Production and characterization of anti‐(mucin MUC1) single‐domain antibody in tobacco (Nicotiana tabacum cultivar Xanthi)

A Ismaili, M Jalali‐Javaran, MJ Rasaee… - Biotechnology and …, 2007 - Wiley Online Library
Biotechnology and applied biochemistry, 2007Wiley Online Library
Members of the Camelidae (camels, dromedaries, llamas, alpacas, guanacos and vicunas)
are known to produce Igs (immunoglobulins) devoid of light chains and CH1s (constant
heavy‐chain domains). The antigen‐specific binding fragments of these heavy‐chain
antibodies therefore comprise one single domain (the so‐called 'VHH') and are of great
importance in biotechnological applications. To evaluate the expression and biological
activity of sdAbs (single‐domain antibodies) in plants, which, on account of their small size …
Members of the Camelidae (camels, dromedaries, llamas, alpacas, guanacos and vicunas) are known to produce Igs (immunoglobulins) devoid of light chains and CH1s (constant heavy‐chain domains). The antigen‐specific binding fragments of these heavy‐chain antibodies therefore comprise one single domain (the so‐called ‘VHH’) and are of great importance in biotechnological applications. To evaluate the expression and biological activity of sdAbs (single‐domain antibodies) in plants, which, on account of their small size and antigen‐recognition properties, would have a major impact on antibody‐engineering strategies, we constructed a pBI121‐VHH gene encoding the recombinant sdAb fragments with specificity for a cancer‐associated mucin, MUC1. Analysis of transgenic tobacco (Nicotiana tabacum cultivar Xanthi) plants by PCR and Western blotting demonstrated the expression of sdAb, while ELISA results with various MUC1 antigens and immunocytochemistry with cancerous cell lines confirmed that the activity of these molecules compared favourably with that of the parent recombinant antibodies. Protein purification was achieved by using sequential (NH4)2SO4 precipitation, gel filtration and immunoaffinity chromatography. Analysis of the purified VHH by ELISA indicated that the purified antibody fragments were able to react successfully with a MUC1‐related peptide. These results reaffirm that the tobacco plant is a suitable host for the production of correctly folded VHH antibody fragments with diagnostic and therapeutic applications.
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