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The genetic engineering of monoclonal antibodies.

Abstract:
A number of recent technological developments have greatly facilitated the genetic engineering of immunoglobulins. The use of PCR has permitted the variable regions to be rapidly cloned either from a specific hybridoma source or as a gene library from non-immunised cells. The conversion of the rodent antibody into a humanized version is now well established. To develop these antibodies for clinical use has required the development of high level expression systems. For the expression of large multimeric glycoproteins, mammalian cell systems generally provide the highest levels of secreted product and therefore are the methods of choice for producing whole recombinant antibodies. Novel antigen-binding units have been developed by joining the two variable domains of an antibody into single-chain polypeptides. Such fragments can be produced in high yield by secretion from E. coli raising the prospect of bulk preparation of these antibody fragments for the development of low-cost immunopurification and assay reagents. Finally, the ability to screen for antigen binding by displaying immunoglobulin variable regions on the surface of filamentous bacteriaphages has opened up the possibility of bypassing the immune system to generate novel antibody specificities in vitro.
Publication status:
Published

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Publisher copy:
10.1016/0022-1759(94)90051-5

Authors


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Institution:
University of Oxford
Division:
MSD
Department:
NDM
Sub department:
Structural Biology
Role:
Author


Journal:
Journal of immunological methods More from this journal
Volume:
168
Issue:
2
Pages:
149-165
Publication date:
1994-02-01
DOI:
EISSN:
1872-7905
ISSN:
0022-1759


Language:
English
Keywords:
Pubs id:
pubs:171640
UUID:
uuid:7e26700d-6784-445e-8d7a-e56f711283ff
Local pid:
pubs:171640
Source identifiers:
171640
Deposit date:
2012-12-19

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