes were performed with 0.1% PCT buffer pH 5.5 or pH 7.4
except for tracks 22-1 and 22-2 where 0.1% PCT supplemented with 25
nM lgG (Herceptin®) or 10 nM lgG, respectively, was used as outlined in
Table 9.
The five tracks (1-5) in cycle 1 were divided in the second to fourth
cycles, ing in totally seven tracks (1-1 to 5-1) in cycle 2, eleven tracks
(1—1-1 to 51) in cycle 3 and en tracks -1 to 1) in cycle 4.
The bound phage particles were eluted as bed in Example 2.
An overview of the selection strategy, describing an increased
stringency in subsequent , using a lowered target concentration and an
increased number of washes, is shown in Table 9.
Amplification of phage particles: Amplification of phage particles
between selection cycle 1 and 2 was performed essentially as bed in
Example 2, with the following exceptions. E. coli ER2738 was used for phage
amplification and M13K07 helper phage was used in 5 x excess. The
amplification of phage particles between the selection cycles 2 and 4 was
done by ming infection of bacteria in solution as follows. After infection
of log phase E. coli ER2738 with phage particles, TSB supplemented with
2 % glucose, 10 ug/ml tetracycline and 100 ug/ml ampicillin was added,
followed by incubation with rotation for 30 min at 37 °C. Thereafter, the
bacteria were infected with M13K07 helper phage in 5 x excess. The infected
bacteria were pelleted by centrifugation, re—suspended in TSB-YE medium
supplemented with 100 uM IPTG, 25 pg/ml kanamycin and 100 ug/ml
ampicillin, and grown overnight at 30 °C. The overnight cultures were pelleted
in a centrifuge, and phage particles in the supernatant were precipitated twice
with PEG/NaCl buffer. Finally, the phage particles were re-suspended in
selection buffer before entering the next selection cycle.
In the final selection cycle, log phase bacteria were infected with eluate
and diluted before spreading onto TBAB plates (30 g/l tryptose blood agar
base, Oxoid cat. no. 0M0233B) supplemented with 0.2 g/l ampicillin in order
to form single colonies to be used in ELISA screening.
WO 2016042083
Table 9. Overview of the maturation selection data.
Cycle ion Phage stock Target Target Selection
from library or species conc. '0I
selection track
Zlib006FcRn.l human 100
Zlib006FcRn.l human 1 OO
Zlib006FcRn.l human 25
Zlib006FcRn.l murine 100
ZIibOO6FcRn.I murine 100
A human 5O
A human 5
[\3 human [\D
A human 5
90N human 5
are AA murine 50
murine 10
human 1 O
human 5
1}) _\. human 1
human 5 A
human 1 O A
H"[\J human 5 A
human 1
cl»NL human 0.5 A
Loo Li's Li's 9"N human 0.25 A
-Ib A murine 10
(91 A L '01I |_\ murine 5
AA II _\A—\ III I AA human 1 A
I human 0.25 A
N—\—\ II I human 0.5 A
I N—\—\ III AAAAAA II human 0.1 A
I human 1 .0"SJ‘NSJ‘NNWP‘SJ‘S"NWP‘WQNNP‘QP‘NNWNP‘NWV‘N oncn-nonAhmmmm-bmmmm-bhmmm-bhmhmhmmA A
iII I iII
human
O. 01
[>3 A I [)3 A I human 0.25 .“NNWNNNWNWWP‘NNNNQNWNWWWNNQNWNN A4:.ngmehmmmLALLmLmmemLLmngh .0" 01
i G)
'P A I'T’N 2—1-2 human 0.1 .0" O‘l
i G)
2—2—1-1 21 and 2—2—2 human 0.5
-4 2—2—2—1 2—2—1 and 2—2—2 human 0.5 “.01.“. Low—h 0"." 01-D- NA 001
W0 42083
Seguencing of potential binders: Individual clones from the different
selection tracks were picked for sequencing. All clones run in the ELISA
screening were sequenced. ication of gene fragments and sequence
analysis of gene fragments were med essentially as described in
Example 2.
ELISA screening of Z ts: Single colonies ning Z variants
(expressed as Z variant ABD fusion proteins as described in Example 2) were
randomly picked from the selected clones of the FcRn maturated library and
grown in 1 ml cultivations essentially as described in Example 2. Preparation
of the periplasmic supernatants was performed as in Example 2 with eight
freeze thawing cycles and the periplasmic fractions were used undiluted in
the ELISA ing. ELISA screenings were performed at both pH 6.0 and
pH 7.4 essentially as described in Example 2 using biotinylated human FcRn
at a concentration of 2 nM in each well. The periplasmic on of the
primary FcRn binder 210193 (SEQ ID NO:2; assayed in above experiments)
was used as a positive control. Periplasm containing the ABD moiety only
was used as a ve control.
ELISA KD analysis of FcRn binding Z variants: A selection of FcRn
binders was subjected to an analysis of the response against a dilution series
of biotinylated human FcRn using ELISA at both pH 6.0 and pH 7.4 as
described above. Biotinylated human FcRn was added at a concentration of
nM and diluted stepwise 1:3 down to 14 pM. As a ound control, all Z
variants were also assayed with no target protein added. Periplasm samples
containing the primary FcRn binder 207918 (SEQ |D.NO:1)was included and
analyzed as a positive control. Periplasm containing the ABD moiety only was
used as a negative control. Data were analyzed using GraphPad Prism 5 and
non-linear regression and KD values (the half maximal effective concentration)
were calculated.
Results
Phage display ion of maturated FcRn binding Z ts:
Selection was performed in totally 14 parallel tracks containing four cycles
each. The different selection tracks ed in target concentration, target
type (human FcRn or murine FcRn), selection time, and wash conditions.
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Sequencing of potential s: Randomly picked clones were
sequenced. Each individual Z variant was given an identification number,
Z#####, as described in e 2. In total, 445 new unique Z variant
molecules were identified.
The amino acid sequences of a subset of the 58 amino acid residues
long Z variants are listed in Figure 1 and in the sequence listing as SEQ ID
NO:17-352. The deduced FcRn binding motifs of these Z ts extend from
residue 8 to residue 36 in sequences with SEQ ID 352. The amino
acid sequences of the 49 amino acid es long polypeptides (BMod)
predicted to constitute the complete three-helix bundle within each of these Z
variants extend from residue 7 to residue 55.
ELISA screening of Z variants: Clones obtained after four selection
cycles were produced in 96-well plates and screened for FcRn binding activity
using ELISA. All randomly picked clones were analyzed. At pH 6.0, 333 of the
445 unique Z variants were found to give a response of 0.3 AU or higher
(corresponding to at least 3x the negative control) against human FcRn at a
concentration of 2 nM. At pH 7.4, 278 of the 445 unique Z variants were found
to give a response of 0.3 AU or higher (corresponding to at least 3x the
negative control) against human FcRn at a concentration of 2 nM. Clones with
a positive signal against human FcRn were found in all tracks (including those
with murine target) except 11-1. The negative ls had absorbances of
0.070-0.096 AU (pH 6.0) and 112 AU (pH 7.4), respectively. The
average response of the blank controls was 0.070 AU (pH 6.0) and 0.062 (pH
7.4).
ELISA KD analysis of FcRn binding Z variants: A subset of Z variants
was selected based on the result in the ELISA experiment described above
(highest ELISA value at pH 6.0 and/or pH 7.4) and subjected to a target
titration in ELISA format. Periplasm samples were incubated with a serial
dilution of biotinylated human FcRn. A periplasm sample with the primary
binder 207918 (SEQ ID NO:1) was also assayed as a ve control.
Obtained values were analyzed and their tive KD values were
calculated (Table 10).
Table 10: Calculated KD values from ELISA titration analysis of Z—ABD
variants from the maturation.
SEC! Kn Kn Kn
ID pFl&0 pFIZ4
vafiant
ch (M) (M) (M) (M)
213574 18 1.2 x 10‘9man——
213578 20 1-0x10'9
9.8x 10'10 3.6 x 10'9
213581 22 1.1x10'9 3.3 x 10'9 213695 84 1.8x 10'9 5.3 x 10'9
213583 23 8.0x10‘10 1.5x10'9 213697 85 1.2x 10‘9 2.4 x 10'9
213585 24 1.2x10'9 1.7x10'9 213706 2.0x 10'9 6.4 x 10'9
213586 25 1.2x10‘9 2.3x10‘9 213708 87 1.9x 10‘9 4.4 x 10'9
213587 26 '9 6.9x10'9 213710 88 1.6x 10'9 2.6 x 10'9
213588 27 1.0 X 10'9 2.3 X 10'9 213711 2.1 x 10'9 4.9 x 10'9
213592 28 9.5x10‘10 1.8x10'9 213714 2.1x10'9 6.0 x 10'9
213594 29 1.3x10'9 6.3x10'9 213716 91 1.8x10'9 5.8 x 10'9
213596 30 1.5x10‘9 3.6x10'9 213719 92 2.6x 10‘9 7.3 x 10'9
213597 31 1.4x10'9 6.0x10'9 213720 93 2.5x 10'9 4.5x 10'7
213598 32 ‘9 1.7x 10'9 213721 94 1.9x10‘9 2.9 x 10'9
213600 33 1.4x10'9 4.0x10'9 213725 95 1.8x10'9 4.9 x 10'9
213604 43 1.3 x 10‘9 4.1 x 10‘9 213727 ‘9 5.9 x 10-9
213605 35 1.3x10'9 3.8x10'9 213728 97 2.6x10'9 6.7 x 10'9
213609 36 1.3x10'9 2.7x10'9 213732 2.1x10'9 9.4 x 10'9
213611 37 ‘9 2.5x10'9 213735 1.6x10'9 9.1 x 10'9
213612 38 '9 8.6X10'9 213736 100 1.7x10'9 3.0 x 10'9
213613 39 1.2x10‘9 4.3x10'9 213740 101 2.0x10‘9 5.0 x 10'9
213615 40 1.2x10'9 3.1x10'9 213742 102 2.4x 10'9 7.6 x 10'9
213616 41 9.6x10‘10 1.7x10-9 213747 103 1.3x 10‘9 2.3 x 10'9
213617 42 1.2x10'9 1.9x10'9 213749 104 2.8x 10'9 1.2 x 10'8
213620 43 1.4x10'9 3.3x10'9 213750 105 2.7x 10'9 8.4 x 10'9
213621 44 8.6x10‘10 1.4x10'9 213751 106 2.0x10'9 3.8 x 10'9
213622 45 1.1x10'9 2.1x10'9 213752 107 '9 5.8 x 10'9
213624 46 1.3x10‘9 3.4x10'9 213758 108 1.9x10‘9 6.5x 10'9
213625 47 1.3x10'9 2.8x10'9 213759 109 2.1x10'9 5.6 x 10'9
213626 48 1.2x10‘9 2.7x10'9 213760 110 2.1x10‘9 5.8 x 10'9
213627 49 1.2x10'9 2.9x10'9 213761 111 '9 3.7 x 10'9
213628 50 1.3x10‘9 5.5x10‘9 213771 112 1.5x 10‘g 2.0 x 10‘9
213629 51 '9 8.5x10'9 213773 113 2.5x10'9 4.9 x 10'9
213633 52 1.5x10'9 6.2x10'9 213776 114 2.2x 10'9 5.5x 10'9
W0 2016;042083
SEQ KD
variant
NO: (M)
213637 55 1.3 x109
213639 57 1.3 x 10-9 2.3 x 10'9 4.7 x 10'9
120 2.0 W" 2.9 x10"’
213641 59 1.1x10‘9 121 2.3x 10-9 4.2x 10'9
213644 60 1.3 x 10-9 122 1.9 x 10'9 5.6 x 10'9
123 ‘9 3.1x10'9
213648 62 1.6 x 10'9 124 2.4 x 10'9 5.5 x 10'9
213651 63 1.2x 10'9 125 2.0x 10'9 3.1 x 10'9
213652 64 1.4x 10'9 126 2.3x10'9 1.1x10'8
127 2.9 x109 3.8 x10"’
213655 66 1.1x10‘9 128 1.9x 10-9 3.8x 10'9
213656 67 1.1 x 10'9 129 2.6x 10'9 5.4x 10'9
130 2.2 x109 4.1x10'9
213659 69 2.2 x 10'9 131 2.2 x 10'9 5.5 x 10'9
132 2.6 X109 42 x199
213664 71 2.4 x 10'9 133 2.3 x 10'9 4.3 x 10'9
134 2.1x10'9 3.1x10'9
213669 73 9.2 x 10-10 135 2.1 x 10'9 3.0 x 10'9
213672 74 2.5 x 10'9 136 2.3 x 10'9 8.7 x 10'9
137 2.5 X109 56 x10'9
213675 76 9.6 x 10'10 138 2.0 x 10'9 2.8 x 10'9
139 2.0 x10‘9 3.4 x10'9
213678 78 2.0x10'9 140 2.1 x 10'9 3.0x 10'9
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Example 9
tion and characterization of Z variants from a maturated library
In this Example, twelve 2 variants were produced in E. coli, purified
and assayed for stability, for binding to FcRn as well as for inhibition of lgG
g to FcRn.
als and methods
Subcloning of Z ts into expression vectors: The DNA of twelve
FcRn binding Z variants (213577 (SEQ ID NO:19), 213578 (SEQ ID NO:20),
213583 (SEQ ID NO:23), 213592 (SEQ ID NO:28), 213616 (SEQ ID NO:41),
213621 (SEQ ID NO:44), 213654 (SEQ ID NO:65), 213663 (SEQ ID NO:70),
213669 (SEQ ID NO:73), 213674 (SEQ ID , 213675 (SEQ ID NO:76)
and 213676 (SEQ ID ) was amplified from the library vector
pAY02592. The subcloning was performed as described in Example 3. The 2
gene fragments were subcloned into the expression vector pAY01448
resulting in the encoded ce MGSSHHHHHHLQ-[2#####]-VD.
Production of 2 variants: Cultivation and purification of the Hiss-tagged
2 variants were performed essentially as described in Example 3. In order to
obtain higher purity, a ed phase chromatography (RPC) step was
added after the IMAC purification of a second batch of the twelve matured
variants and the primary 2 variant 207918. Samples from this batch were
used where indicated.
CD analysis: In order to determine the melting temperatures (Tm) and
assess the secondary structure of the 2 variants (RPC purified batch), CD
analysis was carried out as described in Example 3.
Biacore binding and c analyses: The interaction of FcRn binding
Hise-tagged 2 variants with human FcRn was analyzed in a Biacore 2000
instrument essentially as described in Example 3. Human FcRn (hFcRn) or
lgus FcRn (chRn) purchased from t (cat. no. orb84388 and
orb99075, respectively) were used as target protein. In a first set of
experiments, 100 nM of the 2 variants was ed at pH 6.0 during 2 min at
ul/min over immobilized hFcRn followed by dissociation in buffers of pH
6.0 or pH 7.4 using the co-inject procedure. The dissociation phase was 4 min
and the equilibration time between the analyte injections was 30 min.
In a second set of experiments, approximate kinetic constants (kon and koff)
and affinities (KD) were determined for a subset of 2 ts injected at
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concentrations of 540 nM, 180 nM, 60 nM, 20 nM and 6.7 nM over
immobilized hFcRn. As above, the analytes were injected during 2 min at 30
pl/min, the dissociation phase was 4 min and the equilibration time between
the analyte injections was 30 min.
In a third set of experiments, a kinetic analysis of the twelve matured Z
ts and the primary Z variant 207918 (SEQ ID NO:1) (RPC ed
batches) binding to hFcRn and chRn was performed at pH 6. A
concentration series of Hiss-tagged Z variants (270, 90, 30 and 10 nM) were
injected during 4 min at 30 pl/min over hFcRn and chRn, immobilized in
different flow cells of a CM5 chip surface. 0.005 % PCT pH 6.0 was used as
g buffer and for dilutions of the agged Z variants. Dissociation in
running buffer was allowed for 20 min, followed by e regeneration by
injection of 3 x 30 second pulses of 0.005 % PCT pH 7.4 and equilibration ten
minutes before the start of next cycle.
AlphaLlSA blocking assay: The potential of Z variants to inhibit g
of lgG to FcRn was analyzed in the AlphaLlSA assay described in Example 3.
Results
Production of Z variants: The twelve FcRn binding Z variants
constructed with an N—terminal His6 tag were produced in E. coli. SDS—PAGE
analysis of each final n preparation showed that these predominantly
contained the FcRn binding Z variant. The correct identity and lar
weight of each FcRn binding Z variant was confirmed by HPLC-MS analysis.
CD analysis: Determined melting temperatures are shown in Table 11.
ible folding was seen for all FcRn binding Z variants when overlaying
spectra measured before and after heating to 90 °C.
Biacore binding and kinetic analyses: In a first set of experiments, the
g of the twelve Z variants to human FcRn and the dissociation at
different pH were tested in a Biacore instrument by sequentially injecting each
of the Z variants at pH 6.0 and either buffer pH 6.0 or buffer pH 7.4 over a
chip surface containing FcRn. The ligand immobilization level of the surface
was 890 RU human FcRn. The twelve Z variants showed binding to FcRn at
pH 6.0, and for all variants, faster off-rates were seen at pH 7.4 compared to
pH 6.0.
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The kinetic constants of the Z variants 213577 (SEQ ID NO:19) and
213621 (SEQ ID NO:44) interacting with FcRn at pH 6.0 were determined in a
second set of experiments (see Table 12). c constants were calculated
using curve sets of two or four injected concentrations of 213577 and
213621, respectively.
Table 11: Meltino temperatures for a set of matured FcRn bindino 2 variants.
Z variant SEQ ID NO:
213577 _\ O 03 _\
213578 [\J O 01V
213583 N03 m A
213592 NO) 01 00
213616 4:. _\ O)O
213621 44 49
213654 03 U1 01 00
213663 \lO 030
213669 ‘1 00 4s 01
213674 \l 01 010
213675 \I O? A00
213676 ‘1 ‘1 4s 01
207918 _\ 4s (0
Table 12. Biacore c constants and ties for FcRn binding at pH 6.0.
Zvariant SEQ ID NO: kon(M"s") km:f (s'1) KD (M)
213577 19 3.0 x105 4.0x10'3 13x10'9
213621 44 6.4 x105 3.7x10'3 6X10'9
In a third set of experiments, the kinetic constants of thirteen Hise—
tagged 2 ts interacting with human or cynomolgus FcRn at pH 6.0 were
determined (Table 13). The FcRn immobilization levels of the chip surfaces
were 1196 RU (human) and 788 RU (cynomolgus), respectively. For each 2
variant, c constants were calculated using a curve set of four injected
concentrations.
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Table 13. Biacore kinetic constants and affinities for human and cynomolgus
FcRn binding at pH 6.0.
hFcRn chRn
z variant ID kon (M'1s'1) koff (5") KD (M) kon (M'1s'1) koff (5'1) KD (M)
213577 19 7.2 x105 2.9 x10'3 4.1 x10'9 8.2 x105 4.4 x10'3 5.4 x10'9
213578 20 4.1x105 ‘3 1.8x10'8 5.6x105 1.1x10'2 2.1 x10'8
213583 23 4.5 x105 2.6 x10'3 5.8 x10'9 6.7 x105 4.4 x10'3 6.6 x10'9
213592 28 5.9x105 7.2x 10‘3 1.2x 10'8 7.5x105 '2 1.5x10'8
213616 41 2.9x105 3.1 x10'3 1.0x10'8 4.3x105 4.8x10'3 1.1x10'8
213521 44 4.1x105 2.8 x10‘3 6.8 x10'9 6.1 x105 4.6 x10'3 7.6 x10'9
213654 65 6.0x105 9.5x10'3 1.6x10'8 8.4x105 1.3x10'2 '8
213563 70 3.9 x105 3.4 x10‘3 8.7 x10'9 5.2 x105 5.3 x10'3 1.0 x10'8
213669 73 5.6 x105 2.8 x10'3 4.9 x10'9 8.2 x105 4.6 x10'3 5.6 x10'9
213574 75 5.3 x105 3.7 x10‘3 7.0 x10'9 8.3 x105 5.9 x10'3 7.1 x10'9
213675 76 4.9x105 5.1 x10'3 1.0x10'8 7.5x105 8.0x10‘3 1.1x10'8
213576 77 6.5 x105 3.6 x10‘3 5.5 x10'9 9.6 x105 5.9 x10'3 6.2 x10'9
207918 1 2.6x105 4.2x10'3 1.6x10'8 3.8x105 7.0x10‘3 1.9x10'8
Table 14: Calculated IC50 values from AlphaLlSA no assa .
Z variant SEQ ID NO:
213577
213578
213583
213592 [\JNNA OOOOOCQ
213616
213621
213654
213663 \IO-D- 001-5
213669 ‘1 00
213674 \l 01
213675 \l 03
213676 \l ‘1
AlghaLlSA blocking analysis: The ability of twelve maturated Hisstagged
monomeric Z ts to inhibit lgG binding to FcRn was tested in an
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AlphaLlSA blocking assay. Serial dilutions of the Z variants were incubated
with biotinylated human FcRn and the blocking ability of each respective
variant was measured after on of lgG coated Acceptor beads and
subsequently avidin coated Donor beads. Inhibition could be measured
as a decrease in AlphaLlSA counts for positive Z variants. All twelve tested Z
variants were shown to block lgG binding to FcRn and the calculated IC50
values are shown in Table 14.
Example 10
Comparison of blocking capacity of lgG binding to FcRn
In this Example, the lgG blocking capacity of the FcRn g Z
variant O7918 (SEQ ID NO:1) was compared to Intravenous
immunoglobulin (Mg) and Subcutaneous globulin (SClg) currently
used in the treatment of some autoimmune disorders.
Materials and methods
Blocking of lgG-FcRn immunofluorescence staining: Human or murine
FcRn-eGFP transduced HeLa cells were prepared as described in Example
4. Fixed cells were resuspended in 50 pl of a mix of 50 nM Alexa Fluor® 647-
ated human lgG (Jackson laboratories, cat. no. 009-600—003) and Hise—
tagged 207918, lVlg (Octagam®, Octapharma) or SClg (Gammanorm®,
arma), respectively, diluted at concentrations of 1000, 100, 10, 1, 0.1
or 0 (buffer control) nM in Mcllvanes buffer pH 6.0, containing 2.5 % FBS
Ultra low lgG (Life Technologies) and 0.1 % n (AppliChem). The cells
were incubated for 1 h at 37 °C in the dark, washed with 2 x 100 pl Mcllvanes,
pH 6.0, containing 2.5 % FBS Ultra low lgG and re-suspended in 180 pl of
Mcllvanes, pH 6.0, containing 1 % BSA. Data from 10,000 GFP/FcRn positive
cells were obtained using a FACS Calibur (Beckman Coulter) and the data
was analyzed using Flowing software 2.5.0 (Turku University).
Results
The experiment was performed to determine if the FcRn binding Z
variant Hiss-ZO7918 (SEQ ID NO:1) blocks the lgG-FcRn interaction and
compare the blocking effect to Mg and SClg. Human or murine FcRn-eGFP
transduced HeLa cells were incubated with human Alexa Fluor® 647-
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conjugated lgG. The binding was d with unlabeled Hise-Z07918, lVlg or
SClg at different trations. The results showed that Hise-ZO7918
effectively blocked hlgG binding to hFcRn to a similar extent as |V|g or SClg
(Figure 9).
Example 11
Increased lgG catabolism by FcRn binding Z variants in mice
The ability of the FcRn binding Z variant ZO7918 to block lgG binding
to FcRn in vitro was shown in Example 10. In this example, the blocking
ability of the same Z variant was evaluated in vivo. Blocking of lgG-FcRn
interactions in vivo will lead to increased lgG catabolism and concomitant
d levels of lgG (Mezo 2008, supra).
Materials and methods
Animal study: The FcRn-binding Z variants Z11948 (SEQ ID NO:354)
and ZO7918-PP013 8 (SEQ ID NO:1) identical to Z11948 but with the
N-terminus ng with the amino acids VD instead of AE, in fusion with the
ABD variant PPO13 (SEQ ID NO:377)) or vehicle (PBS buffer), were
administered to male NMRI (Charles , at a dose of 16.3 umol/kg. The
mice were treated with five intravenous injections given at 0, 24, 48, 72 and
96 h. Serum samples were taken at 0, 72, 120 and 168 h (termination of
study) and stored at -20 °C. The concentration of mouse lgG in serum was
quantified by ELISA.
Mouse lgG ELISA: The concentration of mouse lgG in mouse serum
s was analyzed by a mouse lgG ELISA kit (Mabtech 3825-1AD-6) and
performed as described by the manufacturer. The concentration of mlgG was
calculated from a standard curve provided and GraphPad Prism 5 using a
non-linear regression formula. The concentration of lgG in individual mice at
24, 72, 120 and 168 h were related to the level at 0 h and the results are
therefore presented as percentage of lgG (O h).
Results
The results showed a reduction of mouse lgG concentration in mice
treated with pecific Z variants. Both Z11948 and the ABD-fused variant
Z07918-PP013 lowered the concentration of endogenous lgG in mice in vivo.
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Most pronounced effects were obtained with the ABD-fused t and after
120 hours. Thus, the results indicates that the FcRn-specific Z variants
blocked recycling of lgG resulting in increased lgG catabolism and
uent lower levels of lgG in mice.
e 12
In vitro transcytosis of FcRn binding 2 ts
In this Example, the FcRn binding Z ts are tested for their y
to be orted through epithelial or endothelial cells or recycled by FcRn in
vitro. A drug containing a Z variant with the power of transcytosis will facilitate
drug uptake after for example oral or pulmonary administration.
Materials and methods
Cells, for example T84, MDCK, HeLa, CaCoZ, CaLu-1 and/or CaLu-3
cells, with or without endogenous or recombinant expression of FcRn, are
grown in respective growth medium on a membrane in a transwell to form a
monolayer. The integrity of monolayers can be evaluated by measuring the
electrical resistance or adding a probe that is not able to penetrate or being
actively transported over the cell monolayer. A defined monolayer of cells is
pulsed from the apical or basolateral side with ligand such as FcRn binding Z
variants, HSA or lgG in a buffer such as HBSS ’ Balanced Salt
Solution, SigmaAldrich, cat. no. H9269) or growth medium at a suitable pH
and temperature, and chased with buffers such as HBSS or growth medium
at a suitable pH and temperature on the opposite side.
In a variant of this assay, ligands can be chased with buffers such as
HBSS or growth medium at suitable pH and temperature on the same side as
administration to measure recycled ligand as well. This can be done in a
transwell or in a cell culture dish. Cells are seeded into transwell or cell
culture dishes and pulsed with ligands such as FcRn binding Z ts, HSA
or lgG. Endocytosed ligands will bind to FcRn and return to the cell surface at
the same or opposite side as they were loaded. After pulsing, free ligands are
removed by g the cells with cold buffer. To chase ligands, warm buffer
or medium is added to the cells and, after a period in the range from 10
minutes to several hours, the buffer or medium is removed and assayed for
the presence of ligands.
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In a variant of this assay, ligands such as FcRn binding Z variants,
HSA or lgG can be used to block the binding to FcRn by ligands such as
other FcRn binding Z variants, HSA or IgG by administering them at the same
time or sequentially to the cells.
The amount of ligand can be quantified by methods such as ELISA,
HPLC-MS, fluorescent dye or radio labeling.
The results of the experiment described above are ed to show
that the FcRn-specific 2 variants can be transcytosed and/or recycled in vitro.
Example 13
Binding of homodimeric FcRn binding polypeptides to human FcRn/eGFP
transfected HeLa cells
In this Example, the g y of homodimeric FcRn g
polypeptides was investigated and compared to the binding ability of
monomeric primary and maturated Z variants. The production of HeLa cells
expressing human FcRn-eGFP gene transgene was performed as described
in e 4 and the use of these cells for flow try analysis with Alexa
Fluor® 647 d Z variants is described.
Materials and methods
Alexa Fluor® 647 labeling of FcRn binding polypeptides: The two
homodimeric Hise-tagged ptides 211948-(G4S)3—211948 (SEQ ID
NO:369) and Z11948—(G4S)-211948 (SEQ ID NO:368), the primary
monomeric Hise-tagged Z t 207918 (SEQ ID NO:1) and the maturated
monomeric Hise-tagged Z-variants 213583 (SEQ ID NO:23), 213621 (SEQ ID
NO:44), 213654 (SEQ ID NO:65) and 213674 (SEQ ID NO:75) were labeled
with Alexa Fluor® 647 Carboxylic Acid Succinimidyl Ester (Invitrogen cat. no.
A20106). Before labeling, the pH in the sample suspensions (in PBS pH 7.4)
was adjusted to 8.3 by addition of 10 ul of 0.1 M sodium bicarbonate buffer,
pH 8.3, to 90 ul sample suspension. 10 pl of Alexa Fluor® 647 Succinimidyl
Ester dye (10 mg/ml in DMSO corresponding to 4 x molar excess) was added
to 100 pl of each sample suspension. The mixes were incubated at RT in the
dark for 1 h in a wiggling rota mixer. The reaction mixes were ately
transferred to dialysis cassettes (3500 MWCO) (Thermo Scientific cat. no.
66333) and free dye was removed by dialysis in PBS pH 7.4.
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Immunofluorescence staining of human FcRn-eGFP transfected HeLa-
cells with FcRn g polypeptides: hFcRn-eGFP HeLa cells were
harvested by trypsination and washed twice in Mcllvanes buffer, pH 6.0
before counting. 100,000 cells were pipetted per well of a v-bottomed 96 well
plate (Nunc, cat no 277143) and the cells in the plate were subsequently
pelleted at 1,700 rpm for 4 min at 4 °C. The atants were d and
the cells were fixed with 50 ul of 2 % formaldehyde (Sigma h, cat. no.
F8775) in Mcllvanes buffer for 10 min at RT. Cells were thereafter washed
with 2 X 100 pl Mcllvanes buffer, pH 6.0, containing 2.5 % FBS Ultra low lgG
(Life Technologies), and resuspended in nes buffer, pH 6.0, containing
2.5 % FBS Ultra low lgG and 0.1 % saponin (AppliChem, cat no A4518.0100)
ning 640 nM of Alexa Fluor® 647 labeled Hise-tagged polypeptides;
Z11948-(G4S)3-211948 and 211948-(G4S)—211948 and 207918. uced
HeLa cells, incubated with buffer alone, were used as control. The cells were
incubated for 1 h at 8 °C on a shaker in the dark. The cells were then
ted to two different washing conditions; 2 x 150 pl Mcllvanes buffer, pH
6.0, containing 2.5 % FBS ultra low lgG or 2 X 150 pl PBS, pH 7.4, containing
2.5 % FBS Ultra low lgG and a 20 min incubation step in PBS, pH 7.4,
ning 2.5 % FBS Ultra low lgG. After washing, all samples were re-
ded in 180 pl of Mcllvanes, pH 6.0, containing 2.5 % FBS Ultra low
lgG. Data from 10,000 GFP/FcRn positive cells were obtained using a FACS
Calibur (Beckman Coulter) and the data was analyzed using Flowing software
2.5.0 (Turku sity).
Results
Flow cytometry analysis was utilized to determine whether FcRn
binding dimers could bind to human FcRn on human FcRn/eGFP transduced
HeLa cells and to compare their binding ability to the monomeric FcRn
binding Z variants. The analysis was also performed to determine if the pH
dependent detachment from the FcRn protein was affected by the dimeric
format. The experiment was performed at pH 6.0 with washings at pH 6.0 or
pH 7.4 with Alexa Fluor® 647 labeled dimers 211948-(G4S)3-211948 and
211948-(G4S)—211948, and monomers 207918, 213583, 213621, 213654
and 213674. 211948 and 207918 are identical in sequence apart from the
first two amino acid residues (AE vs VD). The calculated MFI values are
presented in Figure 11. The results show that the dimeric format increases
the binding capacity of the FcRn g polypeptides compared to the
corresponding monomer (Figure 11A) and that the maturated Z variants
(213583, 213621, 213654 and 213674) have a higher binding capacity than
the primary 2 variant 207918 (Figure 11B). The data shows that the pH
dependent detachment from FcRn decreases with the use of the dimeric
format, suggesting that FcRn binding dimers may have an improved pH
dependent binding profile compared to corresponding monomeric variants.
Example 14
Comparison of blocking capacity of IgG binding to FcRn
In this Example, the IgG blocking ty of the FcRn binding dimers
Z11948-(G4S)3-211948 and Z11948-(G4S)—211948 was compared to that of
monomeric FcRn binding 2 variants, as well as to intravenous
immunoglobulin (Mg) and subcutaneous immunoglobulin (SCIg) currently
used in the ent of some mune disorders.
Materials and methods
Blocking of IgG-FcRn immunofluorescence staining: Human FcRn-
eGFP transduced HeLa cells were prepared as bed in Example 4.
Fixed cells were ended in 50 ul of a mix of 50 nM Alexa Fluor® 647-
conjugated human lgG (Jackson tories, cat. no. 009—600-003) and His;-
tagged 211948-(G4S)3-211948 (SEQ ID NO:369), 211948-(G4S)—211948
(SEQ ID NO:368), 207918 (SEQ ID NO:1), 213583 (SEQ ID NO:23), 213621
(SEQ ID NO:44); IVIg (Octagam®, Octapharma) or SCIg (Gammanorm®,
Octapharma), respectively, diluted at trations of 1000, 100, 10, 1, 0.1
or 0 (buffer control) nM in Mcllvanes buffer, pH 6.0, containing 2.5 % FBS
Ultra low IgG (Life Technologies) and 0.1 % saponin (AppliChem). The cells
were incubated for 1 h at 37 °C in the dark, washed with 2 x 100 pl Mcllvanes
, pH 6.0, containing 2.5 % FBS Ultra low lgG and re-suspended in 180
pl of nes buffer, pH 6.0, containing 1 % BSA. Data from 10,000
GFP/FcRn positive cells was obtained using a FACS Calibur (Beckman
Coulter) and analyzed using Flowing software 2.5.0 (Turku University).
Results
The experiment was performed to determine if the FcRn binding
dimers 211948-(G4S)3-211948 and 211948-(G4S)-211948 block the IgG—
FcRn interaction, and e the blocking effect to that of the monomeric
FcRn binding Z variants 207918, 213583 and 213621, as well as Mg and
SCIg. Human FcRn-eGFP transduced HeLa cells were incubated with human
Alexa Fluor® 647 ated lgG. The binding was blocked with unlabeled Z
variants, IVIg or SCIg at different trations. The results showed that the
FcRn binding dimers have an ed blocking effect in terms of hIgG
g to hFcRn compared to the monomeric Z variant 207918, Mg and
SCIg (Figure 12A). Furthermore, the blocking capacity of maturated
monomeric 2 ts 213583 and 213621 was improved compared to the
ng capacity of the primary monomeric 2 variant 207918 (Figure 12B).
The calculated IC50 values of the blocking assay are summarized in Table
15.
Table 15: Calculated IC50 values from HeLa cell IoG blockino assa .
Designation SEQ ID NO:
— G4S 3—211948 369
21 1948-(G4S)—Z11948 368
213583 23
Z13621 44
207918
IVIo n.a.
SCI.
Example 15
Production ofdimeric FcRn binding polypeptides
Materials and methods
The 2 variants 217303 (SEQ ID NO:357), 218632 (SEQ ID NO:365),
218633 (SEQ ID NO:366) and 218634 (SEQ ID NO:367) were constructed as
dimers in fusion with the albumin binding variant PP013 (SEQ ID NO:377) in
the general format [2#####]—ASGS-PP013-GT-(G4S)—[2#####]. The resulting
polypeptides were denoted 2AZ3824 (SEQ ID NO:373), 2AZ3869 (SEQ ID
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NO:374), ZAZ3870 (SEQ ID NO:375) and ZAZ3871 (SEQ ID NO:376),
respectively. Dimeric polypeptides of the Z variant 217303 in fusion with
PP013 was also constructed with different linkers or C-terminal fusion of
PP013, resulting in the polypeptides Z17303-GAP(G4S)3TS-PP013-
GT(G4S)3PR-Z17303 and Z17303-GAP(G4S)3TS-Z17303-GT(G4S)3PR-
PP013, denoted ZAZ3715 (SEQ ID NO:371) and ZZA3716 (SEQ ID ),
respectively. Furthermore, 217303 was constructed as a dimer without
PP013, but with an N—terminal Hise-tag resulting in the polypeptide GSS-Hise-
LQ-Z17303-GT(G4S)3-Z17303, denoted 223556 (SEQ ID NO:370).
Cultivation was performed as described in e 3. Purification of
PP013 containing polypeptides was carried out by anti-ABD affinity
chromatography and RPC as bed in Example 6, s cation of
Hiss-tagged 223556 was performed by IMAC as described in Example 3.
Results
The seven FcRn binding dimeric polypeptides, constructed either with
a Hiss-tag or an ABD moiety, were produced in E. coli. The amount of affinity
purified protein, determined spectrophotometrically by measuring the
absorbance at 280 nm, ranged from 2-18 mg per g bacterial pellet. SDS-
PAGE analysis of each final protein preparation showed that these
predominantly contained the FcRn binding polypeptide. The correct ty
and molecular weight of each FcRn binding polypeptide was confirmed by
HPLC-MS analysis.
Example 16
Binding of homo- and/or heterodimeric FcRn binding ptides to human
FcRn/eGFP transfected HeLa cells
In this Example, the binding ability of homo- and/or heterodimeric FcRn
g polypeptides comprising ted Z ts is investigated. HeLa
cells sing human FcRn—eGFP gene transgene, produced as described
in Example 4, are used for flow cytometry analysis with Alexa Fluor® 647
labeled Z variants.
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Materials and methods
Alexa Fluor® 647 labeling of FcRn binding Z variants: Homo- and/or
heterodimeric FcRn binding polypeptides are labeled with Alexa Fluor® 647
Carboxylic Acid imidyl Ester (Invitrogen cat. no. A20106) as described
in Example 13.
Immunofluorescence staining of human FcRn-eGFP transfected HeLa-
cells with FcRn binding polypeptides: hFcRn-eGFP HeLa cells are harvested
by trypsination and washed twice in Mcllvanes buffer, pH 6.0, before
counting. 100,000 cells are pipetted per well of a v-bottomed 96 well plate
(Nunc, cat no 277143) and the cells in the plate are subsequently pelleted at
1,700 rpm for 4 min at 4 °C. The supernatants are removed and the cells are
fixed with 50 pl of 2 % formaldehyde (Sigma Aldrich, cat. no. F8775) in
Mcllvanes buffer for 10 min at RT. Cells are thereafter washed with 2 x 100 pl
Mcllvanes buffer, pH 6.0, containing 2.5 % FBS Ultra low lgG (Life
Technologies), and resuspended in Mcllvanes buffer, pH 6.0, containing 2.5
% FBS Ultra low IgG and 0.1 % saponin (AppliChem, cat no A4518.0100)
containing 640 nM of Alexa Fluor® 647 labeled Hise-tagged homo- and/or
heterodimeric FcRn binding polypeptides and a corresponding monomeric Z
variant.
Examples of formats for homo— and/or dimers include Z#####-
(G4S)3-Z##### and Z#####-(G4S)-Z#####, where Z#### for example is
selected from Z13583 (SEQ ID NO:23), Z13621 (SEQ ID , 213654
(SEQ ID NO:65) or Z13674 (SEQ ID NO:75), or the same Z variants ng
with amino acid residues AE d of VD, as for example in Z17303 (SEQ
ID NO:357), which is identical to 213621 (SEQ ID NO:44) apart from the N-
al AE. Cloning may optionally be performed with a C-terminal Hise tag
as described in Example 3 or with an N-terminal Hise tag as in SEQ ID
NO:362.
uced HeLa cells, incubated with buffer alone, are used as
control. The cells are incubated for 1 h at 8 °C on a shaker in the dark. The
cells are then subjected to two ent washing conditions; 2 x 150 pl
Mcllvanes buffer, pH 6.0, ning 2.5 % FBS Ultra low IgG or 2 x 150 pl
PBS, pH 7.4, containing 2.5 % FBS Ultra low IgG and a 20 min incubation
step in PBS, pH 7.4, containing 2.5 % FBS Ultra low lgG. After washing, all
samples are pended in 180 pl of Mcllvanes, pH 6.0, containing 2.5 %
FBS Ultra low lgG. Data from 10,000 Rn positive cells are obtained
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using a FACS Calibur (Beckman Coulter) and the data is analyzed using
g software 2.5.0 (Turku University).
Results
Flow cytometry analysis is used to determine whether the homo-
and/or dimeric FcRn binding polypeptides comprising maturated Z
variants can bind to human FcRn on human FcRn/eGFP transduced HeLa
cells and compare the binding ability to the ric FcRn binding Z
variants or dimeric variants comprising primary Z variants. The analysis is
also performed to determine if the pH dependent detachment from the FcRn
protein is affected by the dimeric format. The experiments are performed at
pH 6.0 with washings at pH 6.0 or pH 7.4 with Alexa Fluor® 647 labeled FcRn
binding Z variants. The results from the experiment are expected to show that
homo- and/or dimeric formats, as well as the inclusion of maturated Z
variants with an improved affinity for FcRn, increase the binding capacity of
the FcRn binding polypeptides and that the pH dependent detachment from
FcRn is sed for said polypeptides.
Example 17
pH dependent binding ofdimeric polypeptides to human FcRn
In this Example, the capacity ofdimeric polypetides to bind FcRn at
different pH values was investigated by ELISA and compared to the g
capacity of a monomeric Z variant.
Materials and methods
The capacity of the dimeric polypeptides ZA23824 (SEQ ID NO:373),
ZA23869 (SEQ ID ), ZAZ3870 (SEQ ID NO:375) and ZAZ3871 (SEQ
ID NO:376), as well as the ric Z variant 213621 (SEQ ID NO:44), to
bind human FcRn at different pH values was tested in an ELISA where all
binding and washing steps were med at either pH 6.0 or pH 7.4. Half-
area 96-well ELISA plates were coated at 4 °C overnight with 4 ug/ml of
hFcRn (Biorbyt, cat. no. orb84388) d in PBS. The plates were washed
twice in tap water and the wells were blocked with 100 pl of PBSC (PBS, pH
7.4, mented with 1 % casein) for 1.5 h at RT. The blocking solution was
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poured off and the wells subjected to pH 6.0 treatment were washed once
with Mcllvaines phosphate-citrate buffer, pH 6.0. The different FcRn binding
polypeptides were added at a concentration of 100 nM and diluted stepwise
1:10 down to 0.1 pM in either PCC (Mcllvaines phosphate—citrate buffer, pH
6.0, supplemented with 1% casein) or PBSC. 50 pl of the dilutions were
transferred per well and the ELISA plates were incubated for 1.5 h at RT. The
plates were washed four times in either PCT (Mcllvaines phosphate-citrate
buffer, pH 6.0, supplemented with 0.05 % Tween-20) or PBST (PBS, pH 7.4,
mented with 0.05 % Tween-20). Bound polypeptides were detected
with 50 ul/well of a Z specific mouse antibody ced in-house) diluted to 2
ug/ml in either PCC or PBSC. The plates were subsequently incubated for 1.5
h at RT ed by washing as described above. HRP-conjugated goat anti-
mouse lg obtained from DAKO (P0447), diluted 1:5000 in either PCC or
PBSC, was added and the plates were incubated at RT for 1 h. After washing
(as above), 50 pl of ImmunoPure TMB substrate was added to each well and
the plates were developed according to the manufacturer’s recommendations.
After 30 min of development, the ance was measured at 450 nm using
a multi-well plate reader (Victor3) and the EC50 values were calculated using
GraphPad Prism 5.
Results
The analysis was performed to compare the binding potential of
ric versus dimeric format at different pH, but also to determine
r introduced scaffold mutations (Y5F, N528 and D53E; see further in
Examples 24 and 25) would affect the pH dependent g to FcRn. The
experiment was performed in an ELISA format at pH 6.0 or pH 7.4. The
results showed that the dimeric format was or to the monomeric format
in binding FcRn regardless of pH (up to 10x and 85x improvement at pH 6.0
and pH 7.4, respectively). The most potent binding, both at pH 6.0 and pH
7.4, was seen for the dimeric polypeptide ZAZ3824, which also showed a
similar binding capacity (EC50 value) at pH 6.0 and pH 7.4. The ELISA
titration curves are shown in Figure 13, and the calculated EC50 values are
summarized in Table 16.
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Table 16. Calculated E050 values from binding analysis at pH 6.0 and pH 7.4
EC50 (M)
DeSIgnation. . SEQ ID NO:
pH 6.0 pH 7.4
Z13621 44 9.9 x10'10 7.7 x10'9
ZAZ3824 373 9.9 x 10'11 9.1 x 10'11
ZAZ3869 375 3.0 x 10'10 7.3 x 10-10
ZAZ3870 375 2.6 x 10'10 5.7 x 10‘10
ZAZ3871 376 1.4 x 10'10 1.8 x 10‘10
Example 18
Comparison of ng capacity of lgG binding to FcRn
In this e, the potential of ptides to inhibit binding of IgG to
FcRn was analyzed using two different in vitro methods: AlphaLlSA and a cell
based assay.
Materials and methods
lSA blocking assay: The capacity of the dimeric FcRn binding
polypeptides ZZ3556 (SEQ ID NO:370), 5 (SEQ ID NO:371) and
ZZA3716 (SEQ ID NO:372) as well as the ric Z13621 (SEQ ID
NO:44) to block lgG-FcRn interaction was ed using an AlphaLlSA
assay. Human lgG (Roactemra) was immobilized on AlphaLlSA acceptor
beads (Perkin Elmer, cat. no. 6772002) according to the manufacurer’s
recommendations. Human FcRn (Biorbyt, cat. no. orb84388) was biotinylated
essentially as described in Example 2. Polypeptides were serially diluted 1:3
in AlphaLlSA buffer (Perkin Elmer, cat. no. AL000F) pH 6.0 (adjusted using
HCI) to final concentrations of 250 nM to 13 pM in a 384—well plate (Perkin
Elmer, cat. no. G6005350) and incubated for 45 min with 10 nM biotinylated
hFcRn. lgG-coated acceptor beads were added to a final concentration of 10
pg/ml and incubated for 45 min. Finally, streptavidin coated donor beads
(Perkin Elmer, cat. no. 6760002) were added to a final tration of 40
ug/ml and incubated for 30 min. All incubations were performed at RT in the
dark. The plate was analyzed in the EnSpire multiplate reader 2300 (Perkin
Elmer) and the |C50 values were calculated using GraphPad Prism 5.
HeLa cell IgG-FcRn blocking assay: Human FcRn-eGFP transduced
HeLa cells were prepared as described in Example 4. The polypeptides
223556 (SEQ ID ), 2A23715 (SEQ ID NO:371), 22A3716 (SEQ ID
), ZAZ3824 (SEQ ID NO:373), 2A23869 (SEQ ID NO:374), 2A23870
(SEQ ID NO:375), 2A23871 (SEQ ID NO:376), 213621 (SEQ ID NO:44),
218632 (SEQ ID NO:365), 218633 (SEQ ID NO:366) and 218634 (SEQ ID
NO:367), as well as IVlg (Octagam®, Octapharma) or SClg (Gammanorm®,
Octapharma), were each diluted to concentrations of 1000, 100, 10, 1, 0.1 or
0 (buffer control) nM in Mcllvanes buffer, pH 6.0, containing 2.5 % FBS Ultra
low IgG (Life Technologies) and 0.1 % saponin (AppliChem) and 50 nM Alexa
Fluor® 647-conjugated human IgG (Jackson laboratories, cat. no. 009
003). Fixed cells were resuspended in 100 pl of the mixture and were
incubated for 1 h at 37 °C in the dark. Cells were washed and resuspended in
Mcllvanes buffer, pH 6.0, containing 2.5 % FBS Ultra low IgG. Data from
10,000 GFP/FcRn positive cells was obtained using a FACS Calibur
(Beckman Coulter), analyzed using Flowing re 2.5.0 (Turku University)
and IC50 values were calculated using GraphPad Prism 5.
Results
ISA: The y of one monomeric and three dimeric
polypeptides to inhibit IgG binding to FcRn was tested in an AlphaLISA
blocking assay. The s show that the dimeric polypeptides had better IgG
blocking capacity compared to the monomeric format. The two ABD fused
dimeric ptides, 2A23715 and 22A3716, had IC50 values very similar to
that of , which does not contain an ABD . The calculated IC50
values of the AlphaLISA blocking assay are summarized in Table 17.
HeLa cell IgG blocking assay: Human FcRn-eGFP transduced HeLa
cells were incubated with human Alexa Fluor 647-conjugated IgG and
selected polypeptides to assess the ability of the polypeptides to block IgG-
FcRn interactions. Intravenous immunoglobulin (Mg) and aneous
immunoglobulin (Sclg) currently used in the treatment of some autoimmune
disorders, were also included in the test. The experiment was performed at
pH 6.0. The results showed that the dimeric format had an ed IgG
blocking capacity compared to the monomeric format. 2A23715 (longer
linkers) was compared to ZAZ3824 (shorter linkers), and the two constructs
showed similar IC50 values. There was also no difference between IC50
values ed for 2A23715 and 22A3716, i.e. dimer constructs with ABD at
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different positions. All tested ptides had superior lgG blocking effect
compared to Mg and SCIg. The ated |C50 values of the cell blocking
assay are summarized in Table 18.
Table 17: Calculated |C50 values showing lgG blocking capacity of
polypeptides in lSA.
Designation ‘ SEQ ID NO: |C50 (M)
213621 ‘ 44 1.0 x10'9
223556 370 1.9 x 10'10
2A23715 371 1.7 x10'10
22A3716 ‘ 372 1.8 x 10'10
Table 18. Calculated |C50 values showing lgG blocking capacity of
polypeptides in a HeLa cell based assay at pH 6.0.
Designation SEQ ID NO: |C50 (M)
213621 44 2.2 x10'8
218632 365 8.4 x 10'8
218633 366 5.7 x 10'8
218634 367 3.6 x 10'8
223556 370 1.9 x 10'9
2A23715 371 3.6 x 10'9
22A3716 372 3.5 x 10'9
ZAZ3824 373 3.8 x 10'9
2A23869 374 4.7 x 10'9
2A23870 375 5.3 x 10'9
2A23871 376 4.1 x 10'9
SClg - 1.2 x 10'7
Mg - 1.5 x 10'7
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Example 19
Comparison of blocking ty of IgG recycling
In this Example, the effect of homo- and/or heterodimeric FcRn g
polypeptides on lgG ing are investigated in FcRn transduced MDCK.2
cells.
Materials and methods
Lentiviral transduction of MDCK.2 cells: The vector pairs 2k7neo-CMV-
hB2M and pHR—cPPT-CMV-hFcRn-eGFP are nsfected together with
VSV-G pe and gag/pol packaging plasmid into HEK293T cells using
calcium chloride transfection (Zufferey et al., supra; son etal. (2006)
supra). HEK293T culture supernatants containing formed lentiviral particles
with FcRn and 82M transgenes respectively are used to sequentially
transduce MDCK.2 cells (ATCC cat. no. CRL—2936) at low passage number.
The resulting stably transduced MDCK.2 cell lines are denoted hFcRn-eGFP
(transduced with genes for human FcRn-eGFP and hB2M).
ng capacity of lgG recycling: Human GFP transduced
MDCK.2 cells are plated at 25 000 cells/well in a 96—well plate and incubated
overnight at 37 °C, 5 % C02. The cells are incubated with homo— and/or
heterodimeric FcRn binding polypeptides at concentrations ranging from 200
to 0.01 nM in Mcllvanes buffer, pH 6.0, containing 2.5 % FBS Ultra low lgG
before addition of 500 ng/ml Alexa Fluor® 647-conjugated human lgG
(Jackson laboratories, cat. no. 009003) and incubation for one additional
hour. The cells are washed Mcllvanes buffer, pH 6.0, ning 2.5 % FBS
Ultra low lgG and then incubated in PBS, pH 7.4, containing 2.5 % FBS Ultra
low lgG for 2 h in 37 °C, 5 % C02. The supernatants are then analyzed for the
presence of the Alexa Fluor® 647-conjugated human lgG in an EnSpire
multiplate reader (Perkin Elmer). The inhibition curves are analyzed by non-
linear regression using the GraphPad Prism 5 software to determine the |C50
values.
Results
The results from the experiment are expected to show a dose
dependent reduction in lgG recycling through the action of dimeric FcRn
binding polypeptides.
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Example 20
Increased lgG catabolism by dimeric FcRn binding polypeptides in FcRn
transgenic mice
In this Example, the effect of homodimeric FcRn binding polypeptides
on lgG catabolism was investigated in human FcRn transgenic mice on two
different occasions.
Materials and methods
Animal studies: In the first study, homodimeric FcRn-binding
polypeptide ZAZ3715 (SEQ ID NO:371) or ZZA3716 (SEQ ID NO:372), or
vehicle (PBS buffer), was administered at 0 hours by iv ion to male
BS.Cg-chrttm1Dcr Tg(FCGRT)32Dcr/Dch mice (Jackson Laboratory, stock
no. 14565) at a dose of 6 mg/kg. 24 hours prior to polypeptide administration,
500 mg/kg hlgG (Kiovig, Baxter) was administered by iv injection. Serum
samples were collected at -168, 0, 24, 72, 120 and 144 h (termination of
study) and stored at -20 °C.
In the second study, homodimeric inding polypeptide ZAZ3869
(SEQ ID NO:374), ZAZ3870 (SEQ ID NO:375) or ZAZ3871 (SEQ ID NO:376),
or vehicle (PBS buffer), was stered at 0 hours by i.v. injection to male
B6.Cg-chrttm1Dcr RT)32Dcr/Dch mice (Jackson Laboratory, stock
no. 14565) at a dose of 6 mg/kg. 24 hours prior to ptide administration,
500 mg/kg hlgG (Kiovig, Baxter) was administered by iv injection. Serum
samples were collected at -168, 0, 24, 72, 120 and 144 h nation of
study) and stored at -20 °C.
Human lgG ELISA: The concentration of human lgG in mouse serum
samples collected from the two studies was analyzed with a human lgG
AlphaLlSA kit (Perkin Elmer, cat. no. AL2050) as described by the
manufacturer. The concentration of hlgG was calculated from a standard
curve and GraphPad Prism 5 using a non-linear regression formula.
Results
The s from the experiments show a ion in the
concentrations of human lgG over time through the action of the FcRn binding
polypeptides. There were little or no difference in the reduction of lgG levels
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between the two groups receiving the polypeptides ZAZ3715 and 6
(Figure 14A). These results indicate that FcRn binding polypeptides with a
central or C-terminal positioning of ABD are equally ent in sing lgG
catabolism. The polypeptides ZAZ3869, ZAZ3870 and ZAZ3871, respectively,
reduced hlgG levels to a similar extent (Figure 148). The results from the
second ment were in the same range as the results obtained in the first
experiment.
Thus, the results from the two experiments te that the FcRn-
specific ptides blocked recycling of IgG, resulting in increased lgG
catabolism and subsequent lower levels of IgG in human FcRn transgenic
mice.
Example 21
Increased lgG catabolism by dimeric FcRn binding polypeptides in NMRI
mice
In this Example, the effect of homodimeric FcRn binding polypeptides
on lgG catabolism was investigated in NMRI mice.
als and methods
Animal study: Homodimeric FcRn-binding polypeptide ZAZ3715 (SEQ
ID NO:371) or 4 (SEQ ID N02373), or vehicle (PBS buffer), was
administered at 0 hours by iv. injection to female NMRI mice, at a dose of 0.6
or 1.7 umol/kg. Serum samples were collected at 0, 24, 48 and 72 h
(termination of study) and stored at -20 °C.
Mouse IgG ELISA: The concentration of mouse lgG in mouse serum
samples was ed by a mouse IgG ELISA kit (Mabtech, . 3825-
1AD-6) and performed as described by the manufacturer. The concentration
of mlgG was calculated from a standard curve and GraphPad Prism 5 using a
non-linear regression formula. The concentration of lgG in individual mice at
24, 48 and 72 h were related to the level at 0 h and the results are therefore
presented as percentage of lgG (0 h).
PK ELISA: Concentrations of FcRn-binding polypeptides in mouse
serum samples were determined by ELISA. In this assay, 96-well half area
plates were coated with a mouse anti Z polyclonal antibody (produced in-
house) at a concentration of 4 ug/ml in PBS (50 ul/well) and incubated
overnight at 4 °C. Next, the plates were rinsed twice in tap water and blocked
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with ng buffer for 1 hour. An in-house Z variant standard was titrated in
a 3-fold dilution series —300 ng/ml) and d serum samples were
added to the coated ELISA plates (50 ul/well) and incubated for 1.5 h at RT.
The plates were washed 4 times in an automated ELISA washer and 4 ug/ml
(50 l) of a goat anti-ABD polyclonal antibody (produced in-house) was
added. After incubation for 1 h, the plates were washed and 50 ul of anti-goat
lgG-HRP on, cat. no. 711152) at a concentration of 20 ng/ml was
added to each well. After one additional hour of incubation and subsequent
washing, the plates were developed with 50 ul TMB per well and the reactions
were stopped with 50 pl 2M H2804. The absorbance at 450 nm was
measured in a 96-well plate reader (Victor3).
Results
lgG catabolism: The results showed a reduction of mouse lgG
concentration in mice treated with the FcRn-specific polypeptides ZAZ3715
and ZAZ3824, respectively (Figure 15). The result obtained with polypeptide
ZAZ3824 shows that the reduction in endogenous lgG levels is dose
dependent, and the most pronounced effect was observed at 72 h. Notably,
the reduction of lgG levels obtained with the use of dimers was greater than
the ion ed with monomeric 207918 in e 11, even though
the monomer was administrated repeatedly and at much higher dose than the
dimers re Figures 15 and 10 at 72 h). Thus, the results indicate that
the FcRn-specific polypeptides disclosed herein could block recycling of lgG,
resulting in an increased lgG catabolism and subsequent lower levels of lgG
in mice.
Pharmacokinetic analysis: The pharmacokinetic profiles of ZAZ371 5
and ZAZ3824 are shown in Figure 16. The half-life of ZAZ3824 was
approximately 62 hours, which is in line with the half-life obtained in the
pharmacokinetic study presented in Example 6, demonstrating that the
cokinetic properties of the polypeptides are further improved by
binding to FcRn in addition to the prolonged half-life resulting from albumin
binding.
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e 22
Increased IgG catabolism by FcRn binding dimers in cynomolgus monkeys
In this Example, the effect of homo- or heterodimeric FcRn binding
polypeptides on IgG catabolism is investigated in cynomolgus monkeys.
Materials and s
Animal study: Homo- and/or heterodimeric FcRn binding polypeptides
recombinantly fused to PP013 (SEQ ID NO:377) are ed. Examples of
such FcRn binding dimers include SEQ ID NO:371-376 disclosed herein.
The FcRn binding dimers including an albumin binding domain are
then administered to cynomolgus monkeys at a dose of 2, 0.4 and 0.1
pmol/kg. The dimeric polypeptides are injected intravenously at 0 hours. The
monkeys are bled 1 h prior to the first administration and daily up to day 21,
and then once a week up to day 50. Sera are prepared and stored at -20 °C.
The concentration of cynomolgus IgG is determined by ELISA.
Homo- and/or heterodimeric FcRn binding polypeptides without an
albumin binding domain are administered to lgus monkeys at a dose
of 2, 0.4 and 0.1 pmol/kg. The dimeric polypeptides are administered three
times per week for two weeks. The monkeys are bled 1 h prior to the first
administration and daily up to day 21, and then once a week up to day 50.
Sera are prepared and stored at -20 °C. The concentration of cynomolgus
IgG is determined by ELISA.
Cynomolgus IgG ELISA: The tration of cynomolgus IgG in
serum samples is determined with a human/cynomolgus IgG ELISA kit (for
e Mabtech 3850-1AD-6, which is reactive with both human and
cynomolgus IgG) as described by the cturer.
Results
The results from the experiment are expected to show a dose
dependent reduction in the concentrations of cynomolgus IgG through the
action of FcRn binding dimers, with a more pronounced effect for such dimers
that also se an albumin binding domain.
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Example 23
Pharmacokinetic study ofdimeric FcRn binding ptides
In this Example, the serum half-life of homo- and/or heterodimeric
FcRn binding polypeptides is investigated in a pharmacokinetic study
performed in mice.
Materials and methods
Pharmacokinetic study: FcRn binding polypeptides, as homo- and/or
heterodimers alone or recombinantly fused to PPO13 (SEQ ID NO:377) are
administered intravenously (i.v.) to male NMRI mice (Charles River,
Germany) at a dose of 92 nmol/. Sera from groups of three mice are obtained
at 0.08, 6, 18, 78, 120, 168 and 240 hours. The concentration of respective
polypeptide is determined by ELISA.
ELISA: rea 96-well ELISA plates are coated at 4 °C overnight
with 50 ul/well of a goat antibody ic for Z variants in general (produced
in-house) diluted to 4 ug/ml in coating buffer (50 mM sodium carbonate, pH
9.6). The antibody solution is poured off and the wells are blocked with 100 pl
of PBSC for 1.5 h at RT. The sera are diluted in PBSC containing 1 % mouse
serum (matrix) from 1:100 to 1:51 ,200 in a two-fold on series in a
dilutions plate. A standard titration for respective Z variant polypeptide and
four quality ls (very low, low, medium and high control) diluted in matrix
are included on each plate. 50 ul of the dilutions are transferred per well and
the ELISA plates are incubated for 1.5 h at RT. The plates are washed four
times with PBST. Bound Z variant polypeptides are detected with 50 l of
rabbit PO13 lg (produced in-house) or 50 ul/well of mouse anti-Z mAb
(produced in-house) diluted to 4 ug/ml in PBSC. The plates are subsequently
incubated for 1.5 h at RT followed by washes as described above. HRP
conjugated donkey anti-rabbit HRP (Jackson laboratories; cat. no. 711
152), diluted 120,000 in PBSC, is added and the plates are ted for 1 h.
After washing as described above, 50 ul of ImmunoPure TMB ate is
added to the wells and the plates are developed according to the
manufacturer’s recommendations. After 15 min of development, the
absorbance is measured at 450 nm using a multi-well plate reader (Victor3).
The absorbance values are analyzed using GraphPad Prism 5 to determine
the trations —spline curve fit) and area under curve (AUC). The
concentrations are then plotted as their natural logarithms against time. The
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resulting curves are ed to follow a two compartment model and the
al half-life is calculated as ln2 divided by the slope based on the last
three time points.
Results
The results from the experiment described herein are expected to
show a two compartment elimination phase with a terminal half-life of
approximately 60 min for ptides without ABD and approximately 90
hours for polypeptides comprising ABD.
Example 24
Generation, stability study and binding assessment of scaffold-modified FcRn
binding polypeptides
The following Example discloses ld modified FcRn binding Z
variants exhibiting improved stability at elevated temperatures. The Z variants
217347 (SEQ ID NO:358), with the amino acid tutions N528 and D53E,
and 217348 (SEQ ID NO:359), with the amino acid substitutions D36R,
D37Q, S39E, N528 and D53E, are compared to their parent le
211948 (SEQ ID NO:354) in terms of stability and binding capacity to FcRn.
Materials and methods
Generation of ld—modified polypeptides: 217347 (SEQ ID
NO:358), 217348 (SEQ ID NO:359) and 211948 (SEQ ID NO:354) were
cloned with an N-terminal 6 x ine-tag (Hisa) and obtained constructs
encoded polypeptides in the format MGSSHHHHHHLQ-[2#####]. Mutations
were introduced in the plasmids of the modified 2 ts using overlapping
oligonucleotide primer pairs encoding the desired amino acid substitutions
and by applying established molecular biology techniques. The correct
plasmid sequences were verified by DNA sequencing.
E coli (strain T7E2) cells (GeneBridge) were transformed with plasmids
containing the gene fragments ng the original and scaffold modified 2
variants. The cells were cultivated at 37 °C in TSB-YE medium supplemented
with 50 pg/ml kanamycin and protein expression was subsequently induced
by addition of IPTG. Pelleted cells were disrupted using a FastPrep®-24
homogenizer (Nordic Biolabs) and cell debris was removed by centrifugation.
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Each supernatant containing the Z variant as a Hise—tagged protein was
purified by immobilized metal ion affinity chromatography (IMAC) using His
GraviTrapTM columns (GE Healthcare) according to the manufacturers
instructions. Purified Z variants were buffer exchanged to phosphate-buffered
saline (PBS; 1.47 mM KH2PO4, 8.1 mM NagHPO4, 137 mM NaCl, 2.68 mM
KCI, pH 7.4) using PD—10 desalting columns (GE Healthcare). The correct
identity of each polypeptide was verified by GE and HPLC-MS.
ar dichroism oscopy analysis: Circular dichroism (CD)
analysis was carried out as described in Example 3 to determine the melting
temperatures (Tm) and assess potential changes in the secondary structure
of the inventive polypeptides as a result of the amino acid substitutions.
Comparative ity study: The Hise-tagged Z variants, formulated in
PBS pH 7.4, were diluted to 1 mg/ml and 200 pl aliquotes were incubated at
37 °C for 2 weeks. Samples collected prior to and after the stability test were
ed by SDS-PAGE using 10% Bis-Tris NuPAGE gels (lnvitrogen) and by
g 5 pg protein into each well. The stabilty was assessed by the
appearance of new variants after incubation at the elevated temperature and
mutated variants were compared to the original polypeptide.
Binding assessment of scaffold-modified ptides: The Hiss-
tagged Z variants were further assessed in terms of ved binding
capacitiy to FcRn after introduction of alterations in the scaffold, as well as
after having been ted to the stability test, i.e. incubated at 37 °C for 2
weeks. Comparative kinetic constants (kon and koff) and affinities (KD) were
determined using a Biacore 2000 instrument. The target protein human FcRn
(Biorbyt, cat. no. orb 84388) was immobilized on the carboxylated dextran
layer surface of a CM5 chip (GE Healthcare). The immobilization was
performed using amine coupling chemistry according to the cturer’s
protocol and using HBS-EP as running buffer. One flow cell surface on the
chip was activated and deactivated for use as blank during analyte ions.
The immobilization level of hFcRn on the surface was approximately 750 RU.
The Z variants were diluted in running buffer to final concentrations of 3.33,
and 30 nM and injected for 3 min, followed by 15 min of dissociation in
running . Regeneration by three pulses of HBS—EP ed by 10 min
equilibration in running buffer was applied after each analyte injection. c
constants were calculated from the sensorgrams using the Langmuir 1:1
model of the BiaEvaluation software 4.1 (GE Healthcare). Curves of the blank
surface were subtracted from the curves of the ligand surfaces and the data
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from the buffer cycles were subtracted from the data of the ample cycles
to correct for any drift in signal.
Results
Circular dichroism spectroscopy analysis: The Tm of each respective Z
variant as determined from the midpoint of the transition in the CD signal vs.
temperature plot is shown in Table 19. The mutated Z variants showed
preserved alphahelical structure and refolded reversibly after heating to
90 °C.
Table 19: Melting temperatures for original and mutated Z variants.
Designation SEQ ID NO Tm (°C) Original vs modified
Z11948 354 48 Original
217347 358 50 Modified
Z17348 359 44 Modified
Comparative stability study: The d modified Z variants 217347
and 217348 showed an improved stability compared to the al
polypeptide 211948. The second band visible on the gel just above the main
band for 211948 was not visible in s of 217347 and 217348 (Figure
17), Le. the scaffold mutations prevent the formation of the alternative s
observed for the sample in the original scaffold.
Binding assessment of scaffold-modified polypeptides: The
ative kinetic constants for the FcRn-binding Z variants are shown in
Table 20. The affinity was marginally effected by the amino acid substitutions
ND to SE in position 52-53, such as in 217347 (SEQ ID NO:358), as well as
by the substitutions ND to SE in position 52-53 in combination with D36R,
D37Q and S39E, such as in 217348 (SEQ ID NO:359), and onal binders
were obtained with KD in the range of 10'9 M. The assessed variants also had
preserved binding capabilities after 2 weeks incubation at 37 °C.
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Table 20. Comparative kinetic analysis of original and modified Z variants.
Orisgaffoldinal vs
Test sample SEEDFD ka (Ms'1) k,| (5'1) KD (M)*
' modified
211948 (0) 354 Original 1.80x106 4.56x10'3 2.9x10'9
211948 (2w) 354 Original 3.15x106 5.75 x10'3 1.8x10'9
217347 0 358 Modified 1.18x106 7.99 x10'3 6.7x10'9
217347 (2w) 358 Modified 2.27x10 8.79 x10‘ 3.9x10'
217348 (0) 359 Modified 1.82x106 1.00 x10'2 5.5x10'9
217348 (2w) 359 Modified 1.28x106 8.09 x10'3 6.3x10'9
* The KD values should not be regarded
as absolute, as these were determined for
comparative purposes and only included a limited number of sample concentrations.
Example 25
Generation and assessment of onal scaffold-modified FcRn binding
ptides
In this e, additional variants with the scaffold amino acid
substitutions N528 and D53E, and some also with the amino acid substitution
Y5F, were analyzed in terms of their stability and binding to FcRn as
compared to their respective parent FcRn binding Z variant. The results show
that the structure, stability and FcRn binding capacity are retained in the
mutated variants.
Materials and methods
Generation of scaffold-modified polypeptides: The amino acid
substitutions N528 and D53E were introduced in the plasmids of Hise-tagged
Z13578 (SEQ ID , 213583 (SEQ ID NO:23), 213616 (SEQ ID NO:41),
213621 (SEQ ID NO:44) and 213674 (SEQ ID NO:75) using established
molecular biology ques resulting in the respective Z variants 218614
(SEQ ID NO:360), 218615 (SEQ ID NO:361), 218616 (SEQ ID NO:362),
218617 (SEQ ID NO:363) and 218618 (SEQ ID NO:364). Additional
modifications at position 5, were the tyrosine residue was substituted to
alanine, as well as N-terminal cation to start with the amino acid
residues AE instead of VD, resulted in the 2 variants 218632 (SEQ ID
), 218633 (SEQ ID NO:366) and 218634 (SEQ ID NO:367) having
g motifs (BM) cal to 213578, 213616 and 213621, respectively.
Cultivation and purification was performed essentially as described in
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Example 3 and e 9. The five Z ts 218614-218618 were purified
by IMAC only, whereas the three Z variants 218632-218634 were further
purified by RPC.
CD is: CD analysis was d out as bed in Example 3 to
determine the melting temperatures (Tm) and assess potential changes in the
secondary structure of the d Z ts compared to their respective
parent Z variant.
Biacore binding analysis: A binding analysis at pH 6.0, using a Biacore
instrument, was performed essentially as described in Example 3. A
concentration series (270, 90, 30, 10 and 3.3 nM) of the Hiss-tagged Z
variants 218632, 218633 and 218634 and their respective corresponding
parent Z variants 213578, 213616 and 213621, were injected during 4 min at
ul/min over hFcRn yt, cat. no. orb84388) and chRn (Biorbyt, cat.no.
orb99075), immobilized in different flow cells of a CM5 chip surface. 0.005 %
PCT pH 6.0 was used as running buffer and for dilutions of the Hise-tagged 2
variants. Dissociation in running buffer was allowed for 20 min, followed by
surface regeneration by injection of 3 x 30 second pulses of 0.00 5% PCT pH
7.4 and equilibration for 15 min before the start of next cycle.
Results
Cultivation and cation: The FcRn g 2 variants were
constructed with an N—terminal Hiss—tag and produced in E. coli. SDS—PAGE
analysis of each final protein preparation showed that it predominantly
contained the 2 variant. The correct identity and molecular weight of each
FcRn g 2 variant was confirmed by HPLC-MS analysis.
CD analysis: The Tm of the mutated FcRn binding 2 variants were
identical, or nearly identical, to the Tm of the respective parent 2 variant
(Table 21). Furthermore, reversible g was observed for all seven 2
variants by overlaying a obtained before and after heating to 90 °C.
Biacore g analysis: The binding profiles for interactions with
FcRn at pH 6.0 were compared pairwise for three mutated 2 variants and
their respective parent 2 variants; 218632/213578 (SEQ ID NO:365/20),
218633/213616 (SEQ ID NO:366/41) and 218634/213621 (SEQ ID
NO:367/44). Overlays of sensorgrams from the 90 nM injections of the Z
variants over hFcRn and chRn surfaces show that the mutated 2 variants
retained their ability to bind to human and cynomolgus FcRn (Figure 18A—C).
The FcRn immobilization levels of the chip surfaces were 1577 RU for human
FcRn and 1098 RU for cynomolgus FcRn.
Table 21: Meltino temperatures for scaffold mutated and parent Z ts.
—--WZvariant NO: Z variant
218616 362 62 ——m-
218618 364 so
218632 365 56
218633 366 61 m-
218634 367 48 213621 44 49
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ITEMIZED LISTING OF EMBODIMENTS
1. FcRn binding dimer, comprising a first monomer unit, a second
monomer unit and an amino acid linker, wherein said first and second
monomer unit each comprises an FcRn binding motif (BM), which motif
consists of the amino acid sequence
EX2 X3 X4 AXe X7 EIR 16X17 X18 QR X21 AFIX25 X26LX28 X29
wherein, independently from each other,
X2 is selected from A, D, E, F, H, I, K, L, N, Q, R, S, T, V, W and Y;
X3 is selected from A, D, E, F, G, H, l, K, L, M, N, Q, R, S, T, V, W and
X4 is selected from A, D, E, F, G, H, l, K, L, N, Q, R, S, T, V, W and Y;
X5 is selected from A, E, F, G, H, l, K, Q, R, S and V;
X7 is selected from A, F, H, K, N, Q, R, S and V;
X16 is selected from N and T;
X17 is ed from F, W and Y;
X18 is selected from A, D, E and N;
X21 is selected from A, S, V and W;
X25 is selected from D, E, G, H, l, K, L, N, Q, R, S, T, V, W and Y;
X26 is selected from K and S;
X28 is selected from A, D, E, F, H, l, K, L, N, Q, R, S, T, V, W and Y;
and
X29 is selected from D and R,
and wherein said FcRn binding dimer binds FcRn with a higher g
capacity compared to said first monomer unit or said second monomer unit
alone.
2. FcRn binding dimer according to item 1, wherein, ndently
from each other,
X2 is selected from A, D, E, F, H, l, K, L, N, Q, R, S, T, V, W and Y;
X3 is selected from A, D, E, F, H, l, K, L, M, N, Q, R, S, T, V, W and Y;
X4 is selected from A, D, E, F, H, l, K, L, N, Q, R, S, T, V, W and Y;
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X5 is selected from A, E, F, G, H, I, K, Q, R and S;
X7 is selected from A, F, H, K, N, Q, R, S and V;
X16 is selected from N and T;
X17 is selected from F and Y;
X18 iS D;
X21 is V;
X25 is selected from D, E, H, l, K, L, N, Q, R, S, T, V, W and Y;
X26 is selected from K and S;
X28 is selected from A, D, E, F, H, l, K, L, N, Q, R, S, T, V and W; and
X29 is selected from D and R.
3. FcRn binding dimer according to item 1, wherein the BM of at least
one of said first and second monomer units consists of an amino acid
sequence selected from
i) EX2 X3 X4 AXe HEIR WLPNLTX17 X18 QR X21 AFIX25 KLX28 D
wherein, ndently from each other,
X2 is selected from A, D, E, F, H, l, K, L, N, Q, R, S, T, V, W and Y;
X3 is selected from A, D, E, G, H, K, L, M, N, Q, R, S, T, V and Y;
X4 is selected from A, D, E, F, G, l, K, L, N, Q, R, S, T, V and Y;
X6 is selected from A, G, K, R, S and V;
X17 is selected from F, W and Y;
X18 is selected from A, D, E and N;
X21 is selected from A, S, V and W;
X25 is selected from D, G, H, K, L, N, R, V and W;
X28 is selected from A, D, E, H, K, L, N, Q, R, S, T, W and Y;
and
ii) an amino acid ce which has at least 96 % ty to a
sequence defined by i).
4. FcRn binding dimer according to any one of items 1-3, wherein X6X7
is selected from AH and GH in at least one of said first and second monomer
units.
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. FcRn binding dimer ing to item 4, wherein X6X7 is AH in at
least one of said first and second monomer units.
6. FcRn binding dimer according to item 4, wherein X6X7 is GH in at
least one of said first and second r units.
7. FcRn binding dimer according to any preceding item, wherein X17X18
is selected from FD and YD in at least one of said first and second monomer
units.
8. FcRn binding dimer ing to item 7, wherein X17X18 is FD in at
least one of said first and second monomer units.
9. FcRn binding dimer according to any preceding item, wherein the
sequence of the BM of at least one of said first and second monomer units
fulfills at least three of the six conditions l-Vl:
l. X6 is selected from A, G, K and S, such as in ular A;
ll. X7 is H;
lll. X17 is selected from F and Y, such as in particular F;
IV. X18 iS D;
V. X21 is selected from V and W, such as in particular V;
VI. X25 is selected from H and R, such as in particular H.
. FcRn binding dimer according to item 9, wherein the sequence
fulfills at least four of the six conditions l-Vl.
11. FcRn binding dimer according to item 10, wherein the ce
fulfills at least five of the six conditions l-Vl.
12. FcRn binding dimer according to item 11, wherein the sequence
fulfills all of the six conditions l-Vl.
13. FcRn binding dimer ing to any preceding item, n said
first and second monomer units comprise identical BM sequences.
14. FcRn binding dimer according to any one of items 1-12, wherein
said first and second monomer units comprise different BM sequences.
. FcRn binding dimer according to any preceding item, wherein at
least one of said first and second monomer units comprises an FcRn binding
motif BM corresponding to the sequence from position 8 to position 36 in a
sequence selected from the group consisting of SEQ ID NO:1-353, such as
the group ting of SEQ ID NO:17-352.
16. FcRn binding dimer according to item 15, wherein at least one of
said first and second monomer units comprises a BM ponding to the
sequence from position 8 to position 36 in a sequence selected from the
group consisting of SEQ ID NO:1-15, SEQ ID NO:17-140 and SEQ ID
NO:353.
17. FcRn binding dimer according to item 16, wherein at least one of
said first and second monomer units comprises a BM corresponding to the
sequence from position 8 to position 36 in a sequence selected from the
group consisting of SEQ ID NO:1-2 and SEQ ID NO:17-140, such as the
group consisting of SEQ ID NO:17-140.
18. FcRn binding dimer according to item 17, wherein at least one of
said first and second monomer units comprises a BM corresponding to the
sequence from position 8 to position 36 in a sequence selected from the
group ting of SEQ ID NO:1-2, SEQ ID NO:17-92, SEQ ID NO:94-103,
SEQ ID NO:105-125 and SEQ ID NO:127-140, such as the group consisting
of SEQ ID NO:17-92, SEQ ID NO:94-103, SEQ ID NO:105-125 and SEQ ID
NO:127-140.
19. FcRn binding dimer ing to item 16, wherein at least one of
said first and second r units comprises a BM corresponding to the
sequence from position 8 to position 36 in a ce ed from the
group consisting of SEQ ID NO:1-8, SEQ ID NO:13, SEQ ID NO:19-20, SEQ
ID NO:23, SEQ ID NO:28, SEQ ID NO:41, SEQ ID NO:44, SEQ ID NO:65,
SEQ ID NO:70, SEQ ID NO:73, SEQ ID NO:75-77 and SEQ ID NO:353, such
as the group consisting of SEQ ID NO:19-20, SEQ ID NO:23, SEQ ID NO:28,
SEQ ID NO:41, SEQ ID NO:44, SEQ ID NO:65, SEQ ID NO:70, SEQ ID
NO:73 and SEQ ID NO:75-77.
. FcRn binding dimer according to item 18 or 19, wherein at least
one of said first and second monomer units comprises a BM corresponding to
the sequence from position 8 to position 36 in a sequence ed from the
group consisting of SEQ ID NO:1, SEQ ID NO:20, SEQ ID NO:23, SEQ ID
NO:28, SEQ ID NO:41, SEQ ID NO:44, SEQ ID NO:65, SEQ ID NO:73 and
SEQ ID NO:75-77, such as the group consisting of SEQ ID NO:20, SEQ ID
NO:23, SEQ ID NO:28, SEQ ID NO:41, SEQ ID NO:44, SEQ ID NO:65, SEQ
ID NO:73 and SEQ ID 77.
21. FcRn binding dimer according to item 20, wherein at least one of
said first and second monomer units comprises a BM corresponding to the
sequence from on 8 to position 36 in a sequence selected from the
group consisting of SEQ ID NO:1, SEQ ID NO:20, SEQ ID NO:23, SEQ ID
NO:41, SEQ ID NO:44, SEQ ID NO:65, SEQ ID NO:75 and SEQ ID NO:77,
such as the group consisting of SEQ ID NO:20, SEQ ID NO:23, SEQ ID
NO:41, SEQ ID NO:44, SEQ ID NO:65, SEQ ID NO:75 and SEQ ID NO:77.
22. FcRn binding dimer according to item 21, n at least one of
said first and second monomer units ses a BM corresponding to the
sequence from position 8 to position 36 in a ce selected from the
group consisting of SEQ ID NO:1, SEQ ID NO:20, SEQ ID NO:23, SEQ ID
NO:41, SEQ ID NO:44, SEQ ID NO:65 and SEQ ID NO:75, such as the group
consisting of SEQ ID NO:20, SEQ ID NO:23, SEQ ID NO:41, SEQ ID NO:44,
SEQ ID NO:65 and SEQ ID NO:75.
23. FcRn binding dimer according to item 22, wherein at least one of
said first and second monomer units comprises a BM corresponding to the
sequence from position 8 to position 36 in a sequence selected from the
group consisting of SEQ ID NO:1, SEQ ID N023 and SEQ ID NO:75, such
as the group consisting of SEQ ID N023 and SEQ ID NO:75.
24. FcRn binding dimer according to item 22, wherein at least one of
said first and second monomer units comprises a BM corresponding to the
sequence from position 8 to position 36 in a sequence selected from the
group consisting of SEQ ID NO:20, SEQ ID NO:41 and SEQ ID NO:44, such
as the group consisting of SEQ ID N020 and SEQ ID NO:41; the group
consisting of SEQ ID N020 and SEQ ID NO:44; or the group ting of
SEQ ID NO:41 and SEQ ID NO:44.
. FcRn binding dimer according to item 22, n at least one of
said first and second monomer units comprises a BM corresponding to the
sequence from position 8 to position 36 in a ce selected from the
group consisting of SEQ ID NO:1, SEQ ID N023 and SEQ ID NO:44, such
as the group consisting of SEQ ID N023 and SEQ ID NO:44.
26. FcRn g dimer ing to item 24 or 25, wherein at least
one of said first and second monomer units comprises a BM corresponding to
the sequence from position 8 to position 36 in sequence SEQ ID NO:44.
27. FcRn binding dimer according to any preceding item, n both
said first and second monomer units independently comprise a BM
corresponding to the sequence from position 8 to position 36 in a sequence
selected as defined in any one of items 15-26.
28. FcRn binding dimer according to item 27, wherein both said first
and second monomer units independently comprise a BM corresponding to
the sequence from position 8 to position 36 in a sequence selected from the
group consisting of SEQ ID NO:20, SEQ ID NO:23, SEQ ID NO:41, SEQ ID
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NO:44 and SEQ ID NO:75, such as the group consisting of SEQ ID NO:20,
SEQ ID NO:41 and SEQ ID NO:44.
29. FcRn binding dimer according to item 28, wherein both said first
and second monomer units comprise a BM corresponding to the sequence
from position 8 to position 36 in SEQ ID NO:44.
. FcRn binding dimer according to any preceding item, wherein said
FcRn binding motif BM in at least one of said first and second monomers
forms part of a three-helix bundle protein domain.
31. FcRn binding dimer according to item 30, wherein said BM
essentially forms part of two helices with an interconnecting loop, within said
three-helix bundle protein domain.
32. FcRn binding dimer according to item 31, wherein said three—helix
bundle protein domain is selected from bacterial receptor s.
33. FcRn binding dimer ing to item 32, wherein said three—helix
bundle protein domain is selected from domains of protein A from
Staphylococcus aureus or derivatives thereof.
34. FcRn binding dimer according to any preceding item, wherein at
least one of said first and second monomer units comprises a g module
(BMod), which module ts of an amino acid sequence selected from:
iii) K-[BM]—DPSQS XaXbLLXC EAKKL XdXeXfQ;
wherein
[BM] is an FcRn binding motif as defined in any one of items 1—29,
provided that X29 is D;
X3 is selected from A and S;
Xb is ed from N and E;
X0 is selected from A, S and C;
Xd is ed from E, N and S;
Xe is selected from D, E and S;
Xf is selected from A and S;
iv) an amino acid ce which has at least 93 % identity to a
sequence defined by iii).
. FcRn binding dimer ing to any one of items 1-33, wherein at
least one of said first and second monomer units comprises a g module
(BMod), which module ts of an amino acid sequence selected from:
v) K-[BM]—QPEQS XaXbLLXC EAKKL XdXeXfQ;
wherein
[BM] is an FcRn binding motif as defined in any one of items 1-29,
provided that X29 is R;
X8 is selected from A and S;
Xb is selected from N and E;
XC is selected from A, S and C;
Xd is selected from E, N and S;
Xe is selected from D, E and S;
Xf is selected from A and S;
vi) an amino acid sequence which has at least 93 % identity to a
sequence defined by v).
36. FcRn g dimer according to item 34, wherein at least one of
said first and second monomer units comprises a BMod corresponding to the
sequence from position 7 to position 55 in a sequence selected from the
group consisting of SEQ ID NO:1-353, SEQ ID NO:358 and SEQ ID N01360-
364, such as the group consisting of SEQ ID NO:17-352 and SEQ ID
NO:360-364.
37. FcRn binding dimer according to item 36, wherein at least one of
said first and second monomer units comprises a BMod corresponding to the
sequence from position 7 to position 55 in a sequence selected from the
group consisting of SEQ ID NO:1-15, SEQ ID NO:17-140, SEQ ID NO:353,
SEQ ID NO:358 and SEQ ID -364.
38. FcRn binding dimer according to item 37, wherein at least one of
said first and second monomer units ses a BMod ponding to the
sequence from position 7 to position 55 in a sequence selected from the
group consisting of SEQ ID NO:1-2, SEQ ID NO:17-140, SEQ ID NO:358 and
SEQ ID NO:360—364, such as the group consisting of SEQ ID 140 and
SEQ ID NO:360-364.
39. FcRn binding dimer according to item 38, wherein at least one of
said first and second monomer units comprises a BMod corresponding to the
sequence from position 7 to position 55 in a sequence selected from the
group consisting of SEQ ID NO:1-2, SEQ ID NO:17-92, SEQ ID NO:94-103,
SEQ ID NO:105-125, SEQ ID NO:127-140, SEQ ID NO:358 and SEQ ID
NO:360-364, such as the group consisting of SEQ ID NO:17-92, SEQ ID
NO:94-103, SEQ ID NO:105-125, SEQ ID NO:127-140 and SEQ ID -
364.
40. FcRn binding dimer according to item 36, wherein at least one of
said first and second monomer units comprises a BMod corresponding to the
sequence from position 7 to on 55 in a sequence selected from the
group consisting of SEQ ID NO:1-8, SEQ ID NO:13, SEQ ID NO:19-20, SEQ
ID NO:23, SEQ ID NO:28, SEQ ID NO:41, SEQ ID NO:44, SEQ ID NO:65,
SEQ ID NO:70, SEQ ID NO:73, SEQ ID NO:75-77, SEQ ID NO:353, SEQ ID
NO:358 and SEQ ID NO:360-364, such as the group consisting of SEQ ID
NO:19—20, SEQ ID NO:23, SEQ ID NO:28, SEQ ID NO:41, SEQ ID NO:44,
SEQ ID NO:65, SEQ ID NO:70, SEQ ID NO:73, SEQ ID NO:75-77 and SEQ
ID NO:360-364.
41. FcRn binding dimer according to item 39 or 40, wherein at least
one of said first and second monomer units comprises a BMod corresponding
to the sequence from position 7 to on 55 in a sequence selected from
the group consisting of SEQ ID NO:1, SEQ ID NO:20, SEQ ID NO:23, SEQ
ID NO:28, SEQ ID NO:41, SEQ ID NO:44, SEQ ID NO:65, SEQ ID NO:73,
SEQ ID NO:75-77, SEQ ID NO:358 and SEQ ID —364, such as the
group consisting of SEQ ID NO:20, SEQ ID NO:23, SEQ ID NO:28, SEQ ID
NO:41, SEQ ID NO:44, SEQ ID NO:65, SEQ ID NO:73, SEQ ID NO:75-77
and SEQ ID NO:360-364.
42. FcRn binding dimer according to item 41, wherein at least one of
said first and second monomer units comprises a BMod corresponding to the
sequence from position 7 to position 55 in a sequence ed from the
group consisting of SEQ ID NO:1, SEQ ID NO:20, SEQ ID NO:23, SEQ ID
NO:41, SEQ ID NO:44, SEQ ID NO:65, SEQ ID NO:75,SEQ ID NO:77, SEQ
ID NO:358 and SEQ ID NO:360-364, such as the group ting of SEQ ID
NO:20, SEQ ID NO:23, SEQ ID NO:41, SEQ ID NO:44, SEQ ID NO:65, SEQ
ID NO:75, SEQ ID NO:77 and SEQ ID -364.
43. FcRn binding dimer according to item 42, wherein at least one of
said first and second monomer units comprises a BMod corresponding to the
sequence from position 7 to position 55 in a sequence selected from the
group ting of SEQ ID NO:1, SEQ ID NO:20, SEQ ID NO:23, SEQ ID
NO:41, SEQ ID NO:44, SEQ ID NO:65, SEQ ID NO:75, SEQ ID NO:358 and
SEQ ID NO:360-364, such as the group consisting of SEQ ID NO:20, SEQ ID
NO:23, SEQ ID NO:41, SEQ ID NO:44, SEQ ID NO:75 and SEQ ID NO:360-
364.
44. FcRn binding dimer according to item 43, wherein at least one of
said first and second monomer units comprises a BMod corresponding to the
sequence from position 7 to position 55 in a sequence selected from the
group consisting of SEQ ID NO:1, SEQ ID NO:23, SEQ ID NO:75, SEQ ID
NO:358, SEQ ID NO:361 and SEQ ID NO:364, such as the group consisting
of SEQ ID NO:23, SEQ ID NO:75, SEQ ID NO:361 and SEQ ID NO:364.
45. FcRn binding dimer according to item 43, wherein at least one of
said first and second monomer units comprises a BMod corresponding to the
sequence from position 7 to position 55 in a sequence selected from the
group consisting of SEQ ID NO:20, SEQ ID NO:41, SEQ ID NO:44, SEQ ID
, SEQ ID NO:362 and SEQ ID NO:363, such as the group consisting
of SEQ ID NO:20, SEQ ID NO:41, SEQ ID NO:360 and SEQ ID ; the
group consisting of SEQ ID NO:20, SEQ ID NO:44, SEQ ID NO:360 and SEQ
ID NO:363; or the group consisting of SEQ ID NO:41, SEQ ID NO:44, SEQ ID
NO:362 and SEQ ID .
46. FcRn binding dimer according to item 43, wherein at least one of
said first and second monomer units comprises a BMod ponding to the
sequence from position 7 to position 55 in a sequence selected from the
group consisting of SEQ ID NO:1, SEQ ID NO:23 ,SEQ ID NO:44, SEQ ID
NO:358, SEQ ID NO:361 and SEQ ID NO:363, such as the group consisting
of SEQ ID NO:23,SEQ ID NO:44, SEQ ID NO:361 and SEQ ID NO:363.
47. FcRn binding dimer according to item 46, wherein at least one of
said first and second monomer units ses a BMod corresponding to the
sequence from on 7 to position 55 in SEQ ID NO:44.
48. FcRn binding dimer according to any one of items 1-13 and 15-47,
wherein both said first and second r units comprise a BMod
corresponding to the sequence from position 7 to position 55 in a sequence
selected from the group as defined in any one of items 36-47.
49. FcRn binding dimer according to item 48, wherein both said first
and second monomer units comprise a BMod corresponding to the sequence
from position 7 to position 55 in a sequence selected from the group
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consisting of SEQ ID NO:20, SEQ ID NO:23, SEQ ID NO:41, SEQ ID NO:44 ,
SEQ ID NO:75 and SEQ ID NO:360—364, such as the group consisting of
SEQ ID NO:20, SEQ ID NO:41, SEQ ID NO:44, SEQ ID NO:360, SEQ ID
NO:362 and SEQ ID NO:363.
50. FcRn binding dimer according to item 49, wherein both said first
and second monomer units se a BMod corresponding to the sequence
from on 7 to position 55 in SEQ ID NO:44.
51. FcRn binding dimer according to any preceding item, n at
least one of said first and second r units comprises a sequence
selected from the group consisting of:
vii) YAK-[BM-DPSQS SELLXC EAKKL NDSQA P;
wherein [BM] is an FcRn binding motif as defined in any one of items 1-29
and XC is selected from A, S and C; and
viii) an amino acid sequence which has at least 94 % identity to a
sequence d by vii).
52. FcRn binding dimer according to any one of items 1—50, wherein at
least one of said first and second monomer units comprises a sequence
selected from the group consisting of:
ix) FAK-[BM]-DPSQS SELLXC EAKKL SESQA P;
n [BM] is an FcRn binding motif as defined in any one of items 1-29
and XC is selected from A, S and C; and
x) an amino acid sequence which has at least 94 % identity to a
sequence defined by ix).
53. FcRn binding dimer according to any one of items 1-50, wherein at
least one of said first and second monomer units comprises a sequence
selected from the group consisting of:
Xi) FNK—[BM—DPSQS ANLLXC EAKKL NDAQA P;
WO 42083
wherein [BM] is an FcRn binding motif as d in any one of items 1-29
and XC is ed from A and C; and
xii) an amino acid sequence which has at least 94 % identity to a
sequence defined by xi).
54. FcRn binding dimer according to item 33, wherein at least one of
said first and second monomer units comprises a sequence selected from:
ADNNFNK-[BM]—DPSQSANLLSEAKKLNESQAPK;
ADNKFNK-[BM]—DPSQSANLLAEAKKLNDAQAPK;
ADNKFNK-[BMJ-DPSVSKEILAEAKKLNDAQAPK;
ADAQQNNFNK-[BM]-DPSQSTNVLGEAKKLNESQAPK;
AQHDE-[BM]-DPSQSANVLGEAQKLNDSQAPK;
VDNKFNK-[BMj-DPSQSANLLAEAKKLNDAQAPK;
AEAKYAK-[BMj-DPSESSELLSEAKKLNKSQAPK;
VDAKYAK-[BMj-DPSQSSELLAEAKKLNDAQAPK'
VDAKYAK-[BMJ-DPSQSSELLAEAKKLNDSQAPK'
AEAKYAK-[BMj-DPSQSSELLSEAKKLNDSQAPK;
AEAKYAK-[BMj-DPSQSSELLSEAKKLNDSQAP;
AEAKFAK-[BMj-DPSQSSELLSEAKKLNDSQAPK;
AEAKFAK-[BMj-DPSQSSELLSEAKKLNDSQAP;
AEAKYAK-[BMj-DPSQSSELLAEAKKLNDAQAPK;
AEAKYAK-[BMj-DPSQSSELLSEAKKLSESQAPK;
K-[BMj-DPSQSSELLSEAKKLSESQAP;
AEAKFAK-[BM]—DPSQSSELLSEAKKLSESQAPK;
AEAKFAK-[BM]—DPSQSSELLSEAKKLSESQAP;
AEAKYAK-[BM]—DPSQSSELLAEAKKLSEAQAPK;
AEAKYAK-[BMJ-QPEQSSELLSEAKKLSESQAPK;
AEAKYAK-[BM]—DPSQSSELLSEAKKLESSQAPK;
AEAKYAK-[BMJ-DPSQSSELLSEAKKLESSQAP;
AEAKYAK-[BM]—DPSQSSELLAEAKKLESAQAPK;
AEAKYAK-[BMJ—QPEQSSELLSEAKKLESSQAPK;
AEAKYAK-[BM]—DPSQSSELLSEAKKLSDSQAPK;
AEAKYAK-[BMj-DPSQSSELLSEAKKLSDSQAP;
AEAKYAK-[BM]—DPSQSSELLAEAKKLSDAQAPK;
AEAKYAK-[BMJ—QPEQSSELLSEAKKLSDSQAPK;
VDAKYAK-[BM]—DPSQSSELLSEAKKLNDSQAPK;
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VDAKFAK-[BMj-DPSQSSELLSEAKKLNDSQAPK;
VDAKYAK-[BM]—DPSQSSELLAEAKKLNDAQAPK;
VDAKYAK-[BMj-DPSQSSELLSEAKKLSESQAPK;
VDAKFAK-[BM]—DPSQSSELLSEAKKLSESQAPK;
VDAKYAK-[BMj-DPSQSSELLAEAKKLSEAQAPK;
VDAKYAK-[BM]—QPEQSSELLSEAKKLSESQAPK;
VDAKYAK-[BMj-DPSQSSELLSEAKKLESSQAPK;
K-[BM]—DPSQSSELLAEAKKLESAQAPK;
VDAKYAK-[BMj—QPEQSSELLSEAKKLESSQAPK;
VDAKYAK-[BM]—DPSQSSELLSEAKKLSDSQAPK;
VDAKYAK-[BMj-DPSQSSELLAEAKKLSDAQAPK;
VDAKYAK-[BMJ—QPEQSSELLSEAKKLSDSQAPK;
VDAKYAK-[BMj-DPSQSSELLAEAKKLNKAQAPK;
AEAKYAK-[BM]-DPSQSSELLAEAKKLNKAQAPK; and
ADAKYAK-[BM]—DPSQSSELLSEAKKLNDSQAPK;
wherein [BM] is an FcRn binding motif as defined in any one of items 1—29.
55. FcRn g dimer according to any preceding item, wherein at
least one of said first and second monomer units comprises a sequence
selected from the group consisting of:
xiii) AEAKYAK-[BM-DPSQSSELLSEAKKLNDSQAPK;
n [BM] is an FcRn binding motif as d in any one of items 1-29;
xiv) an amino acid sequence which has at least 94 % identity to the
sequence defined in xiii).
56. FcRn binding dimer according to item 55, wherein at least one of
said first and second monomer units comprises a sequence xiii) selected from
the group consisting of SEQ ID NO:354-357, such as selected from SEQ ID
NO:354 and 357.
57. FcRn binding dimer according to item 56, wherein at least one of
said first and second monomer units comprises a sequence xiii) which is SEQ
ID NO:357.
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58. FcRn binding dimer according to any one of items 1-54, wherein at
least one of said first and second monomer units comprises a sequence
selected from the group consisting of:
xv) AEAKFAK-[BM]—DPSQSSELLSEAKKLSESQAPK;
wherein [BM] is an FcRn binding motif as defined in any one of items 1-29;
xvi) an amino acid sequence which has at least 94 % identity to the
sequence defined in xv).
59. FcRn binding dimer according to item 58, wherein at least one of
said first and second monomer units comprises a sequence xv) selected from
the group consisting of SEQ ID NO:365-367.
60. FcRn binding dimer according to any one of items 1-54, wherein at
least one of said first and second monomer units comprises a sequence
ed from the group consisting of:
xvii) VDAKYAK-[BM]—DPSQSSELLSEAKKLSESQAPK;
wherein [BM] is an FcRn binding motif as defined in any one of items 1—29;
xviii) an amino acid ce which has at least 94 % identity to the
sequence defined in xvii).
61. FcRn binding dimer according to item 60, wherein at least one of
said first and second monomer units comprises a sequence xvii) selected
from the group ting of SEQ ID NO:360-364.
62. FcRn g dimer according to any preceding item, n at
least one of said first and second monomer units comprises a sequence
selected from the group consisting of:
xix) AEAKYAK-[BM-RQPESSELLSEAKKLSESQAPK;
n [BM] is an FcRn binding motif as defined in any one of items 1-29;
xx) an amino acid sequence which has at least 94 % identity to the
sequence defined in xix).
63. FcRn binding dimer according to item 62, wherein at least one of
said first and second monomer units comprises a sequence xix) which is SEQ
ID NO:359.
64. FcRn binding dimer according to any one of items 1-54, wherein at
least one of said first and second monomer units comprises a sequence
selected from the group consisting of:
XXi) VDAKYAK-[BM-DPSQSSELLSEAKKLNDSQAPK;
wherein [BM] is an FcRn binding motif as d in any one of items 1-29;
xxii) an amino acid sequence which has at least 94 % identity to the
ce d in xxi).
65. FcRn binding dimer according to item 64, wherein at least one of
said first and second monomer units comprises a sequence xxi) selected from
the group consisting of SEQ ID NO:1-353, such as the group consisting of
SEQ ID NO:17-352.
66. FcRn binding dimer according to item 65, wherein at least one of
said first and second monomer units comprises a sequence xxi) selected from
the group ting of SEQ ID NO:1-15, SEQ ID NO:17-140 and SEQ ID
NO:353, or comprises a sequence xxi) selected from the group consisting of
SEQ ID NO:1-2 and SEQ ID NO:17-140, such as the group consisting of SEQ
ID NO:17-140.
67. FcRn binding dimer according to item 66, wherein at least one of
said first and second monomer units comprises a sequence xxi) selected from
the group consisting of SEQ ID NO:1-2, SEQ ID NO:17-92, SEQ ID NO:94-
103, SEQ ID NO:105-125 and SEQ ID -140, such as the group
consisting of SEQ ID NO:17-92, SEQ ID NO:94-103, SEQ ID NO:105-125
and SEQ ID NO:127-140.
2015/071339
68. FcRn binding dimer according to item 67, wherein at least one of
said first and second monomer units comprises a ce xxi) selected from
the group consisting of SEQ ID NO:1—8, SEQ ID NO:13, SEQ ID NO:19-20,
SEQ ID NO:23, SEQ ID NO:28, SEQ ID NO:41, SEQ ID NO:44, SEQ ID
NO:65, SEQ ID NO:70, SEQ ID NO:73, SEQ ID 77 and SEQ ID
NO:353, such as the group consisting of SEQ ID NO:19-20, SEQ ID NO:23,
SEQ ID NO:28, SEQ ID NO:41, SEQ ID NO:44, SEQ ID NO:65, SEQ ID
NO:70, SEQ ID NO:73 and SEQ ID NO:75-77.
69. FcRn binding dimer according to item 66 or 68, wherein at least
one of said first and second monomer units comprises a sequence xxi)
selected from the group consisting of SEQ ID NO:1, SEQ ID NO:20, SEQ ID
NO:23, SEQ ID NO:28, SEQ ID NO:41, SEQ ID NO:44, SEQ ID NO:65, SEQ
ID NO:73 and SEQ ID NO:75-77, such as the group consisting of SEQ ID
NO:20, SEQ ID NO:23, SEQ ID NO:28, SEQ ID NO:41, SEQ ID NO:44, SEQ
ID NO:65, SEQ ID NO:73 and SEQ ID NO:75-77.
70. FcRn binding dimer according to item 69, wherein at least one of
said first and second monomer units comprises a ce xxi) selected from
the group consisting of SEQ ID NO:1, SEQ ID NO:20, SEQ ID NO:23, SEQ
ID NO:41, SEQ ID NO:44, SEQ ID NO:65, SEQ ID NO:75 and SEQ ID
NO:77, such as the group consisting of SEQ ID NO:20, SEQ ID NO:23, SEQ
ID NO:41, SEQ ID NO:44, SEQ ID NO:65, SEQ ID NO:75 and SEQ ID
NO:77.
71. FcRn g dimer according to item 70 wherein at least one of
said first and second r units comprises a sequence xxi) selected from
the group consisting of SEQ ID NO:1, SEQ ID NO:20, SEQ ID NO:23, SEQ
ID NO:41, SEQ ID NO:44, SEQ ID NO:65 and SEQ ID NO:75, such as the
group consisting of SEQ ID NO:20, SEQ ID NO:23, SEQ ID NO:41, SEQ ID
NO:44, SEQ ID NO:65 and SEQ ID NO:75, such as the group consisting of
SEQ ID NO:20, SEQ ID NO:23, SEQ ID NO:41, SEQ ID NO:44 and SEQ ID
NO:75.
72. FcRn binding dimer according to item 71, wherein at least one of
said first and second monomer units comprises a sequence xxi) selected from
the group consisting of SEQ ID NO:1, SEQ ID N023 and SEQ ID NO:75,
such as the group consisting ofSEQ ID N023 and SEQ ID NO:75.
73. FcRn binding dimer according to item 71, wherein at least one of
said first and second monomer units comprises a sequence xxi) selected from
the group consisting of SEQ ID NO:20, SEQ ID NO:41 and SEQ ID NO:44.
74. FcRn binding dimer ing to item 71, wherein at least one of
said first and second monomer units comprises a sequence xxi) selected from
the group consisting of SEQ ID NO:1, SEQ ID N023 and SEQ ID NO:44,
such as the group consisting of SEQ ID N023 and SEQ ID NO:44.
75. FcRn binding dimer according to item 73 or 74, wherein at least
one of said first and second monomer units comprises a sequence xxi) which
is SEQ ID NO:44.
76. FcRn binding dimer according to any one of items 1-13 and 15-75,
wherein both said first and second r units correspond to a ce
ed from the group as defined in any one of items 55, 56 and 62-75.
77. FcRn binding dimer according to item 76, wherein both said first
and second monomer units pond to a sequence selected from the
group consisting of SEQ ID NO:1, SEQ ID NO:20, SEQ ID NO:23, SEQ ID
NO:41, SEQ ID NO:44, SEQ ID NO:65, SEQ ID NO:75, SEQ ID NO:354,
SEQ ID NO:357 and SEQ ID NO:360—367, such as the group consisting of
SEQ ID NO:20, SEQ ID NO:41, SEQ ID NO:44, SEQ ID NO:360, SEQ ID
, SEQ ID NO:363, SEQ ID NO:365, SEQ ID NO:366 and SEQ ID
NO:367.
78. FcRn binding dimer according to item 77, wherein both said first
and second monomer units pond to SEQ ID N021 or SEQ ID NO:357.
79. FcRn binding dimer according to item 77, wherein both said first
and second monomer units correspond to SEQ ID NO:20, SEQ ID NO:360 or
SEQ ID NO:365.
80. FcRn binding dimer according to item 77, wherein both said first
and second monomer units correspond to SEQ ID NO:41, SEQ ID NO:362 or
SEQ ID NO:366.
81. FcRn binding dimer ing to item 77, wherein both said first
and second monomer units correspond to SEQ ID NO:44, SEQ ID NO:363 or
SEQ ID NO:367.
82. FcRn binding dimer according to any preceding item, wherein said
linker is selected from the group consisting of flexible amino acid linkers, rigid
amino acid linkers and cleavable amino acid linkers.
83. FcRn binding dimer according to item 82, wherein said linker is
arranged between said first monomer unit and said second r unit.
84. FcRn binding dimer according to item 82 or 83, wherein said linker
is a flexible linker comprising amino acid residues selected from the group
consisting of glycine, serine and threonine.
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85. FcRn binding dimer according to claim 84, wherein said linker has
a general formula selected from
(GnSm)p and (SnGm)p,
wherein, ndently,
n=1-7,
m=0-7,
n+ms8and
p=1-7.
86. FcRn binding dimer according to claim 85, wherein n = 1-5.
87. FcRn binding dimer according to any one of claims 85-86, wherein
m = 0-5.
88. FcRn binding dimer ing to any one of claims 85-87, wherein
p = 1-5.
89. FcRn binding dimer ing to any one of claims 86-88, wherein
n=4,m=1andp=1-4.
90. FcRn binding dimer according to claim 89, wherein said linker is
91. FcRn binding dimer according item 89, wherein said linker is G48
92. FcRn binding dimer according to any preceding item, which is
capable of binding to FcRn with at least 2 times, such as at least 3 times,
such as at least 4 times, such as at least 5 times, such as at least 6 times,
such as at least 7 times, such as at least 8 times, such as at least 9 times,
such as at least 10 times, such as at least 25 times, such as at least 50 times,
such as at least 100 times higher capacity than the corresponding first
monomer unit or second monomer unit alone.
93. FcRn binding dimer according to item 92, which is capable of
binding to FcRn at pH 6.0 with at least 2 times, such as at least 3 times higher
capacity than the corresponding first monomer unit or second monomer unit
alone.
94. FcRn binding dimer according to item 92, which is capable of
binding to FcRn at pH 7.4 with at least 2 times, such as at least 3 times, such
as at least 4 times, such as at least 5 times, such as at least 6 times, such as
at least 7 times, such as at least 8 times, such as at least 9 times, such as at
least 10 times higher capacity than the corresponding first r unit or
second monomer unit alone.
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95. FcRn binding dimer according to any preceding item, which is
capable of binding to FcRn at pH 6.0 such that the KB value of the interaction
is at most 1 X 10'7 M, such as at most 1 X 10'8 M, such as at most 1 X 10'9 M,
such as at most 1 X 10‘10 M, such as at most 1 X 10‘11 M, such as at most
1 x 10'12 M.
96. FcRn g dimer according to any preceding item, wherein the
KB value of the interaction between FcRn binding polypeptide and FcRn at pH
7.4 is higher than the K0 value of said interaction at pH 6.0, such as at least 2
times higher, such as at least 5 times higher, such as at least 10 times higher,
such as at least 50 times higher, such as at least 100 times higher than the
KB value of said interaction at pH 6.0.
97. FcRn g dimer according to any preceding item, wherein the
KB value of the interaction between FcRn binding polypeptide and FcRn at pH
7.4 is at least 1 X 10'10 M, such as at least 1 X 10'9 M, such as at least 1 X 10'8
M, such as at least 1 X 10'7 M, such as at least 1 X 10'6 M, such as at least
1 x 10'5 M.
98. FcRn binding dimer ing to any one of items 1-94, wherein
the KD value of said interaction at pH 7.4 is the same as or lower than the KD
value of said interaction at pH 6.0.
99. FcRn g dimer according to any one of items 1—94, n
the KB value of said interaction at pH 7.4 is at most 1 X 10'7 M, such as at
most 1 X 10'8 M, such as at most 1 X 10'9 M, such as at most 1 X 10'10 M, such
as at most 1 X 10'11 M, such as at most 1 X 10'12 M.
100. FcRn binding dimer according to any preceding item, wherein at
least one of said first and second monomer units comprises at least one
additional amino acid at the C-terminal and/or N-terminal end.
101. FcRn binding dimer according to item 100, wherein said at least
one additional amino acid extension improves or simplifies production,
purification, ization in vivo or in vitro, coupling or detection of the
polypeptide.
102. Fusion protein or conjugate sing
- a first moiety consisting of an FcRn binding dimer according to any
preceding item; and
- a second moiety consisting of a polypeptide having a desired
biological activity.
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103. Fusion protein or conjugate according to item 102, wherein the in
vivo half—life of said fusion protein or conjugate is longer than the in vivo half-
life of the polypeptide having a desired biological activity per se.
104. Fusion protein or conjugate according to any one of items 102-
103, wherein said d biological ty is a therapeutic activity.
105. Fusion protein or conjugate according to any one of items 100-
102, n said desired biological activity is a binding activity to a selected
target.
106. Fusion protein or conjugate according to item 105, wherein said
selected target is albumin.
107. Fusion protein or ate according to item 106, wherein said
albumin binding activity is provided by the albumin binding domain of
streptococcal protein G, or a derivative thereof.
108. Fusion protein or conjugate according to any one of items 106-
107, wherein said albumin binding activity increases in vivo half-life of the
fusion protein or conjugate.
109. Fusion protein or conjugate according to any one of items 103-
104, wherein said d biological activity is an tic activity.
110. Fusion protein or conjugate according to any one of items 103-
105, wherein the second moiety having a desired biological activity is a
therapeutically active polypeptide.
111. Fusion protein or conjugate according to any one of items 103-
105 and 109-110, wherein the second moiety having a desired biological
activity is selected from the group consisting of enzymes, hormones, growth
factors, chemokines and cytokines.
112. FcRn g dimer, fusion protein or conjugate according to any
preceding item, which inhibits g of lgG to FcRn.
113. FcRn binding dimer, fusion protein or conjugate ing to item
112, which binds FcRn such that the ability of the FcRn binding dimer to block
lgG binding to FcRn is at least 2 times higher, such as at least 3 times higher,
such as at least 4 times higher, such as at least 5 times higher, such as at
least 10 times, such as at least 15 times, such as at least 20 times, such as at
least 25 times higher ed to the blocking y of the corresponding
first or second monomer unit alone.
114. FcRn binding dimer, fusion protein or conjugate according to item
112 or 113, wherein the KB value of the interaction between said FcRn
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binding ptide, fusion protein or conjugate and FcRn is lower than the
KB value of the ction between lgG and FcRn.
115. FcRn g dimer, fusion protein or conjugate according to any
preceding item, further comprising a label.
116. FcRn binding dimer, fusion protein or conjugate according to item
115, n said label is selected from the group consisting of scent
dyes and metals, chromophoric dyes, chemiluminescent compounds and
bioluminescent proteins, enzymes, radionuclides and radioactive particles.
117. FcRn binding dimer, fusion protein or conjugate according to any
preceding item, comprising a chelating environment provided by a
polyaminopolycarboxylate chelator conjugated to the FcRn binding
polypeptide via a thiol group of a cysteine residue or an amine group of a
lysine residue.
118. FcRn binding dimer, fusion protein or conjugate according to item
117, wherein the polyaminopolycarboxylate chelator is 1,4,7,10-
tetraazacyclododecane-1,4,7,10-tetraacetic acid or a derivative thereof.
119. FcRn binding dimer, fusion protein or conjugate according to item
118, wherein the 1,4,7,10-tetraazacyclododecane-1,4,7,10-tetraacetic acid
derivative is 10-tetraazacyclododecane-1,4,7-tris-acetic 0-
maleimidoethylacetamide.
120. FcRn binding dimer, fusion protein or conjugate according to item
117, wherein the polyaminopolycarboxylate chelator is 1,4,7-
triazacyclononane-1,4,7-triacetic acid or a derivative f.
121. FcRn binding dimer, fusion protein or conjugate according to item
117, n the polyaminopolycarboxylate chelator is
diethylenetriaminepentaacetic acid or derivatives thereof.
122. A cleotide encoding a polypeptide according to any one of
items 1-114.
123. Expression vector comprising a polynucleotide according to item
122.
124. Host cell comprising an expression vector according to item 123.
125. Method of producing a polypeptide according to any one of items
1-114, comprising
- culturing a host cell according to item 124 under conditions
permissive of expression of said polypeptide from said expression vector, and
- isolating said polypeptide.
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126. Composition comprising an FcRn binding dimer, fusion protein or
conjugate according to any one of items 1-121 and at least one
pharmaceutically acceptable excipient or r.
127. Composition according to item 126, further comprising at least
one additional active agent.
128. Composition according to any one of items 126-127, which is
adapted for administration by a route selected from the group consisting of
oral administration, asal administration, pulmonar administration,
vaginal stration, rectal administration, intravenous injection,
intraperitoneal injection, uscular injection, subcutaneous ion and
intradermal ion.
129. FcRn binding dimer, fusion protein or conjugate according to any
one of items 1-121 or composition according to any one of items 126-128 for
use as a medicament.
130. FcRn binding dimer, fusion protein, conjugate or composition for
use ing to item 129, wherein said medicament is intended for treatment
or laxis of an auto-immune condition.
131. FcRn binding dimer, fusion protein, conjugate or composition for
use according to item 129, wherein said medicament is intended for treatment
or prophylaxis of an allo-immune condition.
132. FcRn binding dimer, fusion protein, conjugate or composition for
use according to item 129, wherein said medicament is intended for treatment
or prophylaxis of a condition selected from the group consisting of epilepsy
and seizures.
133. Method of treatment or prophylaxis of a subject in need thereof,
comprising administering to the t a therapeutically or prophylactically
active amount of an FcRn binding dimer, fusion protein or conjugate
according to any one of items 1-121 or composition ing to any one of
items 8.
134. Method according to item 133, for ent or prophylaxis of an
auto-immune condition.
135. Method according to item 133, for treatment or prophylaxis of an
allo-immune condition.
136. Method according to item 133, for treatment or prophylaxis of a
condition selected from the group consisting of epilepsy and seizures.
Claims (19)
1. FcRn binding dimer, sing a first monomer unit, a second monomer unit and an amino acid linker, wherein said first and second 5 monomer unit each comprises an FcRn binding motif BM, which motif consists of the amino acid sequence EX2 X3 X4 AX6 X7 EIR WLPNLX16X17 X18 QR X21 AFIX25 X26LX28 X29 10 wherein, independently from each other, X2 is selected from A, D, E, F, H, I, K, L, N, Q, R, S, T, V, W and Y; X3 is selected from A, D, E, F, G, H, I, K, L, M, N, Q, R, S, T, V, W and 15 X4 is selected from A, D, E, F, G, H, I, K, L, N, Q, R, S, T, V, W and Y; X6 is selected from A, E, F, G, H, I, K, Q, R, S and V; X7 is selected from A, F, H, K, N, Q, R, S and V; X16 is selected from N and T; X17 is selected from F, W and Y; 20 X18 is ed from A, D, E and N; X21 is selected from A, S, V and W; X25 is selected from D, E, G, H, I, K, L, N, Q, R, S, T, V, W and Y; X26 is ed from K and S; X28 is selected from D, E, F, H, I, K, L, N, Q, R, S, T, V, W and Y; and 25 X29 is selected from D and R, and wherein said FcRn binding dimer binds FcRn with a higher binding capacity compared to said first r or said second monomer alone. 30
2. FcRn binding dimer according to claim 1, wherein the BM of at least one of said first and second monomer units consists of an amino acid sequence selected from i) EX2 X3 X4 AX6 HEIR WLPNLTX17 X18 QR X21 AFIX25 KLX28 D wherein, independently from each other, X2 is selected from A, D, E, F, H, I, K, L, N, Q, R, S, T, V, W and Y; X3 is selected from A, D, E, G, H, K, L, M, N, Q, R, S, T, V and Y; X4 is ed from A, D, E, F, G, I, K, L, N, Q, R, S, T, V and Y; X6 is selected from A, G, K, R, S and V; 5 X17 is selected from F, W and Y; X18 is selected from A, D, E and N; X21 is selected from A, S, V and W; X25 is selected from D, G, H, K, L, N, R, V and W; X28 is selected from D, E, H, K, L, N, Q, R, S, T, W and Y; ii) an amino acid sequence which has at least 96 % identity to a sequence defined by i), ed that X28 is not A.
3. FcRn binding dimer according to any one of the preceding claims, wherein said first and second monomer units comprise identical BM ces. 20
4. FcRn g dimer according to any one of claims 1-2, wherein said first and second monomer units comprise different BM sequences.
5. FcRn g dimer according to any one of the preceding claims, wherein at least one of said first and second monomer units comprises an 25 FcRn binding motif BM ponding to the sequence from position 8 to position 36 in a sequence selected from the group consisting of SEQ ID NO:2-205, 207-306 and 308-353, such as the group consisting of SEQ ID NO:17-205, 207-306 and 308-352, such as the group consisting of SEQ ID NO:17-140, such as the group consisting of SEQ ID NO:17-92, SEQ ID 30 NO:94-103, SEQ ID NO:105-125 and SEQ ID NO:127-140, such as the group consisting of SEQ ID NO:19-20, SEQ ID NO:23, SEQ ID NO:28, SEQ ID NO:41, SEQ ID NO:44, SEQ ID NO:65, SEQ ID NO:70, SEQ ID NO:73, SEQ ID NO:75-77, such as the group consisting of SEQ ID NO:20, SEQ ID NO:23, SEQ ID NO:28, SEQ ID NO:41, SEQ ID NO:44, SEQ ID NO:65, SEQ ID 35 NO:73 and SEQ ID NO:75-77, such as the group consisting of SEQ ID NO:20, SEQ ID NO:23, SEQ ID NO:41, SEQ ID NO:44, SEQ ID NO:65, SEQ ID NO:75 and SEQ ID NO:77, such as the group consisting of SEQ ID NO:20, SEQ ID NO:23, SEQ ID NO:41, SEQ ID NO:44and SEQ ID NO:75, such as the group consisting of SEQ ID NO:20, SEQ ID NO:41 and SEQ ID NO:44.
6. FcRn binding dimer according to claim 5, wherein at least one of 5 said first and second monomer units comprises an FcRn g motif BM ponding to the sequence from position 8 to position 36 in a sequence selected from the group ting of SEQ ID NO:20, SEQ ID NO:23, SEQ ID NO:41, SEQ ID NO:44, SEQ ID NO:65, SEQ ID NO:75 and SEQ ID NO:77, such as the group consisting of SEQ ID NO:20, SEQ ID NO:23, SEQ ID 10 NO:41, SEQ ID NO:44, SEQ ID NO:65 and SEQ ID NO:75, such as the group consisting of SEQ ID NO:20, SEQ ID NO:41 and SEQ ID NO:44, such as SEQ ID NO:44.
7. FcRn binding dimer according to any one of the preceding claims, 15 wherein at least one of said first and second monomer units comprises a sequence selected from the group consisting of: xi) AEAKYAK-[BM]-DPSQSSELLSEAKKLNDSQAPK; xv) AEAKFAK-[BM]-DPSQSSELLSEAKKLSESQAPK; 20 xvii) VDAKYAK-[BM]-DPSQSSELLSEAKKLSESQAPK; wherein [BM] is an FcRn binding motif as defined in any one of claims 1-2; 25 an amino acid sequence which has at least 94% identity to the n of the sequence outside the [BM] defined in xi), xv) or xvii), provided that X28 in [BM] is not A.
8. FcRn binding dimer according to claim 7, wherein at least one of 30 said first and second monomer units comprises a sequence selected from the group consisting of SEQ ID NO:355-357 and SEQ ID -367, such as the group consisting of SEQ ID NO:357 and SEQ ID NO:360-367.
9. FcRn binding dimer according to claim 1 or 2, wherein at least one 35 of said first and second monomer units comprises a sequence selected from the group consisting of: xxi) VDAKYAK-[BM]-DPSQSSELLSEAKKLNDSQAPK; wherein [BM] is an FcRn binding motif as defined in any one of claims 1-2; xxii) an amino acid sequence which has at least 94% identity to the portion of the sequence outside the [BM] d in xxi), provided that X28 in [BM] is not A.
10 10. FcRn binding dimer according to claim 9, wherein at least one of said first and second monomer units comprises a sequence xxi) selected from the group ting of SEQ ID NO:2-205, 207-306 and 308-353, such as the group consisting of SEQ ID NO:17-205, 207-306 and 308-352, such as the group consisting of SEQ ID NO:17-140, such as the group consisting of SEQ 15 ID 92, SEQ ID NO:94-103, SEQ ID -125 and SEQ ID NO:127- 140, such as the group consisting of SEQ ID NO:19-20, SEQ ID NO:23, SEQ ID NO:28, SEQ ID NO:41, SEQ ID NO:44, SEQ ID NO:65, SEQ ID NO:70, SEQ ID NO:73, SEQ ID NO:75-77, such as the group consisting of SEQ ID NO:20, SEQ ID NO:23, SEQ ID NO:28, SEQ ID NO:41, SEQ ID NO:44, SEQ 20 ID NO:65, SEQ ID NO:73 and SEQ ID NO:75-77, such as the group consisting of SEQ ID NO:20, SEQ ID NO:23, SEQ ID NO:41, SEQ ID NO:44, SEQ ID NO:65, SEQ ID NO:75 and SEQ ID NO:77, such as the group consisting of SEQ ID NO:20, SEQ ID NO:41, SEQ ID NO:44 and SEQ ID NO:75, such as the group consisting of SEQ ID NO:20, SEQ ID NO:41 and 25 SEQ ID NO:44.
11. FcRn binding dimer according to claim 10, wherein at least one of said first and second monomer units comprises a sequence xxi) selected from the group consisting of SEQ ID NO:20, SEQ ID NO:23, SEQ ID NO:41, SEQ 30 ID NO:44, SEQ ID NO:65, SEQ ID NO:75 and SEQ ID NO:77, such as the group consisting of SEQ ID NO:20, SEQ ID NO:23, SEQ ID NO:41, SEQ ID NO:44, SEQ ID NO:65 and SEQ ID NO:75, such as the group consisting of SEQ ID NO:20, SEQ ID NO:41 and SEQ ID NO:44, such as SEQ ID NO:44. 35
12. FcRn g dimer according to claim 8, wherein said first and second monomer units comprise SEQ ID NO:365 and SEQ ID NO:365; SEQ ID NO:366 and SEQ ID ; or SEQ ID NO:367 and SEQ ID NO:367, respectively.
13. FcRn binding dimer according to any one of the preceding claims, 5 wherein said linker has a general formula selected from (GnSm)p and p, wherein, independently, n = 1-7, m = 0-7, 10 n + m ≤ 8 and p = 1-7.
14. FcRn binding dimer according to any one of the preceding claims, which is capable of binding to FcRn with at least 2 times, such as at least 3 15 times, such as at least 4 times, such as at least 5 times, such as at least 6 times, such as at least 7 times, such as at least 8 times, such as at least 9 times, such as at least 10 times, such as at least 25 times, such as at least 50 times, such as at least 100 times higher capacity than the corresponding first monomer unit or second monomer unit alone.
15. Fusion protein or conjugate comprising - a first moiety consisting of an FcRn g dimer according to any one of the preceding claims; and - a second moiety consisting of a polypeptide having a desired 25 biological activity.
16. FcRn binding dimer, fusion n or conjugate according to any one of the preceding claims, which inhibits binding of IgG to FcRn. 30
17. FcRn binding dimer, fusion protein or conjugate according to claim 16, which binds FcRn such that the ability of the FcRn binding dimer to block IgG binding to FcRn is at least 2 times higher, such as at least 3 times higher, such as at least 4 times higher, such as at least 5 times higher, such as at least 10 times, such as at least 15 times, such as at least 20 times, such as at 35 least 25 times higher compared to the ng ability of the corresponding first or second monomer unit alone.
18. Composition comprising an FcRn binding dimer, fusion protein or conjugate according to any one of the preceding claims and at least one pharmaceutically acceptable ent or carrier. 5
19. Use of a FcRn binding dimer, fusion protein or conjugate according to any one of claims 1-17 in the manufacture of a medicament for the treatment or laxis of a condition selected from the group consisting of auto-immune conditions, allo-immune conditions, epilepsy and seizures. 1 /38 2015/071339 9%: dEmmOmmflfl<_-MT| m<>mOQMU .L/m. EE<¢ <DOEM<WV flflmzznmv JZmJBMHmflw<DMQHM<WM<fl soapmcmamwn mamwom (V) OWOOOMI—IOW I_I KO [\OWC\ L0 1— OW OKOV‘MOOI—IQ <I" L0 NOLO W KO I \l®\lm\l\l\ \ I \ mow \ I \ Ol\Ol\ OO O O [\ O O O IO\IO\. |\ \ I x \IO \ \ I x NNN L\_ N N N L\_ N WO 42083
Applications Claiming Priority (3)
| Application Number | Priority Date | Filing Date | Title |
|---|---|---|---|
| EP14185140 | 2014-09-17 | ||
| EP14185140.2 | 2014-09-17 | ||
| PCT/EP2015/071339 WO2016042083A1 (en) | 2014-09-17 | 2015-09-17 | New polypeptides |
Publications (2)
| Publication Number | Publication Date |
|---|---|
| NZ729218A NZ729218A (en) | 2021-02-26 |
| NZ729218B2 true NZ729218B2 (en) | 2021-05-27 |
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