SELECTIVE HIGH-PERFORMANCE LIQUID-CHROMATOGRAPHIC PURIFICATION OF BISPECIFIC MONOCLONAL-ANTIBODIES

被引：18

作者：

TARDITI, L

CAMAGNA, M

PARISI, A

VASSAROTTO, C

DEMONTE, LB

LETARTE, M

MALAVASI, F

MARIANI, M

机构：

[1] SORIN BIOMED SPA,BIOCHEM ONCOL LABS,RES & DEV DIAG LABS,I-13040 SALUGGIA,ITALY

[2] UNIV TURIN,DEPT GENET BIOL & MED CHEM,I-10124 TURIN,ITALY

[3] HOSP SICK CHILDREN,TORONTO M5G 1X8,ONTARIO,CANADA

[4] CNR,CTR IMMUNOGENET & HISTOCOMPATIBIL,TURIN,ITALY

来源：

JOURNAL OF CHROMATOGRAPHY | 1992年 / 599卷 / 1-2期

关键词：

D O I：

10.1016/0021-9673(92)85453-Z

中图分类号：

O65 [分析化学];

学科分类号：

070302 ; 081704 ;

摘要：

The recent development of improved production techniques for bispecific monoclonal antibodies (biMAbs) has significantly increased interest in specific purification procedures. In this investigation, a general high-performance liquid chromatographic (HPLC) purification method is proposed that allows highly purified biMAbs to be obtained from mouse ascites fluid containing a mixture of different antibodies, i.e., parental MAbs, active biMAb and a mixture of randomly assembled heavy and light chains. Proteins from ascites fluid were precipitated with ammonium sulphate and applied to a high-performance protein A column to separate the total immunoglobulin fraction. BiMAbs were isolated from other immunoglobulins by two subsequent passages through a high-performance hydroxyapatite (HPHT) column. This purification protocol combines specificity of protein A for immunoglobulin G (IgG) and high selectivity of hydroxyapatite for different IgG idiotypes. All purification steps were performed rapidly and reliably by HPLC. This method was applied to the purification of six different biMAbs with consistently high yields, purity and homogeneity. This general purification method may prove extremely valuable when highly pure preparation of biMAbs is required, as for in vivo use.

引用

页码：13 / 20

页数：8

共 31 条

[1]

[Anonymous], 1991, Biologicals, V19, P247

[2]

[Anonymous], 1987, POINTS CONSIDER CHAR

[3]

BURAGGI G, 1987, CANCER DETECT PREV, V10, P335

[4] GENE-TRANSFER BY RETROVIRUS-DERIVED SHUTTLE VECTORS IN THE GENERATION OF MURINE BISPECIFIC MONOCLONAL-ANTIBODIES [J].

DEMONTE, LB ;

NISTICO, P ;

TECCE, R ;

DELLABONA, P ;

MOMO, M ;

ANICHINI, A ;

MARIANI, M ;

NATALI, PG ;

MALAVASI, F .

PROCEEDINGS OF THE NATIONAL ACADEMY OF SCIENCES OF THE UNITED STATES OF AMERICA, 1990, 87 (08) :2941-2945

[5]

DEMONTE LB, 1991, 2ND P INT C BISP ANT, P149

[6]

DEMONTE LB, 1991, J CHEMOTHER S, V3, P315

[7] ISOLATION OF PURE IGG1, IGG2A AND IGG2B IMMUNOGLOBULINS FROM MOUSE SERUM USING PROTEIN A-SEPHAROSE [J].

EY, PL ;

PROWSE, SJ ;

JENKIN, CR .

IMMUNOCHEMISTRY, 1978, 15 (07) :429-436

[8]

FORSGREN A, 1966, J IMMUNOL, V97, P822

[9]

FUNARO A, 1990, J IMMUNOL, V145, P2390

[10] MULTIPLE EPITOPE RECOGNITION - AN APPROACH TO IMPROVED RADIOIMMUNODETECTION OF TUMOR-ASSOCIATED ANTIGENS [J].

GIACOMINI, P ;

SEGATTO, O ;

NATALI, PG .

INTERNATIONAL JOURNAL OF CANCER, 1987, 39 (06) :729-736

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