Overexpression of Prolidase Induces Autophagic Death in MCF-7 Breast Cancer Cells

Ilona Zareba; Thi Yen Ly Huynh; Adam Kazberuk; Joanna Teul; Agnieszka Klupczynska; Jan Matysiak; Arkadiusz Surazynski; Jerzy Palka

doi:10.33594/000000275

Overexpression of Prolidase Induces Autophagic Death in MCF-7 Breast Cancer Cells

Cell Physiol Biochem. 2020 Sep 12;54(5):875-887. doi: 10.33594/000000275.

Authors

Ilona Zareba¹, Thi Yen Ly Huynh¹, Adam Kazberuk¹, Joanna Teul², Agnieszka Klupczynska^{1

3}, Jan Matysiak³, Arkadiusz Surazynski¹, Jerzy Palka⁴

Affiliations

¹ Department of Medicinal Chemistry, Medical University of Bialystok, Bialystok, Poland.
² Department of Pharmaceutical and Biopharmaceutical Analysis, Medical University of Bialystok, Bialystok, Poland.
³ Department of Inorganic and Analytical Chemistry, Poznan University of Medical Sciences, Poznan, Poland.
⁴ Department of Medicinal Chemistry, Medical University of Bialystok, Bialystok, Poland, pal@umb.edu.pl.

PMID: 32918543
DOI: 10.33594/000000275

Abstract

Background/aims: Proline availability for proline dehydrogenase/proline oxidase (PRODH/POX) may represent switching mechanism between PRODH/POX-dependent apoptosis and autophagy. The aim of the study was to evaluate the impact of overexpression of prolidase (proline releasing enzyme) on apoptosis/autophagy in breast cancer MCF-7 cells.

Methods: The model of MCF-7 cells with prolidase overexpression (MCF-7^PL) was obtained. In order to targeting proline for PRODH/POX-dependent pathways substrate for prolidase, glycyl-proline (GP) was provided and proline utilization for collagen biosynthesis was blocked using 2-methoxyestradiol (MOE). Cell viability was determined using Nucleo-Counter NC-3000. The activity of prolidase was determined by colorimetric assay. DNA, collagen and total protein biosynthesis were determined by radiometric method. Expression of proteins was assessed by Western blot and immunofluorescence bioimaging. Concentration of proline was analyzed by liquid chromatography with mass spectrometry.

Results: Prolidase overexpression in MCF-7^PL cells contributed to 10-fold increase in the enzyme activity, 3-fold increase in cytoplasmic proline level and decrease in cell viability and DNA biosynthesis compared to wild type MCF-7 cells. In MCF-7^PL cells MOE and GP significantly decreased the number of living cells. MOE inhibited DNA biosynthesis in both cell lines while GP evoked inhibitory effect on the process only in MCF-7^PL cells. In both cell lines, MOE or MOE+GP inhibited DNA and collagen biosynthesis. Although GP in MCF-7 cells stimulated collagen biosynthesis, it inhibited the process in MCF-7^PL cells. The effects of studied compounds in MCF-7^PL cells were accompanied by increase in the expression of Atg7, LC3A/B, Beclin-1, HIF-1α and decrease in the expression of PRODH/POX, active caspases-3 and -9.

Conclusion: The data suggest that overexpression of prolidase in MCF-7 cells contributes to increase in intracellular proline concentration and PRODH/POX-dependent autophagic cell death.

Keywords: Prolidase; Proline; Autophagy; Collagen biosynthesis; Breast cancer cells MCF-7.

MeSH terms

Apoptosis / drug effects
Autophagic Cell Death / drug effects*
Autophagic Cell Death / physiology
Autophagy / drug effects
Breast Neoplasms / metabolism
Cell Survival / drug effects
Cells, Cultured
Collagen / metabolism
Dipeptidases / metabolism
Dipeptidases / pharmacology*
Fibroblasts / metabolism
Humans
MCF-7 Cells / metabolism
Proline / pharmacology
Proline Oxidase / metabolism

Substances

Collagen
Proline
Proline Oxidase
Dipeptidases
proline dipeptidase

Abstract

MeSH terms

Substances

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