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Expression and Purification of Human Granzyme B Fusion Protein to Induce Targeted Apoptosis in PSMA Positive Prostate Cancer Cells
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Background:
Granzyme B can induce apoptosis in target cells by direct and indirect
activation of caspases and cleavage of central caspase substrates. Prostate-specific membrane
antigen (PSMA) is a type II transmembrane glycoprotein and its expression increases following
prostate cancer progression.
Objective:
In this study, we designed a fusion protein including mutant granzyme B, the influenza
virus hemagglutinin HA-2 N-terminal, and PSMA ligand to construct GrB-HA-PSMA ligand fusion
protein as a molecular agent for selective targeting of PSMA-positive (LNCaP) cells.
Methods:
The DNA sequence of our designed structure was synthesized and cloned into a pET28a
expression vector. The recombinant protein was expressed in E. coli origami bacteria and then
purified. The expression of the recombinant protein was verified by SDS PAGE and ELISA
method. Furthermore, ELISA and flow cytometry assays were utilized to investigate the efficiency
of binding and permeability of the recombinant protein into the LNCaP cells. Finally, cell
proliferation and apoptosis rate were evaluated by MTT assay and flow cytometry assay,
respectively. HeLa and PC3 cell lines were used as controls.
Results:
The results showed that GrB-HA-PSMA ligand fusion protein could specifically bind and
internalize into the PSMA-positive cells. Furthermore, treatment of the cells with GrB-HA-PSMA
ligand fusion protein resulted in increased apoptotic cell death and decreased proliferation of
LNCaP cells.
Conclusion:
Our findings indicate the specificity of GrB-HA-PSMA ligand fusion protein for
PSMA-positive cells and suggest that this fusion protein is a potential candidate for prostate cancer
targeted therapy.
Bentham Science Publishers Ltd.
Title: Expression and Purification of Human Granzyme B Fusion Protein to
Induce Targeted Apoptosis in PSMA Positive Prostate Cancer Cells
Description:
Background:
Granzyme B can induce apoptosis in target cells by direct and indirect
activation of caspases and cleavage of central caspase substrates.
Prostate-specific membrane
antigen (PSMA) is a type II transmembrane glycoprotein and its expression increases following
prostate cancer progression.
Objective:
In this study, we designed a fusion protein including mutant granzyme B, the influenza
virus hemagglutinin HA-2 N-terminal, and PSMA ligand to construct GrB-HA-PSMA ligand fusion
protein as a molecular agent for selective targeting of PSMA-positive (LNCaP) cells.
Methods:
The DNA sequence of our designed structure was synthesized and cloned into a pET28a
expression vector.
The recombinant protein was expressed in E.
coli origami bacteria and then
purified.
The expression of the recombinant protein was verified by SDS PAGE and ELISA
method.
Furthermore, ELISA and flow cytometry assays were utilized to investigate the efficiency
of binding and permeability of the recombinant protein into the LNCaP cells.
Finally, cell
proliferation and apoptosis rate were evaluated by MTT assay and flow cytometry assay,
respectively.
HeLa and PC3 cell lines were used as controls.
Results:
The results showed that GrB-HA-PSMA ligand fusion protein could specifically bind and
internalize into the PSMA-positive cells.
Furthermore, treatment of the cells with GrB-HA-PSMA
ligand fusion protein resulted in increased apoptotic cell death and decreased proliferation of
LNCaP cells.
Conclusion:
Our findings indicate the specificity of GrB-HA-PSMA ligand fusion protein for
PSMA-positive cells and suggest that this fusion protein is a potential candidate for prostate cancer
targeted therapy.
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