Expression and identification of recombinant soluble single-chain variable fragment of monoclonal antibody MC3

doi:10.3748/wjg.v8.i2.258

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Apr 15, 2002 (publication date) through Apr 26, 2024

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World Journal of Gastroenterology

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1007-9327

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Baishideng Publishing Group Inc, 7041 Koll Center Parkway, Suite 160, Pleasanton, CA 94566, USA

Large Intestinal Cancer

World J Gastroenterol. Apr 15, 2002; 8(2): 258-262
Published online Apr 15, 2002. doi: 10.3748/wjg.v8.i2.258

Expression and identification of recombinant soluble single-chain variable fragment of monoclonal antibody MC3

Feng-Tian He, Yong-Zhan Nie, Bao-Jun Chen, Tai-Dong Qiao, Dai-Ming Fan, Rong-Fen Li, Yun-Sheng Kang, Yan Zhang

Feng-Tian He, Rong-Fen Li, Yun-Sheng Kang, Yan Zhang, Department of Biochemistry & Molecular Biology, Third Military Medical University, Chongqing 400038, China

Yong-Zhan Nie, Bao-Jun Chen, Tai-Dong Qiao, Dai-Ming Fan, Institute of Digestive Disease, Xijing Hospital, Fourth Military Medical University, Xi'an 710032, Shaanxi Province, China

Author contributions: All authors contributed equally to the work.

Correspondence to: Dr. Feng-Tian He, Department of Biochemistry & Molecular Biology, Third Military Medical University, Chongqing 400038, China. hefengtian@163.net

Telephone: +86-23-68752262 Fax: +86-23-68753462

Received: September 25, 2001
Revised: December 1, 2001
Accepted: December 5, 2001
Published online: April 15, 2002

Abstract

AIM: To generate soluble single chain variable fragments (ScFv) of monoclonal antibody MC3 recognizing colorectal and gastric carcinomas.

METHODS: mRNA was isolated from the hybridoma cell line producing MC3 and the DNAs encoding variable domains of heavy and light chains (VH and VL) of the antibody were amplified separately by RT-PCR and assembled into ScFv DNA with a linker DNA.The ScFv DNA was ligated into the phagemid vector pCANTAB5E and the ligated sample was transformed into E. coli TG1.The transformed cells were infected with M13KO7 helper phage to yield recombinant phages. After two rounds of panning with gastric carcinoma cell line AGS highly expressing MC3-binding antigen, the phage clones displaying ScFv fragments of the antibody were selected by ELISA. 4 phage clones showing strong signal in ELISA were used to infect E. coli HB2151 to express soluble ScFvs. The soluble ScFvs were identified by Dot blot and Western blot, and their antigen-binding activity was assayed by ELISA. The VH and VL DNAs of the ScFv DNA derived from phage clone 19 were sequenced.

RESULTS: The VH, VL and ScFv DNAs were about 340 bp, 320 bp and 750 bp respectively. After two rounds of panning to the recombinant phages, 18 antigen-positive phage clones were selected from 30 preselected phage clones by ELISA. All the soluble ScFvs derived from the 4 out of the 18 antigen-positive phage clones were about M_r32000 and concentrated in periplasmatic space under the given culture condition. The soluble ScFvs could bind the antigen, and they shared the same binding site with MC3. The sequences of the VH and VL DNAs of the MC3 ScFv showed that the variable antibody genes belonged to the IgG1 subgroup, κ-type.

CONCLUSION: The soluble ScFv of MC3 is successfully produced, which not only provides a possible novel targeting vehicle for in vivo and in vitro study on associated cancers, but also offers the anuibody a stable genetic source.

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