Isolation, Cloning and High- Level Expression of Neutrophil Gelatinase-Associated Lipocalin Lipocalin2 by Baculovirus Expression System through Gateway Technology

Authors

  • Ali Jahanian-Najafabadi Department of Molecular Biology, Pasteur Institute of Iran, Tehran, Iran
  • Mahdi Rouhbakhsh Blood Transfusion Research Centre, High Institute for Research and Education in Transfusion Medicine, Tehran, Iran
  • Mahshid Mohammadi Pour Blood Transfusion Research Centre, High Institute for Research and Education in Transfusion Medicine, Tehran, Iran
  • Mehryar Habibi Roudkenar Blood Transfusion Research Centre, High Institute for Research and Education in Transfusion Medicine, Tehran, Iran
  • Nasser Masroori Blood Transfusion Research Centre, High Institute for Research and Education in Transfusion Medicine, Tehran, Iran
  • Parisa Bahmani Blood Transfusion Research Centre, High Institute for Research and Education in Transfusion Medicine, Tehran, Iran
  • Raheleh Halabian Blood Transfusion Research Centre, High Institute for Research and Education in Transfusion Medicine, Tehran, Iran
Abstract:

Objective(s) Lipocalin 2 (Lcn2) is a 25-kDa glycoprotein that has initially been extracted from neutrophil granules. Expression of Lcn2 is induced under various pathophysiological conditions. It is also known as an early marker of kidney and heart injury. High-level expression of recombinant Lcn2 neutrophil gelatinase-associated(NGAL) in insect cells was the aim of this study. Materials and Methods Lcn2 gene was isolated from HepG2 cell line. The PCR product was cloned into TOPO vector to construct TOPO-Lcn2. Then Lcn2 was transferred to Gateway adapted Baculovirus DNA by LR recombination reaction. The recombinant Baculovirus DNA was transfected into insect cell line. Expression of recombinant Lcn2 was detected by RT-PCR, ELISA and western blot analysis. Results Insertion of Lcn2 into pENTR/D-TOPO vector was confirmed by using PCR. The accuracy of the nucleotides sequence was verified by DNA sequencing. Transfer of the Lcn2 cDNA into the Baculovirus destination vector by LR recombination reaction was confirmed by amplification of a band of about 860 bp length by using forward Lcn2 primer and V5 reverse primer. Next, Lcn2 protein was detected as a prominent band with approximate molecular weight of 30 kDa in SDS-PAGE and western blot analysis. ELISA results revealed high-level expression of Lcn2 by Spodoptera frugiperda (Sf9) cells. Conclusion High-level expression of Lcn2 protein in insect cells is promising for future potential applications. Recombinant Lcn2 might be used for producing monoclonal or polyclonal antibodies and as potential therapeutic agent. Large scale expression and purification are next steps that are on the way.  

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Journal title

volume 15  issue 3

pages  845- 852

publication date 2012-05-01

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