Elimination of dormant, autophagic ovarian cancer cells and xenografts through enhanced sensitivity to anaplastic lymphoma kinase inhibition

Alicia M. Blessing; Janice M. Santiago-O'Farrill; Weiqun Mao; Lan Pang; Jing Ning; Daewoo Pak; Lakshmi Reddy Bollu; Philip Rask; La Kesla Iles; Hailing Yang; Samantha Tran; Ezzeddine Elmir; Geoffrey Bartholomeusz; Robert Langley; Zhen Lu; Robert C. Bast

doi:10.1002/cncr.32985

Elimination of dormant, autophagic ovarian cancer cells and xenografts through enhanced sensitivity to anaplastic lymphoma kinase inhibition

Alicia M. Blessing, Janice M. Santiago-O'Farrill, Weiqun Mao, Lan Pang, Jing Ning, Daewoo Pak, Lakshmi Reddy Bollu, Philip Rask, La Kesla Iles, Hailing Yang, Samantha Tran, Ezzeddine Elmir, Geoffrey Bartholomeusz, Robert Langley, Zhen Lu, Robert C. Bast

Research output: Contribution to journal › Article › peer-review

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Abstract

Background: Poor outcomes for patients with ovarian cancer relate to dormant, drug-resistant cancer cells that survive after primary surgery and chemotherapy. Ovarian cancer (OvCa) cells persist in poorly vascularized scars on the peritoneal surface and depend on autophagy to survive nutrient deprivation. The authors have sought drugs that target autophagic cancer cells selectively to eliminate residual disease. Methods: By using unbiased small-interfering RNA (siRNA) screens, the authors observed that knockdown of anaplastic lymphoma kinase (ALK) reduced the survival of autophagic OvCa cells. Small-molecule ALK inhibitors were evaluated for their selective toxicity against autophagic OvCa cell lines and xenografts. Autophagy was induced by reexpression of GTP-binding protein Di-Ras3 (DIRAS3) or serum starvation and was evaluated with Western blot analysis, fluorescence imaging, and transmission electron microscopy. Signaling pathways required for crizotinib-induced apoptosis of autophagic cells were explored with flow cytometric analysis, Western blot analysis, short-hairpin RNA knockdown of autophagic proteins, and small-molecule inhibitors of STAT3 and BCL-2. Results: Induction of autophagy by reexpression of DIRAS3 or serum starvation in multiple OvCa cell lines significantly reduced the 50% inhibitory concentration of crizotinib and other ALK inhibitors. In 2 human OvCa xenograft models, the DIRAS3-expressing tumors treated with crizotinib had significantly decreased tumor burden and long-term survival in 67% to 79% of mice. Crizotinib treatment of autophagic cancer cells further enhanced autophagy and induced autophagy-mediated apoptosis by decreasing phosphorylated STAT3 and BCL-2 signaling. Conclusions: Crizotinib may eliminate dormant, autophagic, drug-resistant OvCa cells that remain after conventional cytoreductive surgery and combination chemotherapy. A clinical trial of ALK inhibitors as maintenance therapy after second-look operations should be seriously considered.

Original language	English (US)
Pages (from-to)	3579-3592
Number of pages	14
Journal	Cancer
Volume	126
Issue number	15
DOIs	https://doi.org/10.1002/cncr.32985
State	Published - Aug 1 2020

Keywords

GTP-binding protein Di-Ras3 (DIRAS3)
anaplastic lymphoma kinase (ALK)
autophagy
crizotinib
dormancy
ovarian cancer

ASJC Scopus subject areas

Oncology
Cancer Research

MD Anderson CCSG core facilities

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Functional Proteomics Reverse Phase Protein Array Core

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10.1002/cncr.32985

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Blessing, A. M., Santiago-O'Farrill, J. M., Mao, W., Pang, L., Ning, J., Pak, D., Bollu, L. R., Rask, P., Iles, L. K., Yang, H., Tran, S., Elmir, E., Bartholomeusz, G., Langley, R., Lu, Z., & Bast, R. C. (2020). Elimination of dormant, autophagic ovarian cancer cells and xenografts through enhanced sensitivity to anaplastic lymphoma kinase inhibition. Cancer, 126(15), 3579-3592. https://doi.org/10.1002/cncr.32985

Blessing, AM, Santiago-O'Farrill, JM, Mao, W, Pang, L, Ning, J, Pak, D, Bollu, LR, Rask, P, Iles, LK, Yang, H, Tran, S, Elmir, E, Bartholomeusz, G, Langley, R, Lu, Z & Bast, RC 2020, 'Elimination of dormant, autophagic ovarian cancer cells and xenografts through enhanced sensitivity to anaplastic lymphoma kinase inhibition', Cancer, vol. 126, no. 15, pp. 3579-3592. https://doi.org/10.1002/cncr.32985

@article{f8d3eb396173496c81db469f79bf5d5a,

title = "Elimination of dormant, autophagic ovarian cancer cells and xenografts through enhanced sensitivity to anaplastic lymphoma kinase inhibition",

abstract = "Background: Poor outcomes for patients with ovarian cancer relate to dormant, drug-resistant cancer cells that survive after primary surgery and chemotherapy. Ovarian cancer (OvCa) cells persist in poorly vascularized scars on the peritoneal surface and depend on autophagy to survive nutrient deprivation. The authors have sought drugs that target autophagic cancer cells selectively to eliminate residual disease. Methods: By using unbiased small-interfering RNA (siRNA) screens, the authors observed that knockdown of anaplastic lymphoma kinase (ALK) reduced the survival of autophagic OvCa cells. Small-molecule ALK inhibitors were evaluated for their selective toxicity against autophagic OvCa cell lines and xenografts. Autophagy was induced by reexpression of GTP-binding protein Di-Ras3 (DIRAS3) or serum starvation and was evaluated with Western blot analysis, fluorescence imaging, and transmission electron microscopy. Signaling pathways required for crizotinib-induced apoptosis of autophagic cells were explored with flow cytometric analysis, Western blot analysis, short-hairpin RNA knockdown of autophagic proteins, and small-molecule inhibitors of STAT3 and BCL-2. Results: Induction of autophagy by reexpression of DIRAS3 or serum starvation in multiple OvCa cell lines significantly reduced the 50% inhibitory concentration of crizotinib and other ALK inhibitors. In 2 human OvCa xenograft models, the DIRAS3-expressing tumors treated with crizotinib had significantly decreased tumor burden and long-term survival in 67% to 79% of mice. Crizotinib treatment of autophagic cancer cells further enhanced autophagy and induced autophagy-mediated apoptosis by decreasing phosphorylated STAT3 and BCL-2 signaling. Conclusions: Crizotinib may eliminate dormant, autophagic, drug-resistant OvCa cells that remain after conventional cytoreductive surgery and combination chemotherapy. A clinical trial of ALK inhibitors as maintenance therapy after second-look operations should be seriously considered.",

keywords = "GTP-binding protein Di-Ras3 (DIRAS3), anaplastic lymphoma kinase (ALK), autophagy, crizotinib, dormancy, ovarian cancer",

author = "Blessing, {Alicia M.} and Santiago-O'Farrill, {Janice M.} and Weiqun Mao and Lan Pang and Jing Ning and Daewoo Pak and Bollu, {Lakshmi Reddy} and Philip Rask and Iles, {La Kesla} and Hailing Yang and Samantha Tran and Ezzeddine Elmir and Geoffrey Bartholomeusz and Robert Langley and Zhen Lu and Bast, {Robert C.}",

note = "Funding Information: This work was supported by a grant from the National Cancer Institute (NCI) (R01 CA135354 P30CA016672), the MD Anderson Specialized Program in Research Excellence (SPORE) in Ovarian Cancer (NCI grants P50 CA 83639 and CA 217685), the National Foundation for Cancer Research, the Anne and Henry Zarrow Foundation, the Mossy Foundation, the Roberson Endowment, and Stuart and Gaye‐Lynn Zarrow. Alicia M. Blessing is a University of Texas MD Anderson Cancer Center Odyssey Fellow and is supported by the CFP Foundation. Crizotinib was provided by Pfizer Pharmaceuticals. Funding Information: This work was supported by a grant from the National Cancer Institute (NCI) (R01 CA135354 P30CA016672), the MD Anderson Specialized Program in Research Excellence (SPORE) in Ovarian Cancer (NCI grants P50 CA 83639 and CA 217685), the National Foundation for Cancer Research, the Anne and Henry Zarrow Foundation, the Mossy Foundation, the Roberson Endowment, and Stuart and Gaye-Lynn Zarrow. Alicia M. Blessing is a University of Texas MD Anderson Cancer Center Odyssey Fellow and is supported by the CFP Foundation. Crizotinib was provided by Pfizer Pharmaceuticals. Ezzeddine Elmir was supported by the CPRIT Research Training Program (RP170067). Publisher Copyright: {\textcopyright} 2020 American Cancer Society",

year = "2020",

month = aug,

day = "1",

doi = "10.1002/cncr.32985",

language = "English (US)",

volume = "126",

pages = "3579--3592",

journal = "Cancer",

issn = "0008-543X",

publisher = "John Wiley and Sons Inc.",

number = "15",

}

TY - JOUR

T1 - Elimination of dormant, autophagic ovarian cancer cells and xenografts through enhanced sensitivity to anaplastic lymphoma kinase inhibition

AU - Blessing, Alicia M.

AU - Santiago-O'Farrill, Janice M.

AU - Mao, Weiqun

AU - Pang, Lan

AU - Ning, Jing

AU - Pak, Daewoo

AU - Bollu, Lakshmi Reddy

AU - Rask, Philip

AU - Iles, La Kesla

AU - Yang, Hailing

AU - Tran, Samantha

AU - Elmir, Ezzeddine

AU - Bartholomeusz, Geoffrey

AU - Langley, Robert

AU - Lu, Zhen

AU - Bast, Robert C.

N1 - Funding Information: This work was supported by a grant from the National Cancer Institute (NCI) (R01 CA135354 P30CA016672), the MD Anderson Specialized Program in Research Excellence (SPORE) in Ovarian Cancer (NCI grants P50 CA 83639 and CA 217685), the National Foundation for Cancer Research, the Anne and Henry Zarrow Foundation, the Mossy Foundation, the Roberson Endowment, and Stuart and Gaye‐Lynn Zarrow. Alicia M. Blessing is a University of Texas MD Anderson Cancer Center Odyssey Fellow and is supported by the CFP Foundation. Crizotinib was provided by Pfizer Pharmaceuticals. Funding Information: This work was supported by a grant from the National Cancer Institute (NCI) (R01 CA135354 P30CA016672), the MD Anderson Specialized Program in Research Excellence (SPORE) in Ovarian Cancer (NCI grants P50 CA 83639 and CA 217685), the National Foundation for Cancer Research, the Anne and Henry Zarrow Foundation, the Mossy Foundation, the Roberson Endowment, and Stuart and Gaye-Lynn Zarrow. Alicia M. Blessing is a University of Texas MD Anderson Cancer Center Odyssey Fellow and is supported by the CFP Foundation. Crizotinib was provided by Pfizer Pharmaceuticals. Ezzeddine Elmir was supported by the CPRIT Research Training Program (RP170067). Publisher Copyright: © 2020 American Cancer Society

PY - 2020/8/1

Y1 - 2020/8/1

N2 - Background: Poor outcomes for patients with ovarian cancer relate to dormant, drug-resistant cancer cells that survive after primary surgery and chemotherapy. Ovarian cancer (OvCa) cells persist in poorly vascularized scars on the peritoneal surface and depend on autophagy to survive nutrient deprivation. The authors have sought drugs that target autophagic cancer cells selectively to eliminate residual disease. Methods: By using unbiased small-interfering RNA (siRNA) screens, the authors observed that knockdown of anaplastic lymphoma kinase (ALK) reduced the survival of autophagic OvCa cells. Small-molecule ALK inhibitors were evaluated for their selective toxicity against autophagic OvCa cell lines and xenografts. Autophagy was induced by reexpression of GTP-binding protein Di-Ras3 (DIRAS3) or serum starvation and was evaluated with Western blot analysis, fluorescence imaging, and transmission electron microscopy. Signaling pathways required for crizotinib-induced apoptosis of autophagic cells were explored with flow cytometric analysis, Western blot analysis, short-hairpin RNA knockdown of autophagic proteins, and small-molecule inhibitors of STAT3 and BCL-2. Results: Induction of autophagy by reexpression of DIRAS3 or serum starvation in multiple OvCa cell lines significantly reduced the 50% inhibitory concentration of crizotinib and other ALK inhibitors. In 2 human OvCa xenograft models, the DIRAS3-expressing tumors treated with crizotinib had significantly decreased tumor burden and long-term survival in 67% to 79% of mice. Crizotinib treatment of autophagic cancer cells further enhanced autophagy and induced autophagy-mediated apoptosis by decreasing phosphorylated STAT3 and BCL-2 signaling. Conclusions: Crizotinib may eliminate dormant, autophagic, drug-resistant OvCa cells that remain after conventional cytoreductive surgery and combination chemotherapy. A clinical trial of ALK inhibitors as maintenance therapy after second-look operations should be seriously considered.

AB - Background: Poor outcomes for patients with ovarian cancer relate to dormant, drug-resistant cancer cells that survive after primary surgery and chemotherapy. Ovarian cancer (OvCa) cells persist in poorly vascularized scars on the peritoneal surface and depend on autophagy to survive nutrient deprivation. The authors have sought drugs that target autophagic cancer cells selectively to eliminate residual disease. Methods: By using unbiased small-interfering RNA (siRNA) screens, the authors observed that knockdown of anaplastic lymphoma kinase (ALK) reduced the survival of autophagic OvCa cells. Small-molecule ALK inhibitors were evaluated for their selective toxicity against autophagic OvCa cell lines and xenografts. Autophagy was induced by reexpression of GTP-binding protein Di-Ras3 (DIRAS3) or serum starvation and was evaluated with Western blot analysis, fluorescence imaging, and transmission electron microscopy. Signaling pathways required for crizotinib-induced apoptosis of autophagic cells were explored with flow cytometric analysis, Western blot analysis, short-hairpin RNA knockdown of autophagic proteins, and small-molecule inhibitors of STAT3 and BCL-2. Results: Induction of autophagy by reexpression of DIRAS3 or serum starvation in multiple OvCa cell lines significantly reduced the 50% inhibitory concentration of crizotinib and other ALK inhibitors. In 2 human OvCa xenograft models, the DIRAS3-expressing tumors treated with crizotinib had significantly decreased tumor burden and long-term survival in 67% to 79% of mice. Crizotinib treatment of autophagic cancer cells further enhanced autophagy and induced autophagy-mediated apoptosis by decreasing phosphorylated STAT3 and BCL-2 signaling. Conclusions: Crizotinib may eliminate dormant, autophagic, drug-resistant OvCa cells that remain after conventional cytoreductive surgery and combination chemotherapy. A clinical trial of ALK inhibitors as maintenance therapy after second-look operations should be seriously considered.

KW - GTP-binding protein Di-Ras3 (DIRAS3)

KW - anaplastic lymphoma kinase (ALK)

KW - autophagy

KW - crizotinib

KW - dormancy

KW - ovarian cancer

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DO - 10.1002/cncr.32985

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SN - 0008-543X

VL - 126

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JO - Cancer

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ER -

Elimination of dormant, autophagic ovarian cancer cells and xenografts through enhanced sensitivity to anaplastic lymphoma kinase inhibition

Abstract

Keywords

ASJC Scopus subject areas

MD Anderson CCSG core facilities

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