Role of autophagy and lysosomal drug sequestration in acquired resistance to doxorubicin in MCF-7 cells

Baoqing Guo; Adam Tam; Stacey A Santi; Amadeo M Parissenti

doi:10.1186/s12885-016-2790-3

Role of autophagy and lysosomal drug sequestration in acquired resistance to doxorubicin in MCF-7 cells

BMC Cancer. 2016 Sep 29;16(1):762. doi: 10.1186/s12885-016-2790-3.

Authors

Baoqing Guo¹, Adam Tam², Stacey A Santi¹, Amadeo M Parissenti^{3

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Affiliations

¹ Health Sciences North Research Institute, Sudbury, ON, P3E 5J1, Canada.
² Department of Biology, Laurentian University, Sudbury, ON, P3E 2C6, Canada.
³ Health Sciences North Research Institute, Sudbury, ON, P3E 5J1, Canada. aparissenti@hsnri.ca.
⁴ Department of Biology, Laurentian University, Sudbury, ON, P3E 2C6, Canada. aparissenti@hsnri.ca.
⁵ Division of Medical Sciences, Northern Ontario School of Medicine, Sudbury, ON, P3E 2C6, Canada. aparissenti@hsnri.ca.
⁶ Faculty of Medicine, Division of Oncology, University of Ottawa, Ottawa, ON, K1H 8M5, Canada. aparissenti@hsnri.ca.

Abstract

Background: The roles and mechanisms involved in starvation-induced autophagy in mammalian cells have been extensively studied. However, less is known about the potential role for autophagy as a survival pathway in acquired drug resistance in cancer cells under nutrient-rich conditions.

Methods: We selected MCF-7 breast tumor cells for survival in increasing concentrations of doxorubicin and assessed whether the acquisition of doxorubicin resistance was accompanied by changes in doxorubicin and lysosome localization and the activation of autophagy, as assessed by laser scanning confocal microscopy with or without immunohistochemical approaches. The ultrastructure of cells was also viewed using transmission electron microscopy. Cellular levels of autophagy and apoptosis-related proteins were assessed by immunoblotting techniques, while protein turnover was quantified using a flux assay.

Results: As cells acquired resistance to doxorubicin, the subcellular location of the drug moved from the nucleus to the perinuclear region. The location of lysosomes and autophagosomes also changed from being equally distributed throughout the cytoplasm to co-localizing with doxorubicin in the perinuclear region. There was an apparent temporal correlation between the acquisition of doxorubicin resistance and autophagy induction, as measured by increases in monodansylcadaverine staining, LC3-II production, and co-localization of LAMP1 and LC3-II immunofluorescence. Electron microscopy revealed an increase in cytoplasmic vacuoles containing mitochondria and other cellular organelles, also suggestive of autophagy. Consistent with this view, a known autophagy inhibitor (chloroquine) was highly effective in restoring doxorubicin sensitivity in doxorubicin-resistant cells. Moreover, this induction of autophagy correlated temporally with increased expression of the selective cargo receptor p62, which facilitates the delivery of doxorubicin-damaged mitochondria and other organelles to autophagosomes. Finally, we suggest that autophagy associated with doxorubicin resistance may be distinct from classical starvation-induced autophagy, since Beclin 1 and Atg7 expression did not change upon acquisition of doxorubicin resistance, nor did recombinant Bcl2 overexpression or an Atg7 knockdown alter doxorubicin cytotoxicity.

Conclusion: Taken together, our findings suggest that doxorubicin resistance in MCF-7 breast cancer cells is mediated, at least in part, by the activation of autophagy, which may be distinct from starvation-induced autophagy.

Keywords: Autophagy; Breast tumour cells; Doxorubicin; Drug resistance; Drug sequestration; Lysosomes.