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Wiley InterScience

Plant Biotechnology Journal

Plant Biotechnology Journal

Volume 6 Issue 5, Pages 504 - 515

Published Online: 3 Apr 2008

Journal compilation © 2010 Blackwell Publishing Ltd


Plant Biotechnology Journal is published by Wiley-Blackwell in association with the Society for Experimental Biology (SEB) and the Association of Applied Biologists (AAB).
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A novel platform for biologically active recombinant human interleukin-13 production
David J. Wang 1,, Martin Brandsma 2 , Ziqin Yin 3 , Aiming Wang 2,4 , Anthony M. Jevnikar 3,5 and Shengwu Ma 2,3,5,*
  1 A.B. Lucas Secondary School, 656 Tennent Avenue, London, ON, Canada, N5X 1L8
  2 Department of Biology, University of Western Ontario, London, ON, Canada, N6A 5B7
  3 Transplantation Immunology Group, Lawson Health Research institute, London, ON, Canada, N6A 4G5
  4 Agriculture and Agri-Food Canada, 1391 Sanford St., London, ON, Canada, N5V 4T3
  5 Plantigen Inc., 700 Collip Circle, London, ON, Canada, N6A 5B7
  * Correspondence (fax 519-858-5142; e-mail sma@uwo.ca)
 

Present address: Class of 2011, Princeton University, Princeton, NJ 08544, USA

Copyright Journal compilation © 2008 Blackwell Publishing Ltd
KEYWORDS
glycosylation • human interleukin-13 • new expression platform • transgenic plant • type-1 diabetes

ABSTRACT

AbstractIntroductionResultsDiscussionExperimental proceduresAcknowledgementsReferences

Interleukin-13 (IL-13) is a pleiotropic regulatory cytokine with the potential for treating several human diseases, including type-1 diabetes. Thus far, conventional expression systems for recombinant IL-13 production have proven difficult and are limited by efficiency. In this study, transgenic plants were used as a novel expression platform for the production of human IL-13 (hIL-13). DNA constructs containing hIL-13 cDNA were introduced into tobacco plants. Transcriptional expression of the hIL-13 gene in transgenic plants was confirmed by reverse transcriptase-polymerase chain reaction and Northern blotting. Western blot analysis showed that the hIL-13 protein was efficiently accumulated in transgenic plants and present in multiple molecular forms, with an expression level as high as 0.15% of total soluble protein in leaves. The multiple forms of plant-derived recombinant hIL-13 (rhIL-13) are a result of differential N-linked glycosylation, as revealed by enzymatic and chemical deglycosylation, but not of disulphide-linked oligomerization. In vitro trypsin digestion indicated that plant rhIL-13 was more resistant than unglycosylated control rhIL-13 to proteolysis. The stability of plant rhIL-13 to digestion was further supported with simulated gastric and intestinal fluid digestion. In vitro bioassays using a factor-dependent human erythroleukaemic cell line (TF-1 cells) showed that plant rhIL-13 retained the biological functions of the authentic hIL-13 protein. These results demonstrate that transgenic plants are superior to conventional cell-based expression systems for the production of rhIL-13. Moreover, transgenic plants synthesizing high levels of rhIL-13 may prove to be an attractive delivery system for direct oral administration of IL-13 in the treatment of clinical diseases such as type-1 diabetes.


Received 14 September 2007; revised 9 February 2008; accepted 27 February 2008.

DIGITAL OBJECT IDENTIFIER (DOI)
10.1111/j.1467-7652.2008.00337.x About DOI

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