US20140121358A1

US20140121358A1 - Humanized antibody and process for preparing same

Info

Publication number: US20140121358A1
Application number: US13/653,481
Authority: US
Inventors: Hyo Jeong Hong; Cheol Young Maeng; Gi Hyeok Yang; Meong Hee Jang; Mee Sook OH; Jin Soo Song; Young Kug Jang
Original assignee: Aprogen, Inc.
Current assignee: Aprogen Inc
Priority date: 2002-03-22
Filing date: 2012-11-15
Publication date: 2014-05-01
Also published as: AU2003210060A1; EP1532175B1; CN1656121A; EP1532175A1; EP1532175A4; KR20040095291A; AU2003210060B2; CA2492671A1; CN1305905C; US20070021595A1; US8420353B2; CA2492671C; KR100708398B1; WO2003080672A1

Abstract

A humanized antibody is produced by process comprising the steps of: (a) selecting a specificity determining residue (SDR) of the complementarity determining region (CDR) of murine monoclonal antibody heavy chain and light chain variable regions; and (b) grafting said SDR to at least one of the corresponding amino acid sequences in human antibody variable regions.

Description

FIELD OF THE INVENTION

The present invention relates to a process for preparing a humanized antibody by grafting SDRs (specificity determining residues) in CDRs (complementary determining residues) of murine monoclonal antibody to human antibody and the humanized antibody prepared according to said process.

BACKGROUND OF THE INVENTION

For preventing infectious diseases such as hepatitis B, there has generally been used a method of administering immunoglobulins formed in blood plasma against a target antigen. However, the method has the problems that the immunoglobulins generally have low specificity and may contain contaminants.
Murine monoclonal antibody derived from mouse has been reported to have high affinity to antigen and is suitable for mass-production. However, repeated injection of murine monoclonal antibody induces an immune response because the murine antibody is regarded as a foreign antigen in humans (Shawler D. L. et al., J. Immunol., 135, 1530-1535 (1985)).
Accordingly, numerous efforts have been made to generate “humanized antibody” by: grafting the CDR (complementarity determining region) of murine monoclonal antibody variable region which directly binds to antigens, to a human antibody framwork (CDR-grafting method); and replacing the amino acid residues of the human antibody framework region (FR) that influence the CDR conformation with the amino acid residues of murine monoclonal antibody. The humanized antibody thus obtained maintains the affinity and specificity of original murine monoclonal antibody, and minimizes HAMA(human anti-mouse antibody) response in humans (Riechmann et al., Nature, 332, 323-327 (1988); Queen C. et al., Proc. Natl. Acad. Sci. USA, 86, 10029-10033 (1989); Nakatani et al., Protein Engineering, 7, 435-443 (1994)). However, this humanized antibody still causes problems when injected repeatedly into humans (Stephens et al., Immunology, 85, 668-674 (1995); Sharkey et al., Cancer Research, 55, 5935s-5945s(1995)).
Approximately 300 millions of world population carry hepatitis B virus (“HBV”) which may cause chronic infection, leading to cirrhosis and hepatocellular carcinoma (Tiollais P. and Buendia M. A., Sci. Am., 264, 48 (1991)). The HBV envelope consists of three proteins, major protein containing S antigen, middle protein containing S and pre-S2 antigens, and large protein containing S, pre-S2 and pre-S 1 antigens (Neurath A. R. and Kent S. B., Adv. Vir Res., 34, 65-142 (1988)). These surface antigens have been known to play important roles in the process of forming antibodies against HBV in hepatitis patient. The pre-S1 region, in particular, is found on infectious viral particles (Heermann et al., J. Viral., 52, 396-402 (1984)) and plays a role in attachment to cell surface infection (Neurath et al., Cell, 46, 429 (1986); Pontisso et al., Viral., 173, 533, (1989); Neurath et al., Vaccine, 7, 234 (1989)). Thus a monoclonal antibody against the pre-S1 would be effective against viral infection.
The present inventors have previously reported a murine monoclonal antibody (KR127) against HBV pre-S1 (Korean Patent No. 246128), a murine monoclonal antibody KR127 gene encoding same (Korean Patent No. 250832) and a humanized antibody (HZKP 1271) of KR127 prepared by CDR-grafting method (Korean Patent No. 246128).
The present inventors have further endeavored to develop a humanized antibody having minimized adverse immune response (HAMA response) as well as enhanced affinity to antigen, and found that HAMA response can be reduced when the amino acid residues of CDR of mouse antibody are replaced with those of human antibody.

SUMMARY OF THE INVENTION

Accordingly, it is an object of the present invention to provide a process for preparing a humanized antibody which is expected to show lower HAMA response and has higher affinity than humanized antibody of the prior art.
It is another object of the present invention to provide a humanized antibody prepared according to said process.
It is a further another object of the present invention to provide a DNA encoding the heavy chain or light chain of said antibody and a vector 35 comprising said DNA.
It is a still further object of the present invention to provide a microorganism transformed with said vector.
In accordance with one aspect of the present invention, there is provided a process for preparing a humanized antibody comprising the steps of (a) selecting a specificity determining residue (SDR) of the complementarity determining region (CDR) of murine monoclonal antibody heavy chain and light chain variable regions; and (b) grafting the amino acid residues of said SDR to at least one of the corresponding amino acid sequences in human antibody variable regions.

BRIEF DESCRIPTION OF THE DRAWINGS

The above and other objects and features of the present invention will become apparent from the following description of the invention taken in conjunction with the following accompanying drawings; which respectively show:

FIG. 1: the procedure for constructing an expression vector of a chimeric heavy chain;

FIGS. 2A, 2B and 2C: collectively teach the nucleotide and amino acid sequence of the humanized 20 heavy chain variable region;

FIG. 3: the procedure for constructing an expression vector of a chimeric light chain;

FIGS. 4A and 4B: the nucleotide and amino acid sequence of the humanized light chain variable region;

FIG. 5: the affinity to antigen of a humanized antibody having a heavy chain CDR mutant;

FIG. 6: the procedure for constructing an expression vector of the humanized antibody; and

FIG. 7: is a plot showing the results of analysis for MHC class II-binding peptide sequences in heavy chain variable regions of HuKR127 and light chain variable regions of HuKR127, respectively.

DETAILED DESCRIPTION OF THE INVENTION

The humanized antibody of the present invention may be prepared by grafting the amino acid residues of SDR of murine monoclonal antibody to the corresponding amino acid sequences in human antibody variable regions.
SDRs of the murine monoclonal antibody used in the present invention may be determined by independently replacing each amino acid residue of CDR of the murine monoclonal antibody with alanine, selecting transformants which have lower affinity (k_D) to antigen than the original murine antibody and determining the replaced CDR amino acid residues of said transformants as SDRs.
Further, in order to enhance the affinity to antigen, the CDR residues of a mouse antibody that increase the affinity and the framework residues that influence the conformation of CDR loops may also be grafted to the corresponding sites of human antibody.
For example, the present invention describes a process for preparing a humanized antibody for hepatitis B virus (HBV) pre-S1 by using murine monoclonal antibody KR127 (Korean Patent No. 250832) as follows:
After selecting SDR amino acid residues, which play important roles in binding with antigen, from CDR of the murine monoclonal antibody KR127 heavy and light chains, chimeric heavy chain and chimeric light chain genes may be prepared by combining either the variable region of ICR127 antibody heavy chain with the constant region (C₁1) of human antibody or the variable region of KR127 antibody light chain with the constant region (CO of human antibody.
SDRs of the murine monoclonal antibody for HBV pre-S 1 are determined by replacing each amino acid residue of CDR HCDRI (aa 31-35), HCDR2 (aa 50-65) and HCDR3 (aa 95-102) of the heavy chain (SEQ ID NO: 2) and CDR LCDR1 (aa 24-34), LCDR2(aa 50-56) and LCDR3(aa 89-97) of the light chain (SEQ ID NO: 4) of the murine monoclonal antibody KR127 with alanine according to the alanine scanning mutagenesis method and selecting the amino acid residues (SDRs) whose replacement with alanine bring about more than 3 times reduction in the affinity to antigen(KD) as compared with the original murine antibody. Throughout this description, amino acid residue number is assigned according to Kabat numbering scheme (Kabat, E. A. et al, Sequences of Proteins of Immunological Interest. National Institute of Health, Bethesda, Md., 1991).
Examples of preferred SDR include tryptophan at position 33 (it is represented as “Trp33”), Met34, and Asn35 of HCDR1; Arg50, Tyr52, and Pro52a of HCDR2; Glu95, Tyr96, and Glu98 of HCDR3 of the murine monoclonal antibody KR127 heavy chain; Leu27b, Tyr27d, Ser27e; Asn28, Lys30, Tyr32, and Asn34 of LCDR1; Leu50 and Asp55 of LCDR2; and Va189, Gln90, Gly91, Thr92, His93, Phe94, Pro95, and Gln96 of LCDR3 of the murine monoclonal antibody KR127 light chain.
The humanized antibody of the present invention can be prepared by grafting one. or more SDRs determined as above onto the human antibody heavy chain and/or light chain. The human antibody heavy chain which may be used in the present invention is human heavy chain DP7-JH4 consisting of human immunoglobulin germline VH gene segment DP7 (Tomlinson et al., J. Mol. Biol., 227, 776-798, 1992) and JH4 segment (Ravetch et al., Cell, 27, 583-591, 1981). The human antibody light chain which may be used in the present invention is human light chain DPK12-JH4 consisting of human immunoglobulin germline VK gene segment DPK12 (Cox et al., Eur. J. Irnmunol., 24, 827-836 (1994)) and JH4 segment (Hieter et al., J. Biol. Chem., 257, 1516-1522 (1982)).
The humanized heavy chain of the present invention may be prepared by grafting at least one of Trp33, Met34, and Asn35 of HCDR1; Arg50, Tyr52, and Pro52a of HCDR2; Glu95, Tyr96, and Glu98 of HCDR3 of the murine monoclonal antibody KR127 heavy chain to the corresponding amino acid sequences in human antibody heavy chain. The inventive humanized light chain may be prepared by grafting at least one of Leu27b, Tyr27d, Ser27e; Asn28, Lys30, Tyr32, and Asn34 of LCDR1; Leu50 and Asp55 of LCDR2; and Va189, Gln90, Gly91, Thr92, His93, Phe94, Pro95, and Gln96 of LCDR3 of the murine monoclonal antibody KR127 light chain to the corresponding amino acid sequences in human antibody light chain DPH1241(4.
Moreover, the affinity to antigen of the humanized antibody can be enhanced by the follow substitutions:
(a) the amino acid residue at position 32 in HCDR1 of the modified human heavy chain DP7-JH4 by Ala;
(b) the amino acid residue at position 97 in HCDR3 of the modified human heavy chain DP7-JH4 by Arg or Ala;
(c) the amino acid residue at position 98 in HCDR3 of the modified human heavy chain DP7-JH4 by Val; and
(d) the amino acid residue at position 102 in HCDR3 of the modified human heavy chain DP7-3H4 by Arg or Ala.
In addition, Ala71 and Lys73 in framework region 3 in the heavy chain variable region of KR127, which affects the conformation of the CDR loop, may further be grafted to human heavy chain DP7-JH4. Also, Leu36 and Arg46 in framework region 2 in the light chain variable region of KR127, which affects conformation of CDR loop, may be further grafted to human light chain DPH12-3K4.
The heavy chain variable region of humanized antibody of the present invention has the amino acid sequence of SEQ ID NO: 2, preferably encoded by the nucleotide sequence of SEQ ID NO: 1 and the inventive light chain variable region of humanized antibody has the amino acid sequence of SEQ ID NO: 4, preferably encoded by the nucleotide sequence of SEQ ID NO: 3.
The humanized antibody heavy chain and light chain of the present invention may be encoded by a gene comprising a nucleotide sequence deduced from the humanized antibody heavy chain and light chain according to the genetic code. It is known that several different codons encoding a specific amino acid may exist due to the codon degeneracy, and, therefore, the present invention includes in its scope all nucleotide sequences deduced from the humanized antibody heavy chain and light chain amino acid sequence. Preferably, the humanized antibody heavy chain and light chain gene sequences include one or more preferred codons of host cell.
The humanized antibody consisted of the humanized heavy chain HuKR127HC of the present invention and humanized light chain HZKR127I prepared by CDR-grafting has an affinity to antigen of about over 50 times higher than that of the humanized antibody HZKR1271.
The humanized antibody consisting of the humanized heavy chain HuKR127KC of the present invention and humanized light chain HZKR127I prepared by CDR-grafting has an affinity to antigen equal to that of the humanized antibody HZICR127I.
The genes of humanized antibody heavy chain and light chain thus prepared may be inserted to pdCMV-dhfrC-HAV6 vector (KCTC 10028BP) to obtain an expression vector pdCMV-dhfrC-HuKR127 which can express both humanized antibody heavy chain HuKR127HC and light chain HZKR127I. The expression vector of the present invention may be introduced into microorganism, e.g., E. coli DH5a according to a conventional transformation method to obtain transformants E. coli DH5a/pdCMV-dhfrC-HuKR127. The transformants E. coli DH5a pdCMVdhfrC-HuKR127 was deposited on Mar. 13, 2002 with the Korean Collection for Type Cultures(KCTC)(Address: Korea Research Institute of Bioscience and Biotechnology(KRIBB), #52, Oun-dong, Yusong-ku, Taejon, 305-333, Republic of Korea) under the accession number, KCTC 10198BP, in accordance with the terms of Budapest Treaty on the International . . . Recognition of the Deposit of Microorganism for the Purpose of Patent Procedure.
Meanwhile, CHO/HuKR127, CHO (Chinese hamster ovary) cell line transfected with vector pdCMV-dhfrC-HuKR127, was deposited on Mar. 13, 2002 with the Korean Collection for Type Cultures(KCTC) under the accession number, KCTC 10199BP, in accordance with the terms of Budapest Treaty on the International Recognition of the Deposit of Microorganism for the Purpose of Patent Procedure.
The humanized antibody HuKR127 of the present invention produced by culturing the CHO/HuKR127 cell line has a higher affinity to antigen and is expected to reduce HAMA (human anti-mouse antibody) response to a greater extent than the conventional antibody prepared according to the CDR-grafting method.
Accordingly, the humanized antibody of the present invention can be used in preventing hepatitis B virus infection and treating chronic Hepatitis B.
Thus, for preventing hepatitis B virus infection and treating chronic Hepatitis B, a pharmaceutical formulation of the inventive humanized antibody may be prepared in accordance with any of the conventional procedures.
The pharmaceutical composition of the present invention can be administered via various routes including intravenous and intramuscular introduction. It should be understood that the amount of the active ingredient actually administered ought to be determined in light of various relevant factors including the condition to be treated, the chosen route of administration, the age, sex and body weight of the individual patient, and the severity of the patient's symptom; and, therefore, the above dose should not be intended to limit the scope of the invention in any way.
The following Examples are intended to further illustrate the present invention without limiting its scope.

Example 1

Preparation of Mouse/Human Chimeric Heavy Chain Gene

The gene encoding leader sequence and the yl constant region of the human antibody heavy chain were separately prepared by carrying out PCR using pCMV-HKR127HC (Korean Patent No. 246128, KCTC 0531BP) as a template and a primer set of Ryu94 (SEQ ID NO: 5) and HUR43-1 (SEQ ID NO: 6) or HUR46-1 (SEQ ID NO: 9) and HUR31 (SEQ ID NO: 10). The gene encoding heavy chain variable region of the murine monoclonal antibody KR127 was prepared by carrying out PCR using pKR127H (Korean. Patent No. 250832, KCTC 0333BP) as a template and primers HUR44-1 (SEQ ID NO: 7) and HUR45-1 (SEQ ID NO: 8).

Ryu94:

5′-GAG AAT TCA CAT TCA CGA TGT ACT TG-3′

HUR43-1:

CTG CAG CTG GAC CTG ACT CTG GAC ACC ATT-3′

HUR44-1:

5′-CAG GTC CAG CTG CAG CAG TCT GGA CCT GAA CTG-3′

HUR45-1:

5′-TGG GCC CTT GGT GGA GGC TGC AGA GAC AGTGAC-3′

HUR46-1:

5′-GCC TCC ACC AAG GGC CCA TCG GTC TTC CCC CTG-3′

HUR31:

5′-CAG CGG CCG CTC ATT TAC CCG GGG ACA G-3′

Each PCR reaction was carried out using 10 ng of template, 1 ie of each primer (50 ppm), 0.5 p.t of _PfuDNA polymerase (Promega), 4 a of 2.5 mM dNTPmix and 5, ull of 10×Pfu reaction buffer solution. After pre-denaturation at 95 t for 5 minutes, a PCR cycle was repeated 25 times, the cycle being composed of 95 t for 30 sec., 50° C. for 30 sec. and 72° C. for 45 sec. After annealing the DNA fragment obtained by using primers Ryu94 and HUR43-1, the DNA fragment obtained by using primers HUR44-1 and HUR45-1, and the DNA fragment obtained by using primers HUR46-1 and HUR31 were recombined by conducting recombinant PCR using primers Ryu94 and HUR31. The recombinant PCR reaction was carried out using the same reaction buffer solution as used above. After pre-denaturation at 95 t for 5 minutes, a PCR cycle was repeated 30 times, the cycle being composed of: 95 t for 30 sec., 50t for 30 sec. and 72 t for 60 sec., and finally, the extension reaction was carried out at 72 t for 5 min.
The chimeric heavy chain gene thus prepared was cleaved with EcoRI (GAATTC) and Ndel (GCGGCCGC) and inserted at the EcoRTINdel section of vector pcDdA (plasmid which is removed Apal site in the multiple cloning site of pcDNA received from Invitrogen), to obtain, vector pcDdAchKR127HC (FIG. 1). The base sequence of the chimeric heavy chain variable region gene (KR127VH) was confirmed by DNA sequence analysis (FIG. 2).

Example 2

Preparation of Mouse/Human Chimeric Light Chain Gene

The gene encoding reader sequence and the constant region of the human antibody light chain were each prepared by carrying out PCR using pKC-dhfr-FIKR127 (Korean Patent No. 2000-33008, KCTC 0529BP) as a template and a primer set of Ryu86 (SEQ ID NO: 11) and HUR48 (SEQ ID NO: 12) or HUR51 (SEQ ID NO: 15) and CK1D (SEQ ID NO: 16).
The gene encoding light chain variable region of the murine monoclonal antibody KR127 was prepared by carrying out PCR using pKR127K (Korean Patent No. 250832, KCTC 0334BP) as a template and primers HUR49 (SEQ ID NO: 13) and HUR50 (SEQ ID NO: 14).

	Ryu86:
	5′-CAA AGC TTG GAA GCA AGA TGG ATT CA-3′

	HUR48:
	5′-CAA GAT ATC CCC ACA GGT ACC AGA TAC-3′

	HUR49:
	5′-TGT GGG GAT ATC TTG ATG ACC CAA ACT-3′

	HUR50:
	5′-CAC AGA TCT TTT GAT TTC CAG CTT GGT-3′

	HUR51:
	5′-ATC AAA AGA TCT GTG GCT GCA CCA TCT-3′

	CK1D:
	5′-GCG CCG TCT AGA ATT AAC ACT CIC CCC TGT TGA

	AGC TCT TTG TGA CGG GCG AACTCAG-3′

Each PCR reaction was carried out according to the method described in Example 1 except that primers Ryu86 and CK1D were used to ligate the annealed DNA fragments obtained by PCR reactions.
The chimeric light chain gene thus prepared was cleaved with HindlII (AAGCTT) and Xbal (TCTAGA) and inserted at the HindMIXbal section of vector pBluescript KS, to obtain a recombinant plasmid. Subsequently, the recombinant plasmind was cleaved with Hindilll and Apal and inserted at the HindlrII Apal section. of vector pCMV-dhfr (KCTC 8671P), to obtain plasmid pKC-dhfr-chKR127 (FIG. 3). The base sequence of the chimeric light chain varible region gene (KR127VK) was confirmed by DNA sequence analysis (FIG. 4).

Example 3

Mutation of CDR. of Chimeric KR127 Antibody Heavy Chain by Alanine Injection

To examine whether each amino acid residue of KR127 heavy chain HCDR1 (aa 31-35), HCDR2(aa 50-65) and HCDR3 (aa 95-102) binds to antigen, PCR reaction was carried out using vector pcDdA-chKR127HC as a template to prepare a modified gene, wherein an amino acid residue of CDR was replaced with alanine (the replaced amino acid residue No. was indicated as Kabat number) (see FIG. 2).
A forward primer YMOO1N of SEQ ID NO: 17 was designed to provide the sequence corresponding to the reader sequence at the 5′-end of the chimeric heavy chain gene and EcoRI restrition site, and a reverse primer YM003 of SEQ ID NO: 18 was designed to have the sequence corresponding to the N-terminal downstream of CH1 domain of human heavy chain gene and Apal restriction site.

	YMOO1N:
	5′-CCG GAA TTC ACA TTC ACG ATG TAC TTG-3′

	YM003:
	5′-TGC CCC CAG AGG TGC T-3′

The 5′-end primer ym257 of SEQ ID NO: 19 (corresponding to nucleotide Nos. 80 to 112 of SEQ ID NO: 1) was designed to replace Ser31 of HCDR1 with alanine (S31A) and the 3′-end primer YM258 of SEQ ID NO: 20 (corresponding to nucleotide Nos. 101 to 71 of SEQ ID NO: 1), to replace AGT (coding for Ser) of nucleotide Nos. 91 to 93 of HCDRI gene with GCT (coding for alanine).
Each PCR reaction was carried out according to the method described in Example 1 except that primer sets, YMOO1N and YM258; and ym258 and YM003, were used and also that primers YMOO1N and YM003 were used to recombine the annealed DNA fragments obtained by PCR.
The chimeric light chain gene thus prepared was cleaved with EcoRI and Apal and inserted at the EcoRTIApal section of vector pcDdA-chICR127HC prepared in Example 1, to obtain peDdA-chICR127HC-S31A. The base sequence of the humanized antibody heavy chain variable region gene was confirmed by DNA sequence analysis. Vectors containing mutants thus prepared are shown in Table 1.
In Table 1, primer and mutation positions are numbered based on the base sequence of SEQ ID NO: 1.

TABLE 1

	primer	mutation

CDR

primer

position

mutant

vector

	F	ym257	80-112	91-93	S er CACTI-?+0
	R	YM258	101-71	Ala(GCT)		pcDdA-chICR127HC-S31A
	F	yrn259	83-112	Sre CTCT1-?+0
	R	YM260	106-73	94-96	Ala(GCT)	pcDdA-chKR127HC-S32A
	F	ym261	86-117	Trp(TGG)-		pcDdA-chKR127HC-1Y33A
HCDR1	R	YM262	108-76	97-99	Ala(GCG)
	F	ym263	90-118	Met(ATCF)-
	R	YM264	111-79	100-102	Al a(GCG)	pcDdA-chKR127HC-M33A
	F	ym265	94-120	Asn(AAC)-
	R	ym266	112-81	103-105	Ala(GCC)	pcDdA-chKR127HC-N35A
	F	YIV1221	139-174	Arg(CGG)-′		pcalA-chICR.127HC-R50A
	R	YM222	158-128	148-150	Ala(GCC)
	F	YM225	143-178	151-153	I I e(A 1 1)-	pcDdA-chKR127HC-I 51A
	R	YM226	162-131	Ala(GCT)
	F	YM227	145-180	Tvr CT′AT)-
	R	YM228	165-135	154-156	Ala(GCT)	pcDdA-chKR127HC-Y52A
	F	ym229	148_181	Pri-dn′T 1-?+0
	R	YM230	167-136	157-159	AI a(GCT)	pcDdA-chICR127HC-P52aA
	F	ym231	150-186	G lv(GGA)-
	R	YM232	173-145	160-162	A 1 a(GCA)	pcDdA-chICR127HC-G53A
HCDR2	F	vm233	152-188	Asn(C1AT4-
	R	YM234	176-144	163-165	Ala(GCT)	pcDdA-chKR127HC-D54A
	F	ym235	155-193	Glv(GGA)-?+0
	R	YM236	178-146	166-168	A Ia(GCA)	peDdA-chKR127HC-G55A
	F	ym2 3 7	158-194	A cn(GAT′-?+0
		ym238	184-149	169-171	A I a(GCT)	pcDdA-chKR127HC-D56A
	F	ym239	160-195	Thr(M. 1 ′1-
	R	ym240	185-150	172-174	A 1 a(GCT)	pcDdA-chICR127HC-T57A
	F	yrn241	164-196	Acn(A AC1-
	R	ym242	187-150	175-177	Ala(GCC)	pcDdA-ch1CR127HC-N58A
	F	YM207	286-317	Glu(GAG1-
	R	YM208	305-274	295-297	A 1 a(GCG)	pcDdA-chICR127HC-E95A
	F	YN1209	289-316	Tvr(TAC′.)-.
	R	YNI210	307-276	298-300	A 1 a(GCC)	pcDdA-chKR127HC-Y96A
	F	YM211	292-318	Asn(GAC)-?+0
HCDR1	R	YN1217	111-279	Al a CGCG)
	F	YM213	296-321	Gln(CIAG)-.
	R	YM214	315-285	304-306	A I a(GCG)	pcDdA-chKR127HC-E98A
	F	YM255	303-327	Tvr(TAO-.
	R	YM256	319-289	310-312	Ala(GCC)	peDdA-chKR127HC-Y102A

Test Example 1

Expression of Chimeric Antibody Having a Modified Heavy Chain and its Affinity to Antigen

(Step 1) Expression of Chimeric Antibody

COS7 cells (ATCC CRL-1651) were seeded to DMEM media (GIBCO) containing 10% bovine serum and subcultured in an incubator at 37° C. under an atmosphere of 5% CO₂. 1×10⁶cells thus obtained were seeded to the same media and incubated at 37° C. overnight. Thus, 5 lig of plasmid pICC-dhfr-chKR.127 (expressing chimeric light chain) obtained in Example 2, 5 jig of plasmid obtained in Example 3 were diluted with OPTI-1VLEMAGLBCO) to 800 ge. 50 of Lipofectamine (GIBCO) were diluted with the same solution to 800 _Ia. The resulting solutions were added to a 15 rae tube, mixed and then, kept at room temperature for more than 15 minutes. Meanwhile, COS7 cells incubated as above were washed three times with OPTI-MEM I. Then, 6.4 me of OPTI-MEM I was added to the DNA-Lipofectamine mixture and the resulting solution was evenly distributed on the COS7 cells, which were cultured for 48 hours in a 5% CO₂incubator to obtain a supernatant. The resulting solution was subjected to sandwich ELISA analysis using anti-human IgG (Sigma) as a capture antibody and anti-human antigen (Fc-specific)-horseradish peroxidase (PIERCE) as a secondary antibody to confirm the expression of the chimeric antibody.
(step 2) Affinity to Antigen
150 ng of HBV recombinant antigen GST-pre-S1(1-56) (H. S. Kim and H. 3. Hong, Biotechnology Letters, 17, 871-876 (1995)) was coated to each well of a microplate and 5 ng of the supernatant obtained in Step 1 was added to each well. The resulting solution was subjected to indirect ELISA using the same secondary antibody as used in step 1, followed by measuring the absorbance at 450 nm. Further, the affinity to antigen (K_D) of each modified heavy chain was determined by competitive ELISA method (Ryu et al., J. Med. Viral., 52, 226 (1997)) and compared with that of pCK-dhfr-chKR.127 containing wildtype chimeric heavy chain. The result is shown in Table 2.

TABLE 2

		KD
CDR	Mutant	(nM)

	WT	11.0 ± 1.664
ii1	S31A	14.67 ± 2.386
	S32A	8.455 ± 0.840
	W33A	>10000
	M34A	>10000
	N35A	>10000
H2	R50A	>10000 •
	I51A	12.8 ± 1.05
	Y52A	276.8 ± 23.60
	P52aA	170.3 ± 5.318
	G53A	7.697 ± 0.980
	D54A	1.663 ± 0.477
	G55A	5.766 ± 0.211
	D56A	6.59 ± 1.09
	T57A	13.68 ± 4.016
	N58A	1.568 ± 0.085
H3	E95A	• >10000
	Y96A	>10000
	D97A	0.57 ± 0.03
	E98A	64.2 ± 7.78
	Y102A	3.581 ± 0.457

As shown in Table 2, the affinities to antigen of the mutants obtained by replacing Trp33, Met34, or Asn35 of HCDR1; Arg50, Tyr52, or Pro52a of HCDR2; Glu95, Tyr96, or Glu98 of HCDR3 with alanine were more than 3 times lower than that of wild type. However, a mutant having alanine substituting for Asp97 or Tyr102 residue of HCDR3 exhibited an enhanced affinity to antigen.

Example 4

Preparation of HCDR3 Mutants and Their Affinities to Antigen

(step 1) D97R and E98V Mutants
Each mutant was prepared by replacing Asp97 or Glu98 of HCDR3 with arginine as a positively charged amino acid (it is represented as “D97R”) or valine as a neutral amino acid (it is represented as “E98V”) according to the site-directed mutagenesis as used in Example 3. Vectors containing mutants prepared as above are shown in Table 3.

TABLE 3

			mutation
CDR	primer	position	position	mutant	vector

HCDR3	R	P1	312-279	301-303	Asp(GAC)→	pcDdA-chKR127HC-D97R
	F	P2	295-326		Arg(CGG)

	R	PC	312-279	301-303	Asp(GAC)→	pcDdA-chKR127HC-D97V
	F	P4	295-326		Val(GTT)

	R	P5	312-279	304-306	Glu(GAG)→	pcDdA-chKR127HC-E98R
	F	P6	295-326		Arg(CGG

	R	P7	312-297	304-306	Glu(GAG)→	pcDdA-chKR127hc-E98V
	F	P8	295-326		Val(GTT)

Then, each mutant thus obtained was measured for its affinity to antigen in according to the method described in Test Example 1 and compared with that of the wild type.
As shown in FIG. 5, the affinity to antigen of D97R was more than 3 times higher than that of the wild type, which the affinity to antigen of E98V, more than 4 times higher than that of the wild type. However, mutant E98R showed a low affinity to antigen.

(Step 2) D97R/E98V Mutant

To prepare D97R/E98V mutant containing both D97R and E98V, which were found to be mutants having high affinity to antigen, PCR reaction was carried out using pcDdA-chICR127HC-D97R which contains D97R gene as a template and primers P7 and P8.
Then, the D97R/E98V mutant thus obtained was measured for its affinity to antigen in according to the method described in Test Example 1.
As shown in FIG. 5, the affinity to antigen of D97R/E98V was more than 15 times higher than that of the wild type.

(Step 3) D97R/E98V/Y102A Mutant

To prepare D97R/E98V/Y102A mutant containing D97R, E98V and Y102A, PCR reaction was carried out using pcDdA-chICR127HC-RV containing D97R/E98V as a template and primers YM255 and YM256.
Then, the D97R/E98V/Y102A mutant (hereinafter “RVAA”) thus obtained was measured for its affinity to antigen in according to the method described in Test Example 1.
As shown in FIG. 5, the affinity to antigen of D97R/E98V/Y102A was similar to that of D97R/E98V.
(Step 4) D97R/E98V/Y102E and D97R/E98V/Y102R mutants
To prepare D97R/E98V/Y102E mutant and D97R/E98V/Y102R mutant, PCR reaction was carried out using pcDdA-chKR127HC-RV containing D97R/E98V as a template, and primer sets P17/P18 and P19/P20, respectively.
Vctor containing mutants prepared above are shown in Table 4.

TABLE 4

		primer	mutation
	primer	position	postion	mutant	vector

HCDR3	R	P17	312-279	307-309	TYr(TAC)-	pcDdA-chKR12711C-RVAE
	F	P18	295-326		Glu(GAG)

	R	P19	312-279	307-309	TYr(TAC)-	pcDdA-chKR127HC-RVAR
	F	P20	295-326		Arg(CGT)

Then, D97R/E98V/Y102E mutant (hereinafter “RVAE”) and D97R/E98V/Y102R mutant (hereinafter “RVAR”) thus obtained were measured for respective affinities to antigen in according to the method described in Test Example 1.
As shown in FIG. 5, the affinity to antigen of RVAE was similar to that of RVAA, while the affinity to antigen of RVAR was higher than that of RVAA.

Test Example 2

Measurement of Affinity to Antigen of RVAR

The RVAR mutant prepared in step 4 of Example 4 was subjected to competitive ELISA to measure its affinity to antigen as follows:
COS7 cells were transfected with the plasmid prepared in step 4 of Example 4 and the plasmid expressing chimeric light chain (pKC-dhfr-chKR127) prepared in Example 2 to produce an antibody. 5 ng of the antibody thus obtained was reacted with pre-S1 antigen (1×10⁻⁷to 1×10-12 M) at 37° C. for 2 hours. The resulting solution was added to each well of a 96-well microplate coated with pre-S1 antigen and reacted at 37° C. for 30 minutes, and then the resulting solution was subjected to ELISA analysis according to the method described in Example 4. Used as a control is chimeric antibody (chICR127) obtained from COST cells transfected with pcDdA-chKR127HC and pKC-dhfr-chKR127.
The affinity to antigen of RVAR was about 1.8×10⁻¹⁰M, which is 45 times higher than that of chKR127, about 8.2×10-9M

Example 5

Mutation of CDR of Chimeric KR127 Antibody Light Chain by Alanine Injection

To examine the affinity of each amino acid residue of KR127 light chain LCDR1 (aa 24-34), LCDR2(aa 50-60) and LCDR3 (aa 89-97) to antigen, PCR reaction was carried out using vector pKC-dhfr-chKR127 as a template to prepare a modified gene having each amino acid residue of CDR replaced with alanine (the replaced amino acid residue Number was indicated as Kabat number) (see FIG. 2).
Forward primer YM004 of SEQ ID NO: 21 was designed to provide the sequence corresponding to the reader sequence at the 5′-end of the chimeric light chain gene and the HindIII restrition site, and a reverse primer YM009 of SEQ ID NO: 22 was designed to have the sequence corresponding to the N-terminal region of human light chain gene and the BsiWI(CGTACG) restriction site. These primers were used in preparation of mutants of light chain CDR residue.

YM004:

5′-CCA AAG CTT GGA AAG ATG GAT TCA CAG-3′

YM009:

5′-GCA GCC ACC GTA CGT TTG ATT TCC ACC TTG GT-3′

Forward primer YM135 was designed to replace Ser26 of LCDR1 with alanine (S26A) and a reverse primer YM136, to replace AGT coding for Ser at the nucleotide Nos. 76 to 78 of LCDRI gene with GCT coding for alanine.
PCR reactions were carried out according to the method described in Example 1 except that primer sets, YM004/YM135, and YM136/YM009, were used and that primers YM004 and YM009 were used to recombine the annealed DNA fragments obtained by PCR.
The variable region gene of the mutant thus prepared was cleaved with Hind111 and BsiWI and inserted at the HinaTillBsiWI section of vector pKC-dhfr-chKR127, to obtain pKC-dhfr-chKR12713S-S26A. The base sequence of the modified chimeric light chain variable region gene was 5 confirmed by DNA sequence analysis. The vectors containing mutants prepared above are shown in Table 5.
In Table 5, the primer and mutation positions are numbered based on the base sequence of SEQ ID NO: 3.

TABLE 5

	primer	mutation

	Primer	position	position	mutant	vector

LCDR1	F	YM135	67-102	76-78	Ser(AGT)-	pKC-dhfr-chKR127BS-
	R	YM136	86-54		Ala(GCT)	S26A
	F	YM137	69-107	79-81	Gln(CAG)-	pKC-dhfr-chKR127BS-
	R	YM138	91-56		Ala(GCG	Q27A
	F	YM139	70-111	82-84	Ser(AGC)-	pKC-dhfr-chKR127BS-
	R	YM140	94-58		Ala(GCC)	S27aA
	F	YM141	73-114	85-87	Leu(CTC)-	pKC-dhfr-chKR127BS-
	R	YM142	98-64		Ala(GCC)	L27bA
	F	YM143	73-116		Leu(TTA)-	pKC-dhfr-chKR127BS-
	R	YM144	102-68	88-91	Ala(GCA)	L276A
	F	YM145	79-118	91-93	Tyr(TAT)-	pKC-dhfr-chKR127BS-
	R	YM146	103-69		Ala(GCA)	Y27dA
	F	YM147	83-119	94-96	Ser(AGT)-	pKC-dhfr-chKR127BS-
	R	YM148	107-69		Ala(GCT)	S27eA
	F	YM149	84-120	97-99	Asn(AAT)-	pice-dhfr-chKR127BS-
	R	YM150	110-70		Ala(GCT)	N28A
	F	YM151	88-127	100-102	Gly(GGA)-	pKC-dhfr-chKR127BS-
	R	YM152	114-74		Ala(GCA)	G29A
	F	YM153	91-130	103-105	Lys(AAA)-	pKC-dhfr-chKR127BS-
	R	YM154	116-77		Ala(GCA)	K30A
	F	YM155	93-132	106-108	Thr(ACC)-	pKC-dhfr-chKR127BS-
	R	YM156	118-80		Ala(GCC)	T31A
	F	YM103	99-133	109-111	Tyr(TAT)-	pKC-dhfr-chKR127BS-
	R	YM104	120-83		Ala(GCT)	Y32A
	F	N34A-F	106-132	115-118	Asn(AAT)-	pKC-dhfr-chKR127BS-
	R	N34A-R	126-100		Ala(GCT)	Y34A

LCDR2	F	YM129	151-188	163-165	Leu(CTG)-	pKC-dhfr-chKR127BS-
	R	YM130	175-140		Ala(GCG)	L50A
	F	YM131	153-191	166-168	Val(GTG)-	pKC-dhfr-chKR127BS-
	R	YM132	179-145		Ala(GCG)	V51A
	F	YM133	157-192	169-171	Ser(TCT)-	pKC-dhfr-chKR127BS-
	R	YM134	181-147		Ala(GCT)	S52A
	F	K53A-F	163-187	172-174	Lys(AAA)-	pKC-dhfr-chKR127BS-
	R	K53A-R	178-154		Ala(GCA)	K53A
	F	L54A-F	163-189	175-177	Leu(CTG)-	pKC-dhfr-chKR127BS-
	R	L54A-R	180-159		Ala(GCG)	LS4A
	F	D55A-F	170-195	178-180	Asp(GAC)-	pKC-dhfr-chKR127BS-
	R	D55A-R	184-163		Ala(GCC)	D55A
	F	K56A-F	175-198	181-183	Ser(TCT)-	pKC-dhfr-chKR127BS-
	R	K56A-R	190-168		Ala(GCT)	S56A

LCDR3	F	YM113	270-304	280-282	Val(GTG)-	pKC-dhfr-chKR127BS-
	R	YM114	292-258		Ala(GCG)	V89A
	F	YM115	274-307	283-285	Gln(CAA)-	pKC-dhfr-chKR127BS-
	R	YM116	294-259		Ala(GCA)	Q90A
	F	YM117	277-310	286-288	Gly(GGT)-	pKC-dhfr-chKR127BS-
	R	YM118	296-265		Ala(GCT)	G91A
	F	YM119	281-310	289-291	Thr(ACA)-	pKC-dhfr-chKR127BS-
	R	YMI20	302-266		Ala(CCA)	T92A
	F	YM121	282-313	292-294	His(CAT)-	pKC-dhfr-chKR127BS-
	R	YM122	304-271		Ala(GCT)	H93A
	F	YM111	286-314	295-297	Phe(TTT)-	pKC-dhfr-chKR127BS-
	R	YM112	307-274		Ala(GCT)	F94A
	F	YM123	286-317	298-300	Pro(CCT)-	pKC-dhfr-chKR127BS-
	R	YM124	308-278		Ala(GCT)	P95A
	F	114125	292-319	301-303	Gln(CAG)-	pKC-dhfr-chKR127BS-
	R	YM126	311-279		Ala(GCG)	Q96A
	F	YM127	294-320	304-306	Thr(ACG)-	pKC-dhfr-chKR127BS-
	R	YM128	313-282		Ala(GCG)	T97A

Test Example 3

Measurement of Affinity to Antigen of Light Chain Mutant

COST cell was transfected with each of the light chain mutants prepared in Example 5 and the plasmid expressing chimeric heavy chain (pcDdA-chKR127HC) to produce an antibody. The antibody obtained was measured for its affinity to antigen in accordance with the method described in Test Example 1.
Table 6 shows the results obtained for the mutants and pdDA-chKR127HC containing wildtype chimeric KR127 heavy chain.

TABLE 6

	CDR	mutant	Kloow)

	L1	S26A	6.49 ± 0.244
		027A	14.2 + 2.29
		S27aA	37.9 * 6.66
		L27bA	>10000
		L27cA	36.8 * 11.01
		Y27dA	1032.7 + 56.1
		S27eA	>10000
		N28A	>10000
		G29A	23.94 * 2.62
		K30A	>10000
		T31A	13.19 * 1.98
		Y32A	>10000
		N34A	>10000
	L2	LSOA	159.4 + 21.37
		V51A	37.00 + 10.33
		S52A	14.08 * 0.509
		K53A	7.928 * 0.976
		L54A	12.57 + 2.453
		D55A	225.2 * 2.970
		S56A	12.95 ± 0.367
	L3	V89A	121.2 + 4.62
		490A	>10000
		G91A	>10000
		T92A	74.2 + 2.90
		H93A	54.5 + 4.48
		F94A	>10000
		P95A	>10000
		O96A	293.6 * 7.13
		T97A	17.3 ± 2.56

As shown in Table 6, the affinities to antigen of the mutants obtained by replacing the Leu27b, Tyr27d, Ser27e, Asn28, Lys30, Tyr32, and Asn34 of LCDR1; Leu50 and Asp55 of LCDR2; and Va189, Gln90, Gly91, Thr92, His 93, Phe94, Pro95, and Gln96 of LCDR3 with alanine, respectively, were more than 3 times lower than that of the wild type. Therefore, these residues was determined as SDR.

Example 6

Preparation of humanized heavy chain by SDR-grafting method

A humanized heavy chain was prepared using DP7-JH4, a human heavy chain constructed by combining human immunoglobulin germline VH gene segment DP7 (Tomlinson et al., J. Mol. Biol., 227, 776-798, 1992) having an amino acid sequence similar to KR127 heavy chain variable regions and human immunoglobulin germline JH4 segment (Ravetch et al., Cell, 27, 583-591 (1981)).
The Trp33 and Asn35 in HCDR1 of the KR127 were grafted into the DP7-JH4. The Met34 in HCDR1 of the KR127 is identical to that of DP7-JIM. Further, to inhibit lowering the affinity to antigen, Tyr32 in HCDR1 of the KR127 was replaced with alanine of HCDR1 of a human antibody (Gen Bank data base 75023 (SAVVMN)).
The Arg50 and Tyr52 in HCDR2 of the KR127 were grafted onto the DP7-1H4. The Pro52a in HCDR2 of the KR127 is identical to that of DP715 JH4.
The Asp95, Tyr96, Arg97, Va198, and ArgI 02 of HCDR3 were grafted into DP7-JH4.
Further, Ala71 and Lys73 of FR 3 (framwork region 3) in the heavy chain variable region of KR127 antibody which affects the conformation of 20 CDR loops were grafted thereto.
Then, PCR reaction was carried out using primers Ryu 166 of SEQ ID NO: 23 and Hur37 of SEQ ID NO: 24 according to the method described in Example 3 to obtain a humanized heavy chain variable region gene, HuKR127VH-VII.

Ryu 166:

5′-GGA ITT GTC TGC AGT CAT TGT-GGC TCT GCC CTG

GAA CTT-3′

Hur 37:

5′-GAC AAA TCC ACG AGC ACA GTC TAC ATG-3′

The base sequence of the humanized heavy chain variable region gene was determined by DNA sequence analysis (FIG. 2). Then, the gene was cleaved with EcoRI and .Apal and inserted at the EcoRllApal section of vector pdDdA-chKR127HC to obtain pHuKR127HC.
A humanzied antibody was prepared by combining humanized heavy chain thus obtained and the humanized antibody HZKR127I light chain described in Korean. Patent No. 246128 and measured the affinity to antigen was numbered according to the method described in Test Example 2. Humanized antibody HZKR127I was used as a control.
The affinity to antigen of the humanized antibody of about 1.5×10-10 M was about 50 times higher than that of HZKR127I, about 8.2×le M.

Example 7

Preparation of Humanized Light Chain by SDR-Grafting Method

A humanized light chain was prepared using DP7-3134, a human light chian constructed by combining human immunoglobulin germline VK gene segment DPK12 (Cox et al., Eur. J. Immunol., 24, 827-836 (1994)) having an amino acid sequence similar to KR127 light chain variable regions and human immunoglobulin germline 0.1K4 segment (Hieter et al., J. Biol. Chem., 257, 1516-1522 (1982)).
The Tyr27d, Asn28 and Asn34 in LCDR1 of KR127 were grafted into the DPK12-3K4. The amino acid residues at position 27b, 27e, 30 and 15 32 of DP7 is identical to those of KR127 light chain.
The Leu50 and Asp55 in LCDR2 of KR.127 were grafted into the DPK12-3K4 gene.
The Va189, Gly91, Thr92, His93, Phe94, and Gln96 in LCDR3 of KR127 were grafted into the DPK12-JK4. The residues at positions 90 and 20 95 of DP7 is identical to those of KR127.
Further, Leu36 and Arg46 of FR 2 in the light chain variable region of KR127 antibody (which acts on interaction with heavy chain or CDR) were grafted thereto.
Then, PCR reaction was carried out using primers Ryul18 of SEQ ID NO: 25 and Ryu 119 of SEQ ID NO: 26 according to the method described in Example 3 to prepare a humanized light chain variable region gene, HuKR127VH-IV.

Ryu 118:

5′-CTG TGG AGG CTG GCC TGG CTT CTG TAA TAA CCA-3′

Ryu 119:

5′-GGC CAG CCT CCA CAG CTC CTA ATC TAT CTG-3′

The base sequence of the humanized light chain variable region gene was determined by DNA sequence analysis (see HZIV of FIG. 4). Then, the gene was cleaved with HindJII and BsiWI and inserted at the HindlII/BsiWI section of vector pKC-dhfr-chKR127BS to obtain pHuK.R.127KC.
A humanzied antibody was prepared by combining humanized light chain thus obtained and the humanized antibody HZICR1271 heavy chain de(scribed in Korean Patent No. 246128 and its affinity to antigen was measured according to the method described in Test Example 2. Humanized antibody HZKR127I was used as a control.
The affinities to antigen of the humanized antibody of about 8.4×10″⁹M was similar to that of HZICR1271, about 8.2×10″⁹M.

Example 8

Preparation of Humanized Antibody and Measurement of the Affinity to Antigen

To prepare a plasmid containing humanized heavy chain plasmid pHuKR127HC and humanized light chain plasmid pHuKR127KC, the EcoRIMpal fragment containing humanized heavy chain variable region gene of pHuKR127HC and the HindMIBsiWI fragment containing humanized light chain variable region gene of pHuKR127KC were inserted at the EcoRIMpal and HindllBsiWI sections of vector pdCMV-dhfrC-HAVE (KCTC 10028BP), respectively, to obtain plasmid pdCIVW-dhfrC-HuKR127 (FIG. 6). E. coli DH5 a was transformed with the plasmid thus obtained and the transformed E. coli DH5a/pdCMC-dhfrC-HuKR127 was deposited on Mar. 13, 2002 with the Korean Collection for Type Cultures(KCTC) (Address: Korea Research Institute of Bioscience and Biotechnology(KRIBB), #52, Oun-dong, Yusong-ku, Taejon, 305-333, Republic of Korea) under the accession number, KCTC 10198BP, in accordance with the terms of Budapest Treaty on the International Recognition of the Deposit of Microorganism for the Purpose of Patent Procedure.
To prepare cell line expressing the humanized antibody, dhfr-defected CHO (chinese hamster ovary) cells were transformed with plasmid pdCMV-dhfrC-HuICR127 as follows:
CHO cells (ATCC CRL 9096) were seeded to DMEMJF12 media (GIBCO) containing 10% fetal bovine serum and subcultured in an incubator at 37° C. under an atmosphere of 5% CO₂. 5×10⁵cells thus obtained were seeded to the same media and incubated at 37° C. overnight, followed by washing 3 times with OPTI-MEMI solution (GIBCO).
Meanwhile, 5 gg of the plasmid pdCMV-dhfi-C-HuICR127 was diluted in 500 α of OPTI-MEIVII solution. 25 ihe of Lipofectamine was diluted in 500, u-e of the same solution. The resulting solutions were added to a 15 me tube, mixed, and then, kept at room temperature for more than 15 minutes. Then, 2 nit of OPTI-MEM I was added to by DNA-Lipofectamine mixture and the resulting solution was distributed evenly on the COST cells to be kept in a 5% CO₂incubator at 37° C. for 6 hours. Added thereto was 3 in.c, of DMEM/F12 containing 20% fetal bovine serum and cultured for 48 hours.
Then, CHO cells were taken up with trypsin and cultured in-a-MEM media (GIBCO) of 10% dialyzed fetal bovine serum containing G418 (GIBCO BRL; 550. mit) for 2 weeks. After confirming of antibody-producing ability of the transformed clone, the clone was cultured in a-MEM media of 10% dialyzed fetal bovine serum containing 20 nM MTX to induce amplification of gene.
Cell line CHO/HuKR127 having the highest antibody-productivity was selected from the clones and deposited on Mar. 13, 2002 with the Korean Collection for Type Cultures(KCTC) under the accession number, KCTC 10199BP, in accordance with the terms of Budapest Treaty on the International Recognition of the Deposit of Microorganism for the Purpose of Patent Procedure.
To measure the affinity to antigen of the humanized antibody HuKR127, CHO cell line thus obtained was mass cultured in a serum-absence media (CHO-SFMII, GIBCO) and subjected to protein G-shepharose 413 column (Pharmacia). Then, the antibody absorbed on the column was eluted with 0.1 M glycine solution (pH 2.7) and neutralized with 1.0 M tris solution (pH 9.0), followed by dialyzing in PBS buffer (pH 7.0). Further, the affinity to antigen of the purified antibody was determined by the competitive ELISA method described in Test Example 2 and compared with that of a control, humanized HuKR1271. The result was shown in FIG. 7.
As shown in FIG. 7, the affinity to antigen of the humanized antibody of the present invention of 1.6×10^I ^oM was about 50 times higher than 8.2×10⁻⁹M3 of the control group.

Example 9

Confirmation of Immune-Response Induction of Humanized Antibody

To confirm whether the humanized antibody of the present invention (HuKR127) prevents HAMA response, an analysis was conducted according to the TEPITOPE method (Sturniolo et al., Nature Biotechnology, 17, 555-561, 1999) to examine whether a peptide sequences which can bind to MHC (major histocompatibility complex) class II exists in the heavy and light chain variable regions of the humanized antibody.
Tables 8a and 8b show the results of such analysis for MHC class II-5 binding peptide sequences in the heavy chain variable regions of HuKR127 and the light chain variable regions of HuKR127, respectively.

TABLE 7

	HaKR1271	HuICR127

antiboby	peptide	MHC class II	peptide	MHC class II

MHC class	LVQSGAEVV	DRB1_0306	LVQSGAEVK		0
II-binding		DRB1_0307
		DRB1_0308
		DRB1_0311
		DRB1_0421
		DRB1_0701
		DRB1_0703
	VKPGASVKV	DRB1_0102	lUtPGASVKV		0
	FSSSWMNWV	DRB1_0703	FTSAWMNWV		0
	IfIGRIYPGD	DRB1_0801	WMGRIYPSG		0
		DRB1_0817
	FQGRATLTA	DRB1_0401	FQGRVIMTA	ORB1_0305
		DRB1_0402		DRB1 0408
		DRB1_0405		DRB1_0401
		DRB1_0421		DRI31_0402
		DRB1_0426		DRB1_0408
		DRB1_0801		DRB1_0426
		DRI31_0802		DRB1_0801
		DRB1_0B04		DRB1_0802
		DRB1_0806		DRB1_0804
		DRB1_0804		DRB1_0806
		DR81_0813		DRB1_0813
		DRB1_0806		DRB1_0617
		DRBL0817		DRB1_1101
		DRB1_1101		DRB1_1114
		DRB1_1102		DRB1_1120
		DRB1 1104		DRB1_1128
		DRB1-1106		DRB1_1302
		DRB1_1114		DRB1_1305
		DRB1_1120		DRB1_1307
		DRB1_1121		D/W1_1321
		DRB1_1128		DRB1_1323
		DRB1_1302		DRB1_1502
		DRB1_1305
		DRB1_1307
		DRB1_1311
		DRB1_1321
		DRB1_1322
		DRB1_1323
	YWGQGILVT	DRB1_0401	RWGQGTLVT		0
		DRB1_0405
		DRB1_0421
		DRB1_0426
	IGRIYPGDG	DRI350101	MGRIYPSGG	DRB1_0404
		DRB5_0105		DRB1_0405
				DRB1_0410
				DRB1_0423
	YAQKPQGRA	DR1_0802	YAQKFQGRV		0
	VYFCAREYD	DRB1_1304	VYYCAREYR	DRB1_0301
	YWGQGTLVT	DRB1_0401	RWGQGILVT		0
		DRB1_0405
		DRBU1421
		DRB1_0426
total		50		26

TABLE 8a

	HzKR.127I	HuKR127

antiboby	Peptide	MHC class II	peptide	MHC class II

MHC class II-	ILMTQTPLS	DRBL0301	IVMTQTPLS		0
binding		DRB1_0305
		DRB1_0306
		DRB1 0307
		DRB1_0308
		DRB1_0309
		DRBL0311
		DRBL0401
		DRB1 0402
		DRB1_0404
		DRB1_0405
		DRB1_0408
		DRB1_0410
		DRBL0421
		DRB1 0423
		DREli0426
		DRB1_0804
		ERBL1101
		DRBL1102
		DRB1_1104
		DRBL1106
		DRB1_1107
		DRBL1114
		DRB1_1121
		DRB1_1128
		DRB1_1301
		DRB1_1304
		DRB1_1305
		DRB1_1307
		DRB1_1311
		DREIL1321
		DRB1_1322
		DRB1_1323
		DRB1_1327
		DRB1_1328
	LMTQTPLSL	DRBL0101	MCIQMISL		0
		DRB1_0102
		DRB1_0304
	MUMS	ORB1_0101	wILQXPGQP		0
		DRB1_0305
		DRBL0309
		DRBL0401
		DRB10408
		ORM_0421
		DRB10426
		DRB1_0802
		DRB1_1101
		DRB1_1107
		DR/11_1114
		DRB1_1120
		DRB1_1128
		DRB1 1302
		DRB1_1305
		DRB1_1307
		DR/a . . . 1321
		DRB1_1323
		DRB5_0101
		DRB10105
	YYCVQGTHF	DRB1_0101	YYCVQGTHF	DRBLOI01
		DRB1_0701		DRBI_0701
		DRB1_0703		DRBL0703
		DRB1_0104		DRB5_0101
		DRB1_0105		DRB5_0105
	YCVQGTHFP	DR&040/	YCVQGTHFP	ORBL0401
		DRB1_0421		DR/31_0421
		ORB1_0426		DRBL0426

TABLE 8b

	HzKR127I	HuKR127

antiboby	Peptide	MEC class II	peptide	MEC class II

	VGVYYCVQG	DRB1 0806	VGVYYCVQG	DRB1_0806
	IYLVSKLDS	DRB1 0301		DRB1_0402
		D1631-0305		DR13_0404
		DRB1-0306		DRB1_0405
		DRB1-0307
		DRB1-0308		DRB1 01301
		DRB1-0309		DR131-0408
		DRI31-0311
		DRB1-0405
		DRI31-0410
		ORM 01302
DR131 0806	DRB	-1)423
DB1-0813	DRBI-W04
DR131-0817	DB1-1102
19131-1101	DRB1-11(14
DRB1-1102	DRB	-1106
DRB1-1104	DRB111114
	DRB1-1106	IYLVSNRDS	DRB	-1121
DR13E1107	DRB1	1301
DR81 1114	DRB1-1307
121A3I-1120	DRB1-1311
DRB	-1322
DR/31-r1 a
B	IliP
DRB1-1301
DRB1-1302	X1	T3228
DRB1-1301-	DR135	0101
DB1-1305	DRB5	0105
DRB1-1307
DRBE1311
DRB1 1321
DRB1-1322
DRB1-1323
DRB1-1327
DRB1-1328
DRB1-1501
DR13111506
DRB1 0401
DRB1-0404
DRB1-0405
DRB1 13046 _	D R B 1	0	DRDIum---nain
LlYINSFID	8	0	1	0
DRB1 _ 1321	-	DRB1 0421
8	D-0123
LIYLVSNRD	DR131RB1-0126
DR1311304
YLVSNRDSG
	0	YLVSNRDSG	DRB1 0309
40
106
total

As can be seen from Tables 7 and 8, the number of the peptide Sequence in the humanized antibody HuKR127 which binds to MHC class II was fewer than of that the HzKR127I. These results suggest that 35 humanized antibody HuKR127 of the present invention is expected to reduce HAMA response to a greater extent than HzKR127I.
While the embodiments of the subject invention have been described and illustrated, it is obvious that various changes and modifications can be made therein without departing from the spirit of the present invention which should be limited only by the scope of the appended claims.

Claims

1. (canceled)

2. A process for preparing a humanized antibody consisting of the steps of:

(a) first performing alanine scanning mutagenesis for replacing each amino acid residue in the entire complementarily determining region (CDR) of a murine monoclonal antibody heavy chain and light chain variable regions with alanine to produce a series of transformants, selecting a transformant that has a lower affinity to the human antigen (KD) than of the original murine antibody, and determining the replaced amino acid residue of said selected transformant as a specificity determining residue (SDR); and

(b) subsequently grafting all of the said SDR to the corresponding amino acid residues into human antibody variable regions.

3. The process of claim 2, wherein the CDR is selected from the group consisting of HCDR1(aa 31-35), HCDR2(aa 50-65) and HCDR3(aa 95-102) of the heavy chain (SEQ ID NO: 2); and LCDR1(aa 24-34), LCDR2(aa 50-56) and LCDR3(aa 89-97) of the light chain (SEQ ID NO: 4) of the murine monoclonal antibody variable regions of that bind hepatitis B virus pre-S 1 antigen, selecting a transformant that has an affinity to antigen which is more than 3 times lower than the original murine antibody when replaced with alanine, determining the replaced amino acid residue of said transformant as an SDR, and grafting said SDR to the corresponding amino acid sequence in human antibody heavy chain and light chain.

4-24. (canceled)