Directed evolution of cyclic peptides for inhibition of autophagy

Joshua P. Gray; Md Nasir Uddin; Rajan Chaudhari; Margie N. Sutton; Hailing Yang; Philip Rask; Hannah Locke; Brian J. Engel; Nefeli Batistatou; Jing Wang; Brian J. Grindel; Pratip Bhattacharya; Seth T. Gammon; Shuxing Zhang; David Piwnica-Worms; Joshua A. Kritzer; Zhen Lu; Robert C. Bast; Steven W. Millward

doi:10.1039/d0sc03603j

Directed evolution of cyclic peptides for inhibition of autophagy

Joshua P. Gray, Md Nasir Uddin, Rajan Chaudhari, Margie N. Sutton, Hailing Yang, Philip Rask, Hannah Locke, Brian J. Engel, Nefeli Batistatou, Jing Wang, Brian J. Grindel, Pratip Bhattacharya, Seth T. Gammon, Shuxing Zhang, David Piwnica-Worms, Joshua A. Kritzer, Zhen Lu, Robert C. Bast, Steven W. Millward

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Abstract

In recent decades it has become increasingly clear that induction of autophagy plays an important role in the development of treatment resistance and dormancy in many cancer types. Unfortunately, chloroquine (CQ) and hydroxychloroquine (HCQ), two autophagy inhibitors in clinical trials, suffer from poor pharmacokinetics and high toxicity at therapeutic dosages. This has prompted intense interest in the development of targeted autophagy inhibitors to re-sensitize disease to treatment with minimal impact on normal tissue. We utilized Scanning Unnatural Protease Resistant (SUPR) mRNA display to develop macrocyclic peptides targeting the autophagy protein LC3. The resulting peptides bound LC3A and LC3B—two essential components of the autophagosome maturation machinery—with mid-nanomolar affinities and disrupted protein-protein interactions (PPIs) between LC3 and its binding partnersin vitro. The most promising LC3-binding SUPR peptide accessed the cytosol at low micromolar concentrations as measured by chloroalkane penetration assay (CAPA) and inhibited starvation-mediated GFP-LC3 puncta formation in a concentration-dependent manner. LC3-binding SUPR peptides re-sensitized platinum-resistant ovarian cancer cells to cisplatin treatment and triggered accumulation of the adapter protein p62 suggesting decreased autophagic flux through successful disruption of LC3 PPIs in cell culture. In mouse models of metastatic ovarian cancer, treatment with LC3-binding SUPR peptides and carboplatin resulted in almost complete inhibition of tumor growth after four weeks of treatment. These results indicate that SUPR peptide mRNA display can be used to develop cell-penetrating macrocyclic peptides that target and disrupt the autophagic machineryin vitroandin vivo.

Original language	English (US)
Pages (from-to)	3526-3543
Number of pages	18
Journal	Chemical Science
Volume	12
Issue number	10
DOIs	https://doi.org/10.1039/d0sc03603j
State	Published - Mar 14 2021

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General Chemistry

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Gray, J. P., Uddin, M. N., Chaudhari, R., Sutton, M. N., Yang, H., Rask, P., Locke, H., Engel, B. J., Batistatou, N., Wang, J., Grindel, B. J., Bhattacharya, P., Gammon, S. T., Zhang, S., Piwnica-Worms, D., Kritzer, J. A., Lu, Z., Bast, R. C., & Millward, S. W. (2021). Directed evolution of cyclic peptides for inhibition of autophagy. Chemical Science, 12(10), 3526-3543. https://doi.org/10.1039/d0sc03603j

Gray, JP, Uddin, MN, Chaudhari, R, Sutton, MN , Yang, H, Rask, P, Locke, H, Engel, BJ, Batistatou, N, Wang, J, Grindel, BJ , Bhattacharya, P , Gammon, ST, Zhang, S, Piwnica-Worms, D, Kritzer, JA, Lu, Z , Bast, RC & Millward, SW 2021, 'Directed evolution of cyclic peptides for inhibition of autophagy', Chemical Science, vol. 12, no. 10, pp. 3526-3543. https://doi.org/10.1039/d0sc03603j

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title = "Directed evolution of cyclic peptides for inhibition of autophagy",

abstract = "In recent decades it has become increasingly clear that induction of autophagy plays an important role in the development of treatment resistance and dormancy in many cancer types. Unfortunately, chloroquine (CQ) and hydroxychloroquine (HCQ), two autophagy inhibitors in clinical trials, suffer from poor pharmacokinetics and high toxicity at therapeutic dosages. This has prompted intense interest in the development of targeted autophagy inhibitors to re-sensitize disease to treatment with minimal impact on normal tissue. We utilized Scanning Unnatural Protease Resistant (SUPR) mRNA display to develop macrocyclic peptides targeting the autophagy protein LC3. The resulting peptides bound LC3A and LC3B—two essential components of the autophagosome maturation machinery—with mid-nanomolar affinities and disrupted protein-protein interactions (PPIs) between LC3 and its binding partnersin vitro. The most promising LC3-binding SUPR peptide accessed the cytosol at low micromolar concentrations as measured by chloroalkane penetration assay (CAPA) and inhibited starvation-mediated GFP-LC3 puncta formation in a concentration-dependent manner. LC3-binding SUPR peptides re-sensitized platinum-resistant ovarian cancer cells to cisplatin treatment and triggered accumulation of the adapter protein p62 suggesting decreased autophagic flux through successful disruption of LC3 PPIs in cell culture. In mouse models of metastatic ovarian cancer, treatment with LC3-binding SUPR peptides and carboplatin resulted in almost complete inhibition of tumor growth after four weeks of treatment. These results indicate that SUPR peptide mRNA display can be used to develop cell-penetrating macrocyclic peptides that target and disrupt the autophagic machineryin vitroandin vivo.",

author = "Gray, {Joshua P.} and Uddin, {Md Nasir} and Rajan Chaudhari and Sutton, {Margie N.} and Hailing Yang and Philip Rask and Hannah Locke and Engel, {Brian J.} and Nefeli Batistatou and Jing Wang and Grindel, {Brian J.} and Pratip Bhattacharya and Gammon, {Seth T.} and Shuxing Zhang and David Piwnica-Worms and Kritzer, {Joshua A.} and Zhen Lu and Bast, {Robert C.} and Millward, {Steven W.}",

note = "Funding Information: All animal studies were performed in strict accordance with the NIH guidelines for the care and use of laboratory animals and were approved by the UT MD Anderson Institutional Animal Care and Use Committee (IACUC). This work was supported by UT MDACC Startup Funds (SWM), a UT MDACC Moonshot Knowledge Gap Pilot Project, a Cancer Prevention and Research Institute of Texas (CPRIT) Individual Investigator Research Award (RP200166-IIRA, SWM), and the University of Texas MD Anderson Cancer Center Institutional Research Grant (IRG) Program. Additional support came from the MD Anderson SPORE in Ovarian Cancer NCI P50 CA217685, R01 CA135354, R21 CA181994, R01 GM127585, and the shared resources of the MD Anderson CCSG grant NCI P30 CA 16672. We also acknowledge support from T32CA196561 (BJG), F32EB024379 (BJE), and a CPRIT Early Translational Research Award RP170333 (SZ). We also gratefully acknowledge support from The National Foundation for Cancer Research, philanthropic support from the Anne and Henry Zarrow Foundation, and generous donations from Stuart and Gaye-Lynn Zarrow, the Mossy Foundation and the Roberson endowment. Publisher Copyright: {\textcopyright} The Royal Society of Chemistry 2021.",

year = "2021",

month = mar,

day = "14",

doi = "10.1039/d0sc03603j",

language = "English (US)",

volume = "12",

pages = "3526--3543",

journal = "Chemical Science",

issn = "2041-6520",

publisher = "Royal Society of Chemistry",

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T1 - Directed evolution of cyclic peptides for inhibition of autophagy

AU - Gray, Joshua P.

AU - Uddin, Md Nasir

AU - Chaudhari, Rajan

AU - Sutton, Margie N.

AU - Yang, Hailing

AU - Rask, Philip

AU - Locke, Hannah

AU - Engel, Brian J.

AU - Batistatou, Nefeli

AU - Wang, Jing

AU - Grindel, Brian J.

AU - Bhattacharya, Pratip

AU - Gammon, Seth T.

AU - Zhang, Shuxing

AU - Piwnica-Worms, David

AU - Kritzer, Joshua A.

AU - Lu, Zhen

AU - Bast, Robert C.

AU - Millward, Steven W.

N1 - Funding Information: All animal studies were performed in strict accordance with the NIH guidelines for the care and use of laboratory animals and were approved by the UT MD Anderson Institutional Animal Care and Use Committee (IACUC). This work was supported by UT MDACC Startup Funds (SWM), a UT MDACC Moonshot Knowledge Gap Pilot Project, a Cancer Prevention and Research Institute of Texas (CPRIT) Individual Investigator Research Award (RP200166-IIRA, SWM), and the University of Texas MD Anderson Cancer Center Institutional Research Grant (IRG) Program. Additional support came from the MD Anderson SPORE in Ovarian Cancer NCI P50 CA217685, R01 CA135354, R21 CA181994, R01 GM127585, and the shared resources of the MD Anderson CCSG grant NCI P30 CA 16672. We also acknowledge support from T32CA196561 (BJG), F32EB024379 (BJE), and a CPRIT Early Translational Research Award RP170333 (SZ). We also gratefully acknowledge support from The National Foundation for Cancer Research, philanthropic support from the Anne and Henry Zarrow Foundation, and generous donations from Stuart and Gaye-Lynn Zarrow, the Mossy Foundation and the Roberson endowment. Publisher Copyright: © The Royal Society of Chemistry 2021.

PY - 2021/3/14

Y1 - 2021/3/14

N2 - In recent decades it has become increasingly clear that induction of autophagy plays an important role in the development of treatment resistance and dormancy in many cancer types. Unfortunately, chloroquine (CQ) and hydroxychloroquine (HCQ), two autophagy inhibitors in clinical trials, suffer from poor pharmacokinetics and high toxicity at therapeutic dosages. This has prompted intense interest in the development of targeted autophagy inhibitors to re-sensitize disease to treatment with minimal impact on normal tissue. We utilized Scanning Unnatural Protease Resistant (SUPR) mRNA display to develop macrocyclic peptides targeting the autophagy protein LC3. The resulting peptides bound LC3A and LC3B—two essential components of the autophagosome maturation machinery—with mid-nanomolar affinities and disrupted protein-protein interactions (PPIs) between LC3 and its binding partnersin vitro. The most promising LC3-binding SUPR peptide accessed the cytosol at low micromolar concentrations as measured by chloroalkane penetration assay (CAPA) and inhibited starvation-mediated GFP-LC3 puncta formation in a concentration-dependent manner. LC3-binding SUPR peptides re-sensitized platinum-resistant ovarian cancer cells to cisplatin treatment and triggered accumulation of the adapter protein p62 suggesting decreased autophagic flux through successful disruption of LC3 PPIs in cell culture. In mouse models of metastatic ovarian cancer, treatment with LC3-binding SUPR peptides and carboplatin resulted in almost complete inhibition of tumor growth after four weeks of treatment. These results indicate that SUPR peptide mRNA display can be used to develop cell-penetrating macrocyclic peptides that target and disrupt the autophagic machineryin vitroandin vivo.

AB - In recent decades it has become increasingly clear that induction of autophagy plays an important role in the development of treatment resistance and dormancy in many cancer types. Unfortunately, chloroquine (CQ) and hydroxychloroquine (HCQ), two autophagy inhibitors in clinical trials, suffer from poor pharmacokinetics and high toxicity at therapeutic dosages. This has prompted intense interest in the development of targeted autophagy inhibitors to re-sensitize disease to treatment with minimal impact on normal tissue. We utilized Scanning Unnatural Protease Resistant (SUPR) mRNA display to develop macrocyclic peptides targeting the autophagy protein LC3. The resulting peptides bound LC3A and LC3B—two essential components of the autophagosome maturation machinery—with mid-nanomolar affinities and disrupted protein-protein interactions (PPIs) between LC3 and its binding partnersin vitro. The most promising LC3-binding SUPR peptide accessed the cytosol at low micromolar concentrations as measured by chloroalkane penetration assay (CAPA) and inhibited starvation-mediated GFP-LC3 puncta formation in a concentration-dependent manner. LC3-binding SUPR peptides re-sensitized platinum-resistant ovarian cancer cells to cisplatin treatment and triggered accumulation of the adapter protein p62 suggesting decreased autophagic flux through successful disruption of LC3 PPIs in cell culture. In mouse models of metastatic ovarian cancer, treatment with LC3-binding SUPR peptides and carboplatin resulted in almost complete inhibition of tumor growth after four weeks of treatment. These results indicate that SUPR peptide mRNA display can be used to develop cell-penetrating macrocyclic peptides that target and disrupt the autophagic machineryin vitroandin vivo.

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JO - Chemical Science

JF - Chemical Science

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ER -

Directed evolution of cyclic peptides for inhibition of autophagy

Abstract

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