Functional and Stable Expression of Recombinant Human FOXP3 in Bacterial Cells and Development of Antigen-specific Monoclonal Antibodies

doi:10.1093/jb/mvm160

Journal of Biochemistry Advance Access published online on August 30, 2007
Journal of Biochemistry, doi:10.1093/jb/mvm160

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Functional and Stable Expression of Recombinant Human FOXP3 in Bacterial Cells and Development of Antigen-specific Monoclonal Antibodies

Shuiqing Hu¹^,3^,*, Jianxin Dai¹^,*, Huafeng Wei¹^,*, Kexing Fan¹, Huajing Wang¹, Dapeng Zhang¹, Weizhu Qian¹^,2, Bohua Li¹^,2, Hao Wang¹^,2, Tongyu Zhu², Yanyun Zhang³^, and Yajun Guo¹^,2^,3^,

¹International Joint Cancer Institute, Second Military Medical University, 800 Xiangyin Road, Shanghai 200433, People’s Republic of China
²Shanghai Center for Cell Engineering and Antibody, 399 Libing Road, Shanghai 201203, People’s Republic of China
³ E-Institute of Shanghai Universities Immunology Division, Shanghai Jiao Tong University School of Medicine, 227 South Chongqing Road, Shanghai 200025, People’s Republic of China

To whom correspondence should be addressed. Dr.Guo,Yajun, Phone: +86-21-25070241, Fax: +86-21-25074349;, E-mail address: gyj{at}zjbio.org or Phone: +86-21-63852705; E-mail address: yyzhang{at}sibs.ac.cn

Received June 20, 2007; Accepted July 13, 2007

Abstract

FOXP3 is a member of the forkhead/winged-helix family of transcriptionalregulators which plays a key role in CD4⁺CD25⁺ regulatory Tcell (Tregs) function and represents a specific marker for thesecells. In order to understand the functional role of FOXP3 andidentify Tregs both in normal development and relevant diseases,protein-DNA and protein-protein interaction studies involvingthis factor are essentially required. Such investigations wouldbe facilitated by the availability of significant amounts ofpurified FOXP3 protein and specific McAb against FOXP3. Here,we report the purification of human FOXP3 (HFOXP3) expressedin Escherichia coli as a soluble and functional glutathione-S-transferase(GST) fusion protein. Through a single purification procedure,4mg of GST-HFOXP3 recombinant protein was obtained per literof bacterial culture. The biological activity of the recombinantprotein was verified by EMSA assay. The yield of folded FOXP3in the purified GST-FOXP3 was determined by reverse phase HPLC.Besides, we generated and obtained two specific monoclonal antibodiesby immunizing BALB/c mouse with the purified GST-HFOXP3 protein.The resulting HFOXP3 protein and anti-HFOXP3 McAbs might providea useful tool in studying Tregs development and immune regulations.

Key Words: protein expression, purification, FOXP3, monoclonal antibody, Tregs

*These authors contributed equally to this work

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