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Engineering human monoclonal antibody fragments: a recombinant enzyme-linked Fab.

作者信息

Burioni R, Plaisant P, Riccio M L, Rossolini G M, Santangelo R, Vannini A, Satta G

机构信息

Istituto di Microbiologia, Università Cattolica del S. Cuore, Roma, Italy.

出版信息

New Microbiol. 1995 Apr;18(2):127-33.

PMID:7603339
Abstract

A new plasmid vector, pCRP, allowing the expression of human recombinant monoclonal antibody Fab fragments fused with a bacterial acid phosphatase has been constructed. pCRP can accept heavy- and light-chain cDNAs cloned from combinatorial antibody libraries displayed on filamentous phages with the pCombIII system and is able to direct expression to soluble Fabs in which the carboxy-terminus of the heavy chain is fused to the amino-terminus of the mature PhoN nonspecific acid phosphatase of Providencia stuartii. Using the pCRP vector, we expressed two different human recombinant Fabs cloned from combinatorial libraries (one anti-tetenus toxoid and the other anti-HIV-1 gp120) fused with the acid phosphatase. In both cases chimeric antibodies were obtained which retained the antigen-binding ability and the enzymatic activity. Similar Fab-enzyme fusions can be successfully used, even unpurified, in enzyme immunoassays.

摘要

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