4.6 Article

Expression and anticancer activity analysis of recombinant human uPA1-43-melittin

Journal

INTERNATIONAL JOURNAL OF ONCOLOGY
Volume 46, Issue 2, Pages 619-626

Publisher

SPANDIDOS PUBL LTD
DOI: 10.3892/ijo.2014.2750

Keywords

urokinase plasminogen activator; melittin; Pichia pastoris; ovarian cancer; fusion protein

Categories

Funding

  1. National Natural Science Foundation of China [81272875, 30973187, 81302242]
  2. Foundation of Ministry of Education of China for Young Scholars [20110061120084]
  3. Jilin Science and Technology Funds [20110755, 20120957, 20130102094JC, 20140204022YY]
  4. basic scientific research of Jilin University Funds and Young Scholars Program of Norman Bethune Health Science Center of Jilin University [20142116]

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The present study is focused on expression of a target fusion protein which can be used in ovarian cancer target therapy. It aimed to construct human urokinase-type plasminogen activator (uPA)(1-43)-melittin eukaryotic expression vector to express recombinant human uPA(1-43)-melittin (rhuPA)(1-43),-melittin) in P. pastoris and to detect its anticancer effects on ovarian cancer cells. The DNA sequences that encode uPA(1-43)amino acids and melittin were synthesized according to its native amino acid sequences and consequently inserted into pPICZaC vector. Then uPA(1-43)-melittin -pPICZaC was transformed into P. pastoris X-33, and rhuPA(1-43)-melittin was expressed by methonal inducing. The bioactivities of recombinant fusion protein were detected with inhibition effects on growth of ovarian cancer cells, cell cycle detection and TUNEL assay. The results of DNA sequence analysis of the recombinant vector uPA(1-43)-melittin -pPICZaC demonstrated that the DNA encoding human uPA(1-43) amino acids and 1-26 amino acids of melittin was correctly inserted into the pPICZ alpha C vector. After being induced by methonal, fusion protein with molecular weight 7.6 kDa was observed on the basis of SDS-PAGE and western blot analysis. The recombinant protein was able to suppress growth of SKOV3, induce cell cycle arrest and apoptosis of SKOV3 cells. The fusion protein does not have any obvious toxicity on normal tissues. RhuPA(1-43)-melittin was successfully expressed in P. pastoris. Taking uPA(1-43) amino acids specifically binding to uPAR as targeted part of fusion protein, and making use of antitumor activity of melittin, the recombinant fusion protein it was able to inhibit growth of ovarian tumors and to be applied for effective targeted treatment.

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