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A rationally optimized nanoparticle system for the delivery of RNA interference therapeutics into pancreatic tumors in vivo Joann Teo, Joshua A. McCarroll, Cyrille Boyer, Janet Youkhana, Sharon Marie Sagnella, Hien T.T Duong, Jie Liu, George Sharbeen, David Goldstein, Thomas P. Davis, Maria Kavallaris, and Phoebe A. Phillips Biomacromolecules, Just Accepted Manuscript • DOI: 10.1021/acs.biomac.6b00185 • Publication Date (Web): 15 Jun 2016 Downloaded from http://pubs.acs.org on June 16, 2016
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Biomacromolecules is published by the American Chemical Society. 1155 Sixteenth Street N.W., Washington, DC 20036 Published by American Chemical Society. Copyright © American Chemical Society. However, no copyright claim is made to original U.S. Government works, or works produced by employees of any Commonwealth realm Crown government in the course of their duties.
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A rationally optimized nanoparticle system for the delivery of RNA
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interference therapeutics into pancreatic tumors in vivo.
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Joann Teo 1,2#, Joshua A. McCarroll 1,2#, Cyrille Boyer 2,3, Janet Youkhana 4, Sharon M. Sagnella
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1,2
5
Maria Kavallaris 1,2,6*, Phoebe A. Phillips 2,4*
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1
Tumour Biology and Targeting Program, Children’s Cancer Institute, Lowy Cancer Research Centre, UNSW Australia, NSW, Australia.
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2
9 10 11 12
, Jie Liu 4, George Sharbeen 4, David Goldstein
4,5
, Thomas P. Davis
7,8
,
3
Centre for Advanced Macromolecular Design, School of Chemical Engineering, UNSW Australia, NSW, Australia. 4
Pancreatic Cancer Translational Research Group, Lowy Cancer Research Centre, Prince of Wales Clinical School, UNSW Australia, NSW, Australia. 5
14 15
6
18
2,3
Australian Centre for NanoMedicine, UNSW Australia, NSW, Australia.
13
16 17
, Hien T. T Duong
Prince of Wales Hospital, Prince of Wales Clinical School, Sydney, NSW, Australia.
ARC Centre of Excellence in Convergent Bio-Nano Science and Technology UNSW Australia, NSW, Australia. 7
ARC Centre of Excellence in Convergent Bio-Nano Science and Technology Monash Institute of Pharmaceutical Sciences, Monash University, Victoria, Australia. 8
Department of Chemistry University of Warwick, Coventry, United Kingdom.
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# Contributed equally to the study.
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*Corresponding authors: Phoebe. A. Phillips (P.P): Phone: 612-9385-2785; E-mail:
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[email protected];
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[email protected] (M.K.). For P.P: Pancreatic Cancer Translational Research
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Group, Lowy Cancer Research Centre, UNSW Australia. M.K: Tumour Biology and Targeting
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Program, Children’s Cancer Institute, Lowy Cancer Research Centre, UNSW Australia, NSW,
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Australia; Australian Centre for NanoMedicine, UNSW Australia, NSW Australia.
Maria
Kavallaris
(M.K):
Phone:
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612-9385-1556;
Email:
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Keywords: Star polymers, RAFT Polymerization, siRNA, pancreatic cancer cells, orthotopic
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pancreatic cancer mouse model, βIII-tubulin. Running title: Star polymer nanoparticles as
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effective delivery vehicles for siRNA to pancreatic cancer cells.
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Conflict of interest disclosure: The authors declare no competing financial interest.
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ABSTRACT
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Pancreatic cancer is a devastating disease with a dismal prognosis. Short-interfering RNA
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(siRNA) based therapeutics hold promise for the treatment of cancer. However, development of
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efficient and safe delivery vehicles for siRNA remains a challenge. Here, we describe the
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synthesis and physicochemical characterization of star polymers (star 1, star 2, star 3) using
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reversible addition-fragmentation chain transfer polymerization (RAFT) for the delivery of
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siRNA to pancreatic cancer cells. These star polymers were designed to contain different lengths
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of cationic poly(dimethylaminoethyl methacrylate) (PDMAEMA) side-arms and varied amounts
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of poly[oligo(ethylene glycol) methyl ether methacrylate] (POEGMA). We showed that star-
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POEGMA polymers could readily self-assemble with siRNA to form nanoparticles. The star-
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POEGMA polymers were non-toxic to normal cells and delivered siRNA with high efficiency to
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pancreatic cancer cells to silence a gene (TUBB3/βIII-tubulin) which is currently undruggable
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using chemical agents, and is involved in regulating tumor growth and metastases. Notably,
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systemic administration of star-POEGMA-siRNA resulted in high accumulation of siRNA to
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orthotopic pancreatic tumors in mice and silenced βIII-tubulin expression by 80% at the gene and
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protein levels in pancreatic tumors. Together, these novel findings provide strong rationale for
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the use of star-POEGMA polymers as delivery vehicles for siRNA to pancreatic tumors.
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INTRODUCTION
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Pancreatic cancer is ranked as the 4th leading cause of cancer-related deaths in Western societies,
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with a dismal 5-year survival rate of 6% 1. This poor prognosis is due to its resistance to
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chemotherapy drugs and aggressive growth/metastases. Hence, there is an urgent need to develop
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novel therapeutic strategies to treat this disease.
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RNA interference (RNAi) is a powerful gene-silencing mechanism that occurs in mammals 2. In
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brief, this mechanism involves short-interfering RNA (siRNA) assembling within a multi-protein
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RNA induced silencing complex (RISC)
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complementary to target mRNA, which results in its degradation and reduced translation 2. RNAi
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can be manipulated by the introduction of chemically synthesized siRNA to suppress genes
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which are involved in regulating human disease 3. An attractive feature for exploiting the
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therapeutic potential of RNAi is its ability to silence any gene, including those difficult to inhibit
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using chemical inhibitors
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therapeutics for the treatment of many types of human disease, including cancer.
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Microtubules are cytoskeletal proteins that comprise α- and β-tubulin heterodimers which
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contribute to essential cellular processes such as maintenance of cell shape, intracellular
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transport and mitosis 6. β-tubulins’ have been extensively studied in cancer given they are the
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target site for tubulin-binding chemotherapy drugs such as taxanes, vinca alkaloids and
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epothilones 6. However, development of drug resistance and potential off-target toxicity has
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limited their efficacy 6. β-tubulin has 7 different isotypes (βI, βII, βIII, βIVa, βIVb, βV and βVI)
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which share high sequence homology, encoded by different genes and are distinguished by their
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unique carboxy terminal tail 6. The different isotypes have tissue-specific expression 6. High βIII-
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tubulin (encoded by the TUBB3 gene) expression has been reported in different tumor types and
3-5
2
. Together, siRNA-RISC binds with perfect
. This has led to an intense research effort to design RNAi
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is associated with poor patient survival and increased chemoresistance 6. Recently, we
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demonstrated that human pancreatic tumors and pancreatic cancer cells expressed high levels of
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βIII-tubulin 7. Importantly, stable suppression of βIII-tubulin using shRNA in pancreatic cancer
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cells reduced tumor growth and metastases in a clinically-relevant orthotopic pancreatic cancer
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xenograft mouse model 7. Moreover, inhibition of βIII-tubulin expression in pancreatic cancer
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cells increased their sensitivity to chemotherapy drugs in vitro 7. Despite the promise of βIII-
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tubulin as a novel therapeutic target for pancreatic cancer, there are no pharmacological agents
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which can specifically inhibit βIII-tubulin and design of such inhibitors is problematic due to its
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high sequence homology with the other β-tubulin proteins. Therefore, a unique opportunity
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exists to develop siRNA-based therapies to selectively silence βIII-tubulin expression in
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pancreatic cancer cells.
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siRNA requires a delivery vehicle to protect it from degradation within the circulatory system
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and allow it to enter cells
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encapsulate or complex siRNA and deliver it to a host of different cell types 5. Nanoparticle-
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siRNA therapies are in clinical trial to treat a number of diseases and have been shown to be safe
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8-10
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to produce; can be synthesized in large-scale amounts with high reproducibility for clinical
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translation; are non-toxic; can self-assemble with siRNA; and have high tumor bioavailability
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and retention time.
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Star polymers have received increased attention over the last several years as delivery vehicles
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for different therapeutic agents
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large-scale quantities, and importantly their structure is well-defined and can be easily tailored
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for a desired application 16. For example, their internal core and /or peripheral side-arms can be
3-5
. To overcome this problem nanotechnology has been used to
. However, despite their potential there is still a need to develop nanomaterials which are easy
11-17
. They are cost-effective to produce, can be synthesized in
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modified to control their size or to incorporate biodegradable components that allow them to be
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processed within a cell
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contain moieties to actively target specific cell types 16. Notably, studies have demonstrated that
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star polymers can be designed to self-assemble DNA or siRNA and deliver it to different cell
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types in vitro. Cho et al.
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. Their side-arms can also be manipulated to increase their stability or
11, 12
showed that star polymers synthesized using atom transfer radical
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copolymerization (ATRP) can complex siRNA or DNA and deliver them to different non-tumor
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cell types in vitro. A study reported by Pafiti et al.
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using “living” polymerization and containing dimethylaminoethyl methacrylate (DMAEMA)
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were able to deliver siRNA to mouse myoblasts and silence a gene with greater efficiency
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compared to linear DMAEMA homopolymers. However, while these studies provided proof-of-
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principle for the use of star-shaped nanoparticles as carriers for siRNA, they did not examine
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their ability to deliver siRNA and silence target gene expression in vivo. Moreover, there have
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been no studies to determine whether star polymers could be used as a delivery vehicle for
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siRNA to solid tumors in mouse models which closely mimic the human setting.
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Recently, we reported on the design and synthesis of cationic star polymers using DMAEMA as
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the monomer via reversible addition-fragmentation chain transfer (RAFT) polymerization, which
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complexed siRNA resulting in nanoparticles with a size of ~ 35 nm
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siRNA complexes were able to deliver siRNA and silence target gene expression in lung and
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pancreatic cancer cells
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(intratumoral) delivery of siRNA to silence gene expression in tumor cells in vivo
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despite their clinical potential for local delivery of RNAi agents, most cancer therapeutics require
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systemic administration in an effort to target both primary and metastatic tumor sites
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limitation of highly charged cationic nanoparticles for systemic delivery of siRNA is their
18
15
showed that star polymers synthesized
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. These nanoparticle-
. We also showed that star polymers may be used for local
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. However,
19
. A
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toxicity and potential to interact with serum proteins present in the bloodstream, which can lead
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to the formation of large aggregates and poor gene-silencing activity. To overcome this problem
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researchers have utilized PEGylation [incorporation of poly(ethylene glycol) (PEG) or
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poly[oligo(ethylene glycol) methyl ether methacrylate] (POEGMA)] as a strategy to shield the
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positive charge of cationic nanoparticles, thereby reducing toxicity and masking serum protein
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aggregation
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silencing activity by preventing or retarding the ability of siRNA to complex with nanoparticles,
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as well as inhibit cellular uptake and endosomal escape within the cell
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describe the synthesis and characterization of a series of core crosslinked star polymers with
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various compositions. We demonstrate that star-POEGMA-siRNA nanocomplexes are non-toxic
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and act as highly effective delivery vehicles for siRNA to pancreatic cancer cells. We also show
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for the first time that star-POEGMA-siRNA nanoparticles accumulate at high levels in pancreatic
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tumors in mice and potently silence βIII-tubulin expression and decrease tumor growth.
20, 21
. However, it is also recognized that PEGylation can impede siRNA gene
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. In this study, we
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MATERIALS AND METHODS
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Materials. Dimethylaminoethyl methacrylate (DMAEMA, 99%, Sigma-Aldrich), oligoethylene
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glycol methylether methacrylate (OEGMA, Sigma-Aldrich) and dimethylaminoethyl acrylate
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(DMAEA, Sigma-Aldrich) were de-inhibited by passing through a basic alumina column. N,N’-
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methylenebisacrylamide (Sigma-Aldrich, 98%) and N,N’-bis(acryloyl)cystamine (Sigma-
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Aldrich, 99%) were used without additional purification. 4-cyanopentanoic acid dithiobenzoate
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was prepared as previously described
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supplementary information). The initiator, 2,2′-azobisisobutyronitrile (AIBN), was crystallized
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twice using methanol. High purity N2 (Linde gases) was used for reaction solution purging. All
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other reactants were used as received without further purification. Dulbecco’s Modified Eagle’s
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Medium (DMEM, Lonza, USA), heat inactivated fetal calf serum (FCS), horse serum and 2 nM
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L-glutamine were purchased from SAFC Biosciences (Lexena, KS, USA). Cell culture
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consumables were obtained from Thermo Fisher Scientific (Lafayette, CO, USA). Lipofectamine
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2000TM was purchased from Life Technologies (Carlsbad, CA, USA). All reagents used to
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measure gene-silencing activity using real-time PCR (qPCR) were purchased from Life
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Technologies (Carlsbad, CA, USA). 18S Quantitect housekeeping gene primer assay was
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purchased from Qiagen (Valencia, CA, USA). BCA protein assay kit was purchased from Pierce
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(Danvers, MA. USA). siRNAs were purchased from GE Lifesciences (Lafayette, CO, USA).
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AlexaFlour-488 conjugated and AlexaFlour-647 conjugated siRNAs for nanoparticle cell uptake
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studies were purchased from Qiagen (Valencia, CA, USA). Primary antibodies: anti-βIII-tubulin
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(clone TUJ1) was purchased from Covance (Richmond, CA, USA), anti-GAPDH (clone 6C5)
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was purchased from Sapphire Bioscience (Waterloo, NSW, Australia) and anti-CD31 was
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purchased from AbCam, Ltd, Australia. Horseradish peroxidase (HRP)-conjugated IgG goat
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anti-mouse secondary antibody was purchased from GE Healthcare (Buckinghamshire, UK).
23
(a brief description of its preparation is provided in the
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Eight well chamber slides were purchased from Ibidi (Martinsried, Germany). ProLong® Gold
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Antifade Reagent with DAPI, LysoTracker® Red DND-99, Hoechst 33342 were purchased from
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Life Technologies (Carlsbad, CA, USA), D-Luciferin potassium salt was purchased from Gold
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Biotechnology (St Louis, MO, USA) and growth-factor reduced matrigel from BD Biosciences
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(San Jose, CA, USA).
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Synthesis of star-POEGMA polymers.
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Synthesis of the POEGMA arm homopolymer. Oligo(ethylene glycol) methyl ether
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methacrylate [OEGMA (MW 300 g/mol), 15.0 g, 0.05 mol], 2,2’-azobisisobutyronitrile (AIBN,
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33.0 mg, 2 × 10-4 mol), 4-cyanopentanoic acid dithiobenzoate (CPADB, 0.310 g, 1.11 × 10-3
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mol) and dry toluene (50 ml) were added to a round bottom flask, (100 ml), and stirred. The
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mixture was then degassed with nitrogen at 0 oC for 1 hour. The solution was stirred at 65 °C for
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14 hours and quenched. An aliquot was then collected and analyzed using GPC and 1H NMR.
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The monomer conversion was ~70%. The mixture was concentrated by rotary evaporation and
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the polymer precipitated in petroleum ether (low boiling point) to remove trace amounts of
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monomer. The purified POEGMA was analyzed by NMR, GPC and UV-visible spectroscopy.
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The molecular weight was calculated by NMR spectroscopy (Mn, NMR = 10,600 g/mol) to be close
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to the theoretical value (Mn, theor. = 10,100 g/mol) and corresponded with GPC results (Mn, GPC =
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11,500 g/mol, PDI = 1.14).
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Synthesis of PDMAEMA homopolymers. Two homopolymers of PDMAEMA were prepared
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by RAFT polymerization with a molecular weight of ~ 5,000 and 10,000 g/mol.
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Dimethylaminoethyl methacrylate (DMAEMA, Mw = 157 g/mol, 7.78 g, 0.05 mol), 2,2’-
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azobisisobutyronitrile (AIBN, 31.8 mg, 1.94 × 10-4 mol), 4-cyanopentanoic acid dithiobenzoate 8 ACS Paragon Plus Environment
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(CPADB, 0.271 g, 9.7 × 10-4 mol) and dry acetonitrile (30 ml) were added to a round bottom
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flask (100 ml), and stirred. The reaction mixture was cooled and degassed using nitrogen at 0 oC
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for 1 hour. The solution was stirred at 65 °C for 14 hours and then quenched. An aliquot was
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collected for GPC and 1H NMR analyses (monomer conversion ~ 70%). The solvent was
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removed using rotary evaporation and the red polymer mixture was dissolved in acetone. The
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polymer was precipitated twice in petroleum ether to remove any traces of monomer. The
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polymer was collected and dried under vacuum. The purified PDMAEMA was analyzed by
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NMR, UV-vis and GPC. The molecular weight was determined using NMR spectroscopy (Mn,
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NMR
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with GPC results (Mn, GPC = 5,100 g/mol, PDI = 1.09).
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A similar procedure was employed for the synthesis of PDMAEMA (Mn = 10,700 g/mol),
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dimethylaminoethyl methacrylate [DMAEMA (Mw =157 g/mol), 7.78 g, 0.05 mol], 2,2’-
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azobisisobutyronitrile (AIBN, 17.0 mg, 1.03 × 10-4 mol), 4-cyanopentanoic acid dithiobenzoate
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(CPADB, 0.145 g, 5.19 × 10-4 mol) and dry acetonitrile (30 ml) were added to a round bottom
193
flask (100 ml) and stirred. The reaction was cooled and degassed using nitrogen at 0 oC for 1
194
hour. This solution was then stirred for 14 hours at 65 °C. Following this the reaction was
195
quenched and an aliquot assessed by GPC and 1H NMR. The monomer conversion was ~70%.
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Rotary evaporation was used to concentrate the mixture and the polymer precipitated twice in
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petroleum ether to remove any traces of monomer. The purified PDMAEMA was analyzed by
198
NMR, UV-vis and GPC. The molecular weight was calculated using NMR spectroscopy (Mn,
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NMR
200
agreement with the GPC results (Mn, GPC = 10,700 g/mol, PDI = 1.09).
= 5,000 g/mol) was close to the theoretical value (Mn, theor. = 5,600 g/mol) and correlated
= 10,000 g/mol) and was close to the theoretical value (Mn, theor. = 10,500 g/mol) and in good
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Synthesis of PDMAEMA/POEGMA core crosslinked star via the arm first methodology
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(Star 1). PDMAEMA (Mn,
203
11,500 g/mol, 5.1 g, 4.43 × 10-4 mol) were added to a vial containing a magnetic stirrer, together
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with AIBN (78 mg, 4.76 × 10-4 mol) and toluene (100 ml). Crosslinker [(N,N’-
205
bisacryloyl(cystamine), 3.0 g, 1.15 × 10-2 mol] and dimethylaminoethyl acrylate (DMAEA, 0.80
206
g, 5.59 × 10-3 mol) were then added and the vials sealed and purged with nitrogen for 1 hour at 0
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o
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polymerization process, aliquots were collected and analyzed by 1H NMR and GPC. 1H NMR
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analysis confirmed the high conversion of crosslinker and DMAEA. Next, the reaction mixture
210
was concentrated under vacuum. Core crosslinked star polymers were precipitated twice in cold
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petroleum ether/diethyl ether mixture (05/95 v/v) to remove the residual arms to yield a yellow
212
product (yield ~60%). The purified core crosslinked star polymer was analyzed by GPC (Mn, GPC
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= 125,000 g/mol and PDI = 1.19), FTIR and NMR spectroscopy to determine its composition
214
(feed ratio: fOEGMA/fDMAEMA 34/66 mol-% (or 50/50 w-%), final composition: fOEGMA/fDMAEMA
215
48/52 mol-% (or 64/36 w-%). The purified core crosslinked star polymer was solubilized in
216
methanol and then stored in fridge to avoid irreversible crosslinking. Core crosslinked star
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polymers were dissolved in methanol and dialyzed with water/HCl (pH = 3.0) for 24 hours. A
218
further dialysis against water was then carried out for 48 hours. Finally, the solution was freeze
219
dried to yield POEGMA/PDMAEMA star polymers and characterized by NMR, FTIR
220
spectroscopy, DLS and TEM.
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Synthesis of PDMAEMA/POEGMA star using an arm first approach (Star 2). The
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synthesis of star 2 was carried out using similar techniques as described above for star 1. In brief,
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PDMAEMA (Mn = 10,700 g/mol, 5.0 g, 4.67 × 10-4 mol) and POEGMA (Mn = 11,500 g/mol, 5.0
GPC
= 5,100 g/mol, 5.1 g, 1 × 10-3 mol) and POEGMA (Mn
GPC
=
C. The vials were then incubated in an oil bath for 24 hours at 70 °C. At the end of the
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g, 4.34 × 10-4 mol) were added to a vial containing a magnetic stir bar, together with AIBN (50
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mg, 3.06 × 10-4 mol) and toluene (100 ml). Crosslinker (N,N’-bisacryloyl(cystamine) (1.910 g,
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7.34 × 10-3 mol) and DMAEA (0.500 g, 3.49 × 10-3 mol) were added. The mixture was
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polymerized according to the previous condition. The core crosslinked star polymer was
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precipitated twice in cold mixture petroleum ether/diethyl ether (5/95 v/v) to remove the residual
229
arms to yield a yellow product (yield ~65%). The purified core crosslinked star polymer was
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analyzed by GPC (Mn,
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purification to determine its composition (feed ratio: fOEGMA/fDMAEMA 34/66 mol-% (or 50/50 w-
232
%), final composition: fOEGMA/fDMAEMA 51/49 mol-% (or 66/34 w-%). The purified core
233
crosslinked star polymer was dissolved in methanol and stored in the fridge to avoid irreversible
234
crosslinking. Core crosslinked star polymers were solubilized in methanol and dialyzed with
235
water/HCl (pH = 3.0) for 24 hours. A further dialysis against water was then carried out for 48
236
hours. The resulting solution was freeze dried to yield PDMAEMA/POEGMA core crosslinked
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star polymers and characterized by NMR, FTIR spectroscopy, DLS and TEM.
238
Synthesis of PDMAEMA/POEGMA star via the arm-first methodology (Star 3). The
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synthesis of star 3 was carried out using similar techniques as above. In brief, PDMAEMA (Mn =
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10,700 g/mol, 5.25 g, 4.91 × 10-4 mol) and POEGMA (Mn = 11,500 g/mol, 0.83 g, 7.21 × 10-5
241
mol) were added into a vial containing a magnetic stir bar along with AIBN (33 mg, 2× 10-4 mol)
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and toluene (100 ml). Crosslinker (N,N’-bisacryloyl(cystamine) (1.139 g, 4.38 × 10-3 mol) and
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DMAEA (0.308 g, 2.15 × 10-3 mol) were then added. The mixture was polymerized according to
244
the previous conditions. The core crosslinked star polymer was precipitated twice in cold diethyl
245
ether/petroleum spirit (90/10 v/v) to remove unreacted arm to yield a yellow product (yield
246
~80%). The purified core crosslinked star polymer was analyzed by GPC (Mn,
GPC
= 145,000 g/mol and PDI = 1.29), and by NMR and FTIR after
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GPC
= 145,000
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g/mol and PDI = 1.29), and by NMR and FTIR after purification to determine its composition
248
(feed ratio: fOEGMA/fDMAEMA 7.7/92.3 mol-% (or 14/86 w-%), final composition: fOEGMA/fDMAEMA
249
12.5/87.5 mol-% (or 21.5/78.5 w-%). The purified core crosslinked star polymer was then
250
analyzed by GPC (Mn,
251
solubilized in methanol and dialyzed with acidic water (pH = 3.0) for 24 hours, and then further
252
dialyzed using water (pH = 6.5) for 48 hours. Finally, the freeze dried polymer was analyzed by
253
NMR and FTIR.
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Physicochemical characterization of star-POEGMA polymers.
255
Gel permeation chromatography (GPC) measurements. DMAc GPC analyses of the
256
polymers were performed in N,N-dimethylacetamide [DMAc; 0.03% w/v LiBr, 0.05% 2, 6–di-
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butyl-4-methylphenol (BHT)] at 50 °C (flow rate = 1 mL.min-1) using a Shimadzu modular
258
system comprised of an SIL-10AD auto-injector, a PL 5.0-mm bead-size guard column (50 × 7.8
259
mm) followed by four linear PL (Styragel) columns (105, 104 and 103). A RID-10A differential
260
refractive-index detector was used. Calibration was achieved using commercial poly(methyl
261
methacrylate) and polystyrene standards ranging from 500 to 106 g/mol. The star polymer
262
molecular weight was determined using poly(methyl methacrylate) calibration. The star polymer
263
solutions were filtered before analysis using 0.45 µm filter.
264
Nuclear magnetic resonance (NMR). The structures of the polymers which were synthesized
265
were analyzed by NMR spectroscopy as described previously by Boyer et al. 18.
266
UV-visible spectroscopy. UV-visible spectra were recorded using methods described previously
267
by Boyer et al. 18.
GPC
= 120,000 g/mol and PDI = 1.35) and by NMR. The polymer was
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Dynamic light scattering (DLS). DLS measurements were performed as described previously
269
by Boyer et al.
270
influence of larger aggregates (Table 1). Intensity and volume distributions are also presented in
271
Figure S16. The polydispersity index (PDI) was used to describe the width and size distribution
272
of star polymers with and without siRNA using the DTS software along with a Cumulants
273
analysis of the measured intensity autocorrelation function; it is related to the standard deviation
274
of the hypothetical Gaussian distribution (i.e. PDI = s2/ZD2, where s is the standard deviation and
275
ZD is the Z average mean size).
276
Transmission electron microscopy (TEM). The size and shape of the star-POEGMA polymers
277
were examined using a transmission electron microscope (TEM, JEOL1400) at an accelerating
278
voltage of 100 kV. The star-POEGMA polymers were dispersed in water (1 mg/mL). The
279
solution was deposited onto 200 mesh, holey film, copper grid (ProSciTech) and dried at room
280
temperature for 4 hours before analysis.
281
siRNA binding to star-POEGMA polymers. Agarose gel electrophoresis was used to assess
282
the ability of star polymers (star 1, star 2, star 3) to complex with siRNA as described 18.
283
Biological characterization of star-POEGMA polymers.
284
Cell culture. The human pancreatic cancer cell line MiaPaCa-2 was maintained in DMEM
285
culture medium supplemented with 10% fetal calf serum, 2.5% horse serum, and 2 mM of L-
286
glutamine as described 24-26. Human HPAF-II pancreatic cancer cells were grown in DMEM with
287
10% fetal calf serum and 2mM of L-glutamine as described
288
human pancreatic ductal epithelial (HPDE) cells (a kind gift from Ming Tsao, Ontario Cancer
289
Institute) were grown in keratinocyte-serum-free (KSF) medium supplemented with 50 mg/ml
18
. The number-average hydrodynamic particle size was reported to reduce the
13 ACS Paragon Plus Environment
24-26
. Normal non-tumorigenic
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bovine pituitary extract (BPE) and 5 ng/ml epidermal growth factor (EGF) as previously
291
described 24, 27. All cells were regularly tested for mycoplasma and were negative.
292
Toxicity analysis. The toxicity profile of star POEGMA-siRNA complexes were examined in
293
MiaPaCa-2 (1.1×105) cells. In brief, cells were plated into 6-well plates the day (16 hours) before
294
transfection. The next day, cells were transfected with star, star 1, star 2 or star 3 at increasing
295
w/w ratios with siRNA (100nM). Cells incubated in cell culture media alone served as controls.
296
Cells were trypsinized, collected, and trypan blue exclusion studies were performed to determine
297
the number of viable cells 24 hours post-transfection.
298
siRNA transfection. To examine star-POEGMA-siRNA gene silencing activity, MiaPaCa-2 and
299
HPAF-II cells were transfected with siRNA targeted against the microtubule protein, βIII-tubulin
300
(encoded by the TUBB3 gene) which is expressed at high levels in pancreatic cancer cells
301
Briefly, cells were seeded into 6-well plates (1.1×105) the day prior to transfection. Cells were
302
then transfected with increasing amounts of star-POEGMA-siRNA complexes [8:1 – 30:1 (w/w)
303
ratio
304
GUACGUGCCUCGAGCCAUUUU-3′, antisense: 5′-UUCAUGCACGGAGAGCUCGGUAA-
305
3′.
306
GCUAUGGCUGAAUACAAAUUUU-3′, antisense: 5′-UUCGAUACCGACUUAUGUUUAA-
307
3′ or cells transfected with TUBB3 siRNA (also referred to as βIII-tubulin siRNA) complexed to
308
Lipofectamine 2000 (L2K) served as positive and negative controls respectively. Total RNA and
309
whole cell lysates were collected 72 hours post-transfection, and βIII-tubulin mRNA and protein
310
levels measured using qPCR and western blotting as described 24.
with
Cells
siRNA].
treated
with
TUBB3
siRNA
non-silencing
(100nM)
(Control)
siRNA
14 ACS Paragon Plus Environment
sense
sense
strand:
strand:
24, 28
.
5′-
5′-
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Intracellular uptake. To observe the cellular uptake and pattern of distribution of star-
312
POEGMA-siRNA complexes, MiaPaCa-2 cells were seeded into 8 well chambers slides
313
(1.2×103 cells) the day prior to transfection. The next day, cells were transfected with
314
fluorescently labeled (AlexaFlour-488, green) siRNA (100 nM) complexed to star-POEGMA
315
polymers (star 1, star 2, star 3) for 4 hours at 37°C. Cells transfected with fluorescent siRNA
316
complexed to L2K or fluorescent siRNA by itself served as positive and negative controls
317
respectively. Twenty four hours post-transfection, cells were incubated with 1 µM
318
LysoTracker® (diluted with culture medium) for 1 hour. The cells were washed 3 times in warm
319
PBS for 5 minutes, and then fixed with 4% paraformaldehyde for 3 minutes. Slides were
320
mounted using ProLong® Gold Antifade Reagent with DAPI. Uptake of siRNA was visualized
321
as previously described by Boyer et al. 18.
322
Real-time PCR (qPCR). βIII-tubulin (TUBB3) mRNA expression in MiaPaCa-2 and HPAF-II
323
cells was measured using qPCR as described
324
gene 18S (18S Quantitect primer assays, Qiagen).
325
Western blotting. Seventy two hours post-transfection with star-POEGMA-βIII-tubulin siRNA,
326
MiaPaCa-2 and HPAF-II cells were harvested and βIII-tubulin and GAPDH expression was
327
measured in whole cell lysates as previously described 24.
328
Inhibition of endocytosis. To examine which endocytic pathways may be involved in the
329
internalization of star-POEGMA-siRNA, MiaPaCa-2 cells were plated into 8 well chambers
330
slides (1.2×103 cells) the day before transfection. The next day, MiaPaCa-2 cells were incubated
331
with a clathrin-dependent inhibitor chlorpromazine (5 µg/ml) or two different clathrin-
332
independent inhibitors, methyl-β-cyclodextrin (MβCD, 5 mM) and genestein (200 µM) for 2
24
. All data were normalized to the housekeeping
15 ACS Paragon Plus Environment
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333
hours. The specificity and effectiveness of each inhibitor was confirmed as previously described
334
by our laboratory
335
siRNA (red) complexed to star-POEGMA polymers (star 1, star 2, star 3) for 1 hour at 37°C. The
336
nucleus was then labeled with Hoechst 33342 (blue). Live cell images were taken to visualize
337
siRNA uptake using a Zeiss LSM 780 confocal microscope.
338
Pancreatic cancer mouse models. i) Subcutaneous model: Eight-week old BALB/c nude mice
339
were used. All animal experiments were approved by the Animal ethics committee, UNSW
340
Australia (ACEC 13/130B). In brief, 4x106 MiaPaCa-2 cells were injected subcutaneously into
341
the flank of mice as previously described
342
were randomized into treatment groups and administered intratumorally with star 3-βIII-tubulin
343
siRNA (2mg/kg) twice weekly for 2 weeks. Mice injected with star 3-control siRNA served as
344
controls. Tumor size was measured twice weekly as previously described
345
experiment, tumors were harvested and RNA and protein lysates prepared as previously
346
described
347
Bioanalyzer with an RNA integrity number (RIN) a value >7. βIII-tubulin expression was
348
measured by qPCR, western blotting and immunohistochemistry as described
349
model: Eight-week old BALB/c nude mice were used. In brief, human pancreatic cancer cells
350
(MiaPaCa-2 and HPAF-II) were xenografted orthotopically into the tail of the pancreas as we
351
have described previously 24-26.
352
Star 3-siRNA biodistribution in Vivo. To examine the biodistribution of siRNA complexed to
353
star 3 in vivo, mice with orthotopic pancreatic MiaPaCa-2 (6 weeks post-tumor cell implantation)
354
or HPAF-II (3 weeks post-tumor implantation) tumors were administered (via the tail vein) with
355
star 3 complexed to fluorescently-labeled siRNA (AlexaFluor-647, Red). Mice injected with
24
29
. Subsequently, the cells were transfected with AlexaFlour-647 labeled
18
. Once tumors reached the size of ≥50 mm3, mice
18
. At the end of the
. Total RNA integrity was confirmed using an Agilent Technologies 2100
16 ACS Paragon Plus Environment
24
. ii) Orthotopic
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PBS or siRNA alone served as controls. One, four and twenty-fours post-injection mice were
357
humanely euthanized and hearts, lungs, livers, spleens, kidneys and pancreatic tumors were
358
collected and infrared fluorescence measured using the IVIS imaging system as described
359
After imaging, pancreatic tumor tissue was snap-frozen in OCT embedding media and siRNA
360
uptake
361
immunofluorescence staining and confocal microscopy.
362
Gene-silencing activity of star 3 in vivo. To examine the gene-silencing activity of star 3-βIII-
363
tubulin in vivo, MiaPaCa-2 pancreatic tumors were established as described above. Six-weeks
364
post-tumor cell injection mice were randomized into treatment groups and administered
365
systemically (via the tail vein) with star 3-βIII-tubulin siRNA (4mg/kg) once daily for 3 days.
366
Mice treated with control siRNA served as controls. Twenty four hours after the final injection
367
pancreatic tumors were harvested and βIII-tubulin expression measured by qPCR, western
368
blotting and immunohistochemistry as described 24.
369
Statistics. Data are presented as the means of at least three independent experiments ± standard
370
error of the mean (SEM) (error bars). Graphpad Prism-6 was used to perform ANOVA or paired
371
two-tailed Student’s t tests followed by Tukey’s or Dunnet post tests were used to measure
372
statistical differences between experimental and control groups, with p < 0.05 considered
373
statistically significant.
and
extravasation
from
tumor
vessels
in
tissue
374
17 ACS Paragon Plus Environment
sections
visualized
24
.
by
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375
RESULTS AND DISCUSSION
376
Synthesis and characterization of star polymers. The core crosslinked star-POEGMA
377
polymers were prepared using an arm-first approach and living radical polymerization
378
(reversible addition fragmentation chain transfer polymerization, RAFT) 30-32. In a first step, the
379
synthesis of poly[oligo(ethylene glycol) methyl ether methacrylate] (POEGMA) and
380
poly(dimethylaminoethyl methacrylate), (PDMAEMA) was carried out using 4-cyanopentanoic
381
acid dithiobenzoate as the chain transfer agent and 2,2’-azobisisobutyronitrile (AIBN) as the
382
radical initiator. The chosen POEGMA polymer is closely related to poly(ethylene glycol) (PEG)
383
and has similar low-fouling properties. The polymerizations were performed for 14 hours at 65oC
384
to yield a monomer conversion of around ~70%. The ratio between the monomer and RAFT
385
agent was varied to control the molecular weight of polymers. PDMAEMA with two different
386
molecular weights, 5,100 and 10,700 g/mol and POEGMA with a molecular weight of 11,500
387
g/mol were prepared with a narrow molecular weight distribution (PDI < 1.20) (Figure S1-S3).
388
After several rounds of purification by precipitation, homopolymer chains were extended using a
389
diacrylamide monomer [(N,N'-bis(acryloyl)cystamine)] as a crosslinker, AIBN as the initiator
390
and dimethylaminoethyl acrylate (DMAEA) as a co-monomer at 70oC in toluene for 24 hours
391
(Figure S4). To obtain the greatest incorporation of arm into the star polymers with the lowest
392
molecular weight distribution, we used a [Arm]:[DMAEA]:[crosslinker] ratio of ~ 1:4:8. High
393
monomer and crosslinker conversion (≥85% for both monomers) were observed by NMR
394
analysis after 24 hours (Figure S5 exhibits a typical NMR of unpurified star polymer). GPC
395
analysis showed the formation of high molecular weight polymer, which confirmed the
396
formation of core crosslinked star polymers, but also some residual arms (Figures S6-S8). After
397
additional purification by precipitation in petroleum ether/diethyl ether mixture (the composition
398
is optimized according to the star) to remove unreacted arm, the different star-POEGMA 18 ACS Paragon Plus Environment
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399
polymers were further characterized by NMR, FTIR and GPC to confirm their structures. Three
400
different star polymers [Star 1 (48 mol-% POEGMA with short-cationic side arms), Star 2 (51
401
mol-% POEGMA with long-cationic side arms) and Star 3 (12.5 mol-% POEGMA with long-
402
cationic side arms)] were obtained (Figure 1). GPC demonstrated the synthesis of star-POEGMA
403
polymers with a low molecular weight distribution (PDI < 1.35) (Figure 2A and Table 1), whilst
404
NMR confirmed the presence of (CH3)2N (DMAEMA) and OCH3 (POEGMA) groups at 2.3
405
ppm and 3.3 ppm, respectively (Figures S9-S11). The molar composition was determined using
406
the following equation: f
407
IOCH3correspond to the dimethylamino group (before quaternization) at 2.3 ppm and methoxy
408
groups (OCH3) at ~3.4 ppm, respectively (Figures S9-S11). FTIR showed the incorporation of
409
crosslinker by the characteristic amide band at 1,660 cm-1, while ether (O-C) and tertiary amine
410
(N-C) bands appeared at 1,150 and 1,230 cm-1 (Figure S12). Subsequently, the star-POEGMA
411
polymers were quaternized using an acidic aqueous solution ([HCl] = 10-3M, pH = 3.0). After
412
purification by dialysis to remove unreacted HCl, the star-POEGMA polymers were freeze dried
413
and analyzed by NMR using deuterium oxide (Figure 2B and Figures S13-S15) and by FTIR
414
(Figure 2C). Figure 2B showed the presence of quaternized tertiary amine at 2.9 ppm, while
415
FTIR confirmed the presence of ester [(C=O)O], amide [(C=O)N], quaternized tertiary amine
416
(N-C) and ether (O-C) bands at 1,730, 1,650, 1,230 and 1,150 cm-1 (Figure 2C). After re-
417
dispersion in water, we measured the size of the star-POEGMA polymers using dynamic light
418
scattering. All three star-POEGMA polymers were soluble in water and displayed sizes ranging
419
from 25-35 nm (±5-10 nm) (Table 1). Figure 2D displays the number distribution, while Figure
420
S16 shows the volume and intensity distribution, and the presence of small aggregates.
421
Transmission electron microscopy confirmed the formation of small spherical nanoparticles
DMAEMA
= (I(CH3)2/6)/ [(IOCH3 /3) + (I(CH3)2/6)], where I(CH3)2 and
19 ACS Paragon Plus Environment
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422
(Figure 2E). Collectively, these results demonstrated the successful synthesis of three star
423
polymers with different structural properties including, length of cationic side-arms and
424
percentage incorporation of POEGMA.
425
siRNA binding efficiency of star-POEGMA polymers. To examine how the length of the
426
cationic side-arms and percentage of POEGMA would effect star polymer capacity to bind
427
siRNA, increasing amounts of star 1 (short cationic side-arm and 48 mol-% POEGMA), star 2
428
(long cationic side-arm and 51 mol-% POEGMA) or star 3 (long cationic side-arm and 12.5 mol-
429
% POEGMA) were mixed with siRNA. The complexes of star-POEGMA-siRNA were then
430
separated on an agarose gel. siRNA alone travelled to the cathode (bottom of gel) due to its high
431
negative charge (Figure 3A-C). siRNA complexed to either star 1 or star 2 [18:1 (w/w) ratio] did
432
not migrate suggesting that complexation between the siRNA and the star-POEGMA polymers
433
had been achieved (Figure 3A and 3B). Star 3 complexed with siRNA [10:1 (w/w) ratio] more
434
readily compared to star 1 and star 2 (Figure 3C). Indeed, the amount of star 3 needed to
435
complex siRNA was not too dissimilar to star polymers without POEGMA (star) (Figure 3C).
436
Previously, we had shown that star complexed siRNA at an 8:1 (w/w) ratio
437
difference in siRNA binding efficiency between the POEGMA star polymers (star 1, star 2, star
438
3) and non-POEGMA star polymers (star) was most likely due to steric hindrance of POEGMA
439
and overall reduction in net positive surface charge due to the presence of the POEGMA. For
440
example, star polymers without POEGMA had a zeta-potential of +50 mV 18, while, star 1 had a
441
zeta potential of +18 mV (±8 mV), star 2 and star 3 +25 mV (±10 mV) (Table 1). After
442
complexation with siRNA, the zeta potential of all three star-POEGMA polymers decreased to
443
+9 mV (±4 mV) for star 1, +18 mV (±8 mV) for star 2, and +12 mV (±5 mV) for star 3,
444
indicating that the siRNA and star-POEGMA polymers formed a complex via an electrostatic 20 ACS Paragon Plus Environment
18
. Hence, the
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445
interaction (results not shown). Notably, the size of each star-POEGMA nanoparticle when
446
complexed to siRNA did not significantly change. Star 3 before complexing siRNA had an
447
overall size of 35 nm (±10 nm) (Table 1), and after complexing siRNA the size was slightly
448
increased to 38 nm (±10 nm) (results not shown). The size and surface charge of the star-
449
POEGMA-siRNA complexes are ideal for taking advantage of the disrupted tumor vasculature
450
observed in many different types of solid tumors. Most recently, studies have reported that
451
nanoparticle-siRNA complexes with a size between 50-100 nm, and which contain a slight
452
positive surface charge are able to penetrate solid tumors via passive delivery and the ‘enhanced
453
permeability and retention effect’ in pre-clinical animal models
454
show that star-POEGMA polymers are able to effectively self-assemble with siRNA to form
455
small uniform nanoparticles, and whilst the length of the cationic side-arm does not influence the
456
ability of star polymers to interact with siRNA, the amount of POEGMA does have an impact on
457
their ability to form a complex with siRNA.
458
Pancreatic cancer cell uptake of star-POEGMA polymers. To assess the ability of star-
459
POEGMA polymers to deliver siRNA to pancreatic cancer cells, we transfected MiaPaCa-2 cells
460
with star 1, star 2 or star 3 complexed to fluorescently labeled (AlexaFlour 488, Green) siRNA,
461
and examined its pattern of distribution 24 hours post-transfection using confocal microscopy.
462
Additionally, to assess whether siRNA could be released into the cell cytosol, we also examined
463
the co-localization of siRNA with endosomes / lysosomes using the LysoTracker®-Red stain 24
464
hours post-transfection. Confocal microscopy demonstrated that all three star-POEGMA
465
nanoparticles could deliver fluorescent siRNA into the cytoplasm of pancreatic cancer cells
466
(Figure 3D; panels I, II and III). Interestingly, lysoTracker® staining and high power
467
magnification confocal microscope images of MiaPaCa-2 cells transfected with star 3-siRNA 21 ACS Paragon Plus Environment
33-35
. Together, these results
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Page 22 of 51
468
showed that siRNA which were internalized into the cells had markedly less co-localization [as
469
indicated by free siRNA (Green)] with endosomes [(Red), indicating endosomal release)] (Figure
470
3D panel VI) when compared to siRNA delivered by star 1 or star 2 (evidenced by yellow
471
punctate dots in the cytoplasm which indicate co-localization of siRNA with endosomes) (Figure
472
3D panels IV, V). This result suggests that the physicochemical properties of star 3 (long
473
cationic side-arms and 12.5 mol-% POEGMA) may allow for more siRNA to be released from
474
within endosomes allowing it to enter the cell cytoplasm. However, it is also possible that star 3-
475
siRNA complexes may utilize different intracellular trafficking pathways compared to star 1 and
476
2 within MiaPaCa-2 cells that allow the complexes to be rapidly disassembled and/or degraded
477
or recycled by endosomal membrane receptors. Future work in our laboratory will further
478
characterize the internalization and trafficking processes of star 3 in pancreatic cancer cells.
479
Cell toxicity profile of star-POEGMA polymers. Based on our data showing that the
480
incorporation of POEGMA did not adversely affect the ability of star polymers to interact with
481
siRNA and deliver it to pancreatic cancer cells, we next examined if the presence of POEGMA
482
could influence their cytotoxicity profile. MiaPaCa-2 cells were transfected with increasing
483
amounts of star 1, star 2 or star 3 complexed to non-functional siRNA (100 nM) [8:1 – 30:1
484
(w/w) with siRNA]. As a comparison, cells were transfected with increasing concentrations (w/w
485
ratio with siRNA) of non-POEGMA star polymers bound to siRNA (star). The viability of the
486
cells was assessed 24 hours post-transfection by phase contrast microscopy (data not shown) and
487
by analysis of cell counting using trypan blue. Previously, we had shown that star polymers
488
without POEGMA when complexed to siRNA were non-toxic in cancer cells at an 8:1 (w/w)
489
ratio
490
cells (Figure 4A-C). However, at the higher concentrations, star polymers without POEGMA
18
. We confirmed this result showing at 8:1 (w/w) ratio, star was non-toxic to MiaPaCa-2
22 ACS Paragon Plus Environment
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(star) showed marked toxicity in the cancer cells with a 70% decrease in cell viability at the 20:1
492
(w/w) ratio after 24 hours (Figure 4A-B). In contrast, both star 1 and star 2 complexed to siRNA
493
displayed no toxicity at the 20:1 (w/w) ratio (Figure 4-B). At 30:1 (w/w) there was no toxicity in
494
MiaPaCa-2 cells transfected with star 1-siRNA, and only a very slight decrease (≈15%) in cell
495
viability in cells transfected with star 2-siRNA (Figures 4A-B). In contrast, a 90% decrease in
496
cell viability was observed in cells treated with the star polymers without POEGMA complexed
497
to siRNA (Figure 4A-B). Star 3 was also non-toxic at all of the examined concentrations [8:1 –
498
18:1 (w/w)] (Figure 4C). Similar results were obtained using a colorimetric cell proliferation
499
assay (results not shown). These results are in accordance with a previous study reported by Cho
500
et al.
501
copolymerization (ATRP) and containing a short PEG block (2KDa) were also less toxic in cells
502
when compared to cationic nanoparticles. The increased toxicity observed with star polymers
503
without POEGMA at the higher concentrations is not unexpected and is typical for most highly
504
charged cationic nanoparticles. Both poly(amidoamine) (PAMAM) dendrimers and highly
505
branched polyethylenimine (PEI) polymers possess positively charged surface groups, and have
506
been reported to destabilize cell surface membranes leading to mitochondrial-mediated cell death
507
36, 37
508
significantly improves their cytotoxic profile.
509
Star-POEGMA-siRNA gene silencing activity in pancreatic cancer cells. To determine if
510
star-POEGMA nanoparticles were able to release siRNA into the cytosol of pancreatic cancer
511
cells and induce post-transcriptional gene silencing, we transfected MiaPaCa-2 cells with
512
increasing amounts of star 1, star 2 and star 3 complexed with siRNA (100nM) targeted against
513
the microtubule protein βIII-tubulin. At an 8:1 (w/w) ratio with βIII-tubulin siRNA both star 1
12
which showed that star polymers synthesized using atom transfer radical
. Together, these results demonstrate that the incorporation of POEGMA into star polymers
23 ACS Paragon Plus Environment
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Page 24 of 51
514
and star 2 did not silence βIII-tubulin expression (Figure 4D-E). This result is expected based on
515
the fact that both nanoparticles failed to complex with siRNA at the 8:1 (w/w) ratio (Figure 3A-
516
B). However, at the 30:1 (w/w) ratio, star 1-βIII-tubulin siRNA significantly silenced βIII-
517
tubulin gene expression in MiaPaCa-2 cells by 44% (p50% (p
