TY - JOUR
T1 - Development of an extended half-life GM-CSF fusion protein for Parkinson's disease
AU - Yeapuri, Pravin
AU - Olson, Katherine E.
AU - Lu, Yaman
AU - Abdelmoaty, Mai Mohamed
AU - Namminga, Krista L.
AU - Markovic, Milica
AU - Machhi, Jatin
AU - Mosley, R. Lee
AU - Gendelman, Howard E.
N1 - Funding Information:
The authors would like to thank Jared Lacovelli, Brian T Wipke, and Eric Huang, employees at Moderna, Inc. for mRNA LNP formulation reagents and for rodent brain sample analysis employing the nCounter® Nanostring analyzer. We would also like to thank Dr. David G. Standaert for the AAV2/1 constructs used in this study, Dr. Nui Meng and the UNMC Genomics and DNA Sequencing Core for their data analysis and guidance, and the UNMC Flow Cytometry Research Facility staff for flow cytometric analysis support. We thank the Vice Chancellor's Office, of the University of Nebraska Medical Center , for Core Facility support, and data analysis support from Bioinformatics and Systems Biology Core at UNMC which is supported by Nebraska Research Initiative (NRI) and NIH 5P30CA036727 and 2P20GM103427 . Lastly, we thank Aaron Schwab and Mackenzie J. Thurston, for their help with flow cytometry and IHC. The authors are solely responsible for the contents of this publication and do not represent the official views of NIGMS or NIH.
Funding Information:
This research was supported by Moderna, Inc . and National Institutes of Health grants P01 DA028555 , R01 NS36126 , P01 NS31492 , P01 MH64570 , P01 NS43985 , P30 MH062261 , and 2R01 NS034239 (HEG and RLM). The University of Nebraska DNA Sequencing Core is partially supported by the NIGMS (National Institute for General Medical Science) COBRE - 1P30GM110768-01 and INBRE - P20GM103427-14 grants and Fred & Pamela Buffett Cancer Center Support Grant - P30CA036727 . This research was also partly supported by the University of Nebraska Foundation, which include donations from the Margaret R. Larson Professorship, the Carol Swarts, M.D. Emerging Neuroscience Research Laboratory, the Frances and Louie Blumkin, and the Harriet Singer Research Foundations. We are also thankful for the EndNote software site license form the INBRE grant from NIH ( 2P20GM103427 ).
Publisher Copyright:
© 2022 Elsevier B.V.
PY - 2022/8/1
Y1 - 2022/8/1
N2 - Transformation of CD4+ T cell effector to regulatory (Teff to Treg) cells have been shown to attenuate disease progression by restoring immunological balance during the onset and progression of neurodegenerative diseases. In our prior studies, we defined a safe and effective pathway to restore this balance by restoring Treg numbers and function through the daily administration of the cytokine granulocyte-macrophage colony-stimulating factor (GM-CSF). These studies were conducted as a proof-of-concept testing in Parkinson's disease (PD) preclinical models and early phase I clinical investigations. In both instances, they served to ameliorate disease associated signs and symptoms. However, despite the recorded efficacy, the cytokine's short half-life, low bioavailability, and injection site reactions proved to be limitations for any broader use. To overcome these limitations, mRNA lipid nanoparticles encoding an extended half-life albumin-GM-CSF fusion protein were developed for both mouse (Msa-GM-CSF) and rat (Rsa-GM-CSF). These formulations were tested for immunomodulatory and neuroprotective efficacy using 1-methyl-4-phenyl-1,2,3,6-tetrahydropyridine (MPTP) and human wild-type alpha-synuclein (αSyn) overexpression preclinical models of PD. A single dose of the extended half-life mouse and rat mRNA lipid nanoparticles generated measurable GM-CSF plasma cytokine levels up to four days. Increased Treg frequency and function were associated with a resting microglial phenotype, nigrostriatal neuroprotection, and restoration of brain tissue immune homeostasis. These findings were substantively beyond the recorded efficacy of daily recombinant wild-type GM-CSF with a recorded half-life of six hours. Mechanistic evaluation of neuropathological transcriptional profiles performed in the disease-affected nigral brain region demonstrated an upregulation of neuroprotective CREB and synaptogenesis signaling and neurovascular coupling pathways. These findings highlight the mRNA-encoded albumin GM-CSF fusion protein modification linked to improvements in therapeutic efficacy. The improvements achieved were associated with the medicine's increased bioavailability. Taken together, the data demonstrate that mRNA LNP encoding the extended half-life albumin-GM-CSF fusion protein can serve as a benchmark for PD immune-based therapeutics. This is especially notable for improving adherence of drug regimens in a disease-affected patient population with known tremors and gait abnormalities.
AB - Transformation of CD4+ T cell effector to regulatory (Teff to Treg) cells have been shown to attenuate disease progression by restoring immunological balance during the onset and progression of neurodegenerative diseases. In our prior studies, we defined a safe and effective pathway to restore this balance by restoring Treg numbers and function through the daily administration of the cytokine granulocyte-macrophage colony-stimulating factor (GM-CSF). These studies were conducted as a proof-of-concept testing in Parkinson's disease (PD) preclinical models and early phase I clinical investigations. In both instances, they served to ameliorate disease associated signs and symptoms. However, despite the recorded efficacy, the cytokine's short half-life, low bioavailability, and injection site reactions proved to be limitations for any broader use. To overcome these limitations, mRNA lipid nanoparticles encoding an extended half-life albumin-GM-CSF fusion protein were developed for both mouse (Msa-GM-CSF) and rat (Rsa-GM-CSF). These formulations were tested for immunomodulatory and neuroprotective efficacy using 1-methyl-4-phenyl-1,2,3,6-tetrahydropyridine (MPTP) and human wild-type alpha-synuclein (αSyn) overexpression preclinical models of PD. A single dose of the extended half-life mouse and rat mRNA lipid nanoparticles generated measurable GM-CSF plasma cytokine levels up to four days. Increased Treg frequency and function were associated with a resting microglial phenotype, nigrostriatal neuroprotection, and restoration of brain tissue immune homeostasis. These findings were substantively beyond the recorded efficacy of daily recombinant wild-type GM-CSF with a recorded half-life of six hours. Mechanistic evaluation of neuropathological transcriptional profiles performed in the disease-affected nigral brain region demonstrated an upregulation of neuroprotective CREB and synaptogenesis signaling and neurovascular coupling pathways. These findings highlight the mRNA-encoded albumin GM-CSF fusion protein modification linked to improvements in therapeutic efficacy. The improvements achieved were associated with the medicine's increased bioavailability. Taken together, the data demonstrate that mRNA LNP encoding the extended half-life albumin-GM-CSF fusion protein can serve as a benchmark for PD immune-based therapeutics. This is especially notable for improving adherence of drug regimens in a disease-affected patient population with known tremors and gait abnormalities.
KW - Extended half-life
KW - Fusion proteins
KW - Granulocyte-macrophage colony-stimulating factor
KW - Lipid nanoparticle (LNP)
KW - Long-acting
KW - Neuroprotection
KW - Parkinson's disease
KW - Regulatory T cell (Treg)
KW - T cell
KW - mRNAs
UR - http://www.scopus.com/inward/record.url?scp=85133191818&partnerID=8YFLogxK
U2 - 10.1016/j.jconrel.2022.06.024
DO - 10.1016/j.jconrel.2022.06.024
M3 - Article
C2 - 35738463
AN - SCOPUS:85133191818
SN - 0168-3659
VL - 348
SP - 951
EP - 965
JO - Journal of Controlled Release
JF - Journal of Controlled Release
ER -
