RGD-decorated cholesterol stabilized polyplexes for targeted siRNA delivery to glioblastoma cells
- 135 Downloads
The development of an effective and safe treatment for glioblastoma (GBM) represents a significant challenge in oncology today. Downregulation of key mediators of cell signal transduction by RNA interference is considered a promising treatment strategy but requires efficient, intracellular delivery of siRNA into GBM tumor cells. Here, we describe novel polymeric siRNA nanocarriers functionalized with cRGD peptide that mediates targeted and efficient reporter gene silencing in U87R invasive human GBM cells. The polymer was synthesized via RAFT copolymerization of N-(2-hydroxypropyl)-methacrylamide (HPMA) and N-acryloxysuccinimide (NAS), followed by post-polymerization modification with cholesterol for stabilization, cationic amines for siRNA complexation, and azides for copper-free click chemistry. The novel resultant cationic polymer harboring a terminal cholesterol group, self-assembled with siRNA to yield nanosized polyplexes (~ 40 nm) with good colloidal stability at physiological ionic strength. Post-modification of the preformed polyplexes with PEG-cRGD end-functionalized with bicyclo[6.1.0]nonyne (BCN) group resulted in enhanced cell uptake and increased luciferase gene silencing in U87R cells, compared to polyplexes lacking cRGD-targeting groups.
KeywordsCancer targeting siRNA delivery Glioblastoma cRGD peptide Cholesterol modification
GBM is the most common malignant brain tumor in adults and is an incurable disease characterized by rapid tumor growth, neovascularization, and aggressive invasion throughout the brain . The standard of care (SOC) for GBM is maximal safe surgical resection followed by radiation therapy with concomitant and adjuvant temozolomide (TMZ) delivered via the established “Stupp protocol” . Notwithstanding, patients diagnosed with GBM have a devastatingly low median life expectancy of < 2 years, with SOC treatment remaining largely palliative. There is therefore an urgent need for new therapeutic modalities.
The RNA interference (RNAi) is an established therapeutic approach based on the delivery of small interfering RNAs (siRNAs) into target cells to induce sequence-specific gene silencing. While RNAi has significant potential as a therapeutic strategy in oncology [3, 4], the therapeutic utility of “unpackaged” siRNAs is limited due to their intrinsic instability and poor delivery into target tissues. Moreover, delivery in the setting of GBM is further limited by the poor penetration of drugs into the tumor due to the presence of the blood-brain and blood-tumor barriers. Targeting of integrins has been demonstrated to be a rational approach to circumvent these delivery and penetration issues. These proteins are key mediators in GBM cell growth, invasion, and angiogenesis with avβ3 and avβ5 integrin family receptors further overexpressed on the endothelial cells of tumor vessels. Cylic Arg-Gly-Asp motifs (cRGD) bind to these integrins and thus allows selective targeting. To date, several studies have demonstrated the utility of an RGD-based targeting strategy in the GBM setting .
To effectively implement RNAi as a strategy in the treatment of GBM, an effective biodegradable delivery system is essential. To this end, a number of cationic polymers have been employed for siRNA delivery, including poly(ethylene imine),  poly(l-lysine),  poly(amido amine)s , and N-(2-hydroxypropyl)-methacrylamide (HPMA)-based cationic polymers [9, 10, 11]. Moreover, poly(N-(2-hydroxypropyl)-methacrylamide) (pHPMA) has been approved for clinical use following demonstration of a favorable safety profile [12, 13]. A pHPMA derivative-p(HPMA-DMAE) has further been studied for gene delivery in ovarian cancers having the advantage of intrinsic degradable properties  and low cytotoxicity . However, an inherent problem with positively charged siRNA polyplexes is the tendency to aggregate or dissociate upon interaction with serum proteins, leading to premature siRNA release in vitro [16, 17, 18]. Currently, PEGylation of gene delivery carriers is the typical approach to improve stability and pharmacokinetic profiles . The most common strategy involves the direct introduction of PEG into the synthetic polymer chains as diblock or graft copolymer. However, the presence of PEG during complexation may influence the nucleic acid complexation and condensation capacity as well as size and morphology of formed nanoparticles, due to the anti-compaction force from PEG steric repulsion [20, 21, 22]. One alternative strategy involves post-PEGylation of the desired polyplexes, with several studies showing that this method can increase stability in vivo [23, 24, 25]. However, the presence of a PEG corona covering the surface of polyplexes also has drawbacks; it inhibits cellular uptake and endosomal escape of the siRNA complexes, potentially leading to a substantial decrease in the gene-silencing efficiency . One method to resolve this (PEG) dilemma is the linking of PEG to the siRNA complexes via disulfide bonds, enabling PEG detachment from the siRNA complex in response to changes in environmental redox potential [27, 28]. To further increase the stability of PEGylated siRNA polyplexes, additional sophisticated approaches have been explored including disulfide cross-linking , quaternary amines [30, 31], and hydrophobic interactions [20, 28, 32]. In particular, hydrophobic moieties, e.g., cholesterol, can assist the spontaneous assembly of polyplexes through hydrophobic interactions in aqueous solutions, rendering polyplexes more resistant to dissociation, eventually leading to a long longer circulation times in vivo [7, 33].
To circumvent the many challenges discussed above, we have designed and implemented a novel polymeric siRNA nanocarrier functionalized with cRGD peptide to facilitate GBM cellular uptake and mediate efficient reporter gene silencing. Herein, we describe the synthesis, characterization, and utility of ω-cholesteryl p(HPMA-r-NAS) polymers containing the reactive group NAS using RAFT polymerization. Cholesterol conjugation was performed by heating the polymer in the presence of a cholesterol-modified radical initiator, to form a stable group at the ω chain-end. After polymerization, the NAS groups of the polymer were modified with reducible azide groups containing disulfide bonds. HPMA groups were further derivatized with a cationic group (N,N′-dimethyl-aminoethanol, DMAE) coupled to the secondary hydroxyl group of HPMA via a hydrolysable carbonate ester. The resulting polymers formed small siRNA polyplexes through both polycation electrostatic interaction and siRNA and hydrophobic interaction via cholesterol. Subsequently, these polyplexes were post-modified with PEG-cRGD modified with bicyclo[6.1.0]nonyne (BCN) using copper-free click chemistry to shield surface charge and enable ligand-mediated cell binding and uptake [25, 34]. In vitro experiments showed enhanced cellular uptake of PEG-cRGD modified polyplexes, which in turn resulted in improved transfection efficiency as compared to non-PEGylated particles.
Materials and methods
N-(2-hydroxypropyl) methacrylamide (HPMA) , 2-(dimethylamino)ethyl 1H-imidazole-1-carboxylate (DMAE-CI) , and imidazole-1-sulfonyl azide hydrochloride  were synthesized as previously described. Azobis(isobutyronitrile) (AIBN), 4,4′-azobis (N,N′-cyanopentanoic acid) (V501), cholesterol, dicyclohexylcarbodiimide (DCC), 4-(dimethylamino)pyridine (DMAP), and all other reagents and solvents used in the synthesis were obtained from Sigma-Aldrich and were used without further purification. 2,5-Dioxopyrrolidin-1-yl 4-((((1R,8S,9s)-bicyclo[6.1.0] non-4-yn-9-ylmethoxy)carbonyl)amino)butanoate (BCN, SX-A1036) was purchased from Synaffix BV (Oss, The Netherlands). cRGD-azide was provided by ChinaPeptides Co.,Ltd. (Shanghai, China). Agarose multi-purpose was purchased from Roche Molecular Biochemicals (Mannheim, Germany). Six times DNA Loading Dye was purchased from Fermentas (St. Leon-Roth, Germany). SYBR Safe DNA gel stain, lipofectamine 2000, DEME/F12 medium, Opti-MEM, G418, and heat-inactivated fetal bovine serum (HI-FBS) were purchased from Life Technologies (Breda, The Netherlands). Luc2 siRNA targeted for luc2 luciferase, scrambled siRNA (siCon), and a Cy5-labeled Luc2 siRNA were obtained from Dharmacon, Inc. (Eindhoven, The Netherlands). The sequence of the sense strand of the Luc2 siRNA is 5′-GGACGAGGACGAGCACUUCUU-3′ and the antisense strand sequence is 3′-UUCCUGCUCCUGCUCGUGAAG-5′. The Cy5 fluorophore within the Cy5-labeled Luc2 siRNA was conjugated to the 3′ terminus of the anti-sense strand.
Synthesis of monomers
Synthesis of cholesteryl V501 derivative (C-V501-C)
Synthesis of 2-((2-azidoethyl) disulfanyl) ethan-1-amine hydrochloride
The synthesis procedures were similar as previously published with slight modifications (Scheme S1) . Typically, cystamine dihydrochloride salt (3.22 g, 14.3 mmol), K2CO3 (6.00 g, 43.4 mmol), and CuSO4.5H2O (35.73 mg, 143.1 μmol) were dissolved in methanol (60 mL). Imidazole-1-sulfonyl azide hydrochloride (3.00 g, 14.3 mmol) was added to the suspension and the mixture was stirred at room temperature for 12 h. Next, the mixture was concentrated by evaporation of the solvent under reduced pressure, diluted with H2O (180 mL), and extracted with DCM (3 × 120 mL). The combined organic layers were dried (MgSO4), filtered, and concentrated. Silica gel flash chromatography gave yellow waxy solids (DCM/MeOH/NH4OH, 50:2:1–80:20:1), the yield was 0.80 g (32%, Rf = 0.5). The monomer was characterized by ATR-IR and NMR δ 1H NMR (400 MHz, DMSO-d6) (Fig. S3).
Synthesis of BCN-PEG and BCN-PEG-cRGD
NH2-PEG5000-COOH (100 mg, 0.02 mmol, 1 equiv.), cyclooctyne-NHS (BCN-NHS; 9.0 mg, 0.024 mmol, 1.2 equiv.), and triethylamine (8.5 μL, 0.06 mmol, 3 equiv.) were dissolved in 1.3 mL DMSO; the reaction mixture was stirred at room temperature overnight. The final product was precipitated in cold ether twice, then dissolved in milliQ water, followed by dialysis against water (MWCO 3000, Merck Millipore, Germany) for 2 days. After filtration and freeze-drying, the BCN-PEG-COOH (BCN-PEG) was obtained as a white powder (90 mg, 85.7%). 1H NMR (400 MHz, DMSO): δ = 7.05 (s, 1H;OC(=O)NH), 7.05 (s, 1H;C=ONH), 4.52 (t, 2H; PEG-OH), 4.00 (d, 2H; BCN-CH2-O(=O)), 3.66 (t, 2H; PEG-CH2), 3.48 (bs, 440H; PEG), 3.04 (s, 2H; OCONHCH2), 2.90 (s, 2H; C=ONHCH2), 2.0–2.21 (m, 4H; CH2C(=O)NH2, alkane), 1.99 (m, 2H; NHCH2CH2), 1.69–1.41 (m, 6H; alkane), 1.54–1.13 (m, 1H; alkane), 0.80–0.71 (m, 2H; alkane).
To a solution of NH2-PEG6000-NH2 (300 mg, 0.05 mmol) in DMSO (1.5 mL), cyclooctyne-NHS (BCN-NHS 75.3 mg, 0.2 mmol, 4 equiv.), and trimethylamine (41.8 μL, 0.3 mmol, 6 equiv.) were added. The solution was subsequently stirred for 16 h at room temperature. Next, the solution was dropped into cold ether twice to precipitate the formed product. The precipitate was subsequently dissolved in 10 mL water and dialyzed against water using a membrane with a molecular weight cut off of 3000 for 2 days. After filtration and freeze-drying, BCN-PEG-BCN was obtained as a white powder (270 mg, 85.7%). Then, BCN-PEG-BCN (41.6 mg, 6.41 μmol) was dissolved in 1 mL dry DMSO, followed by the addition of cylic RGD-azide (4.0 mg, 6.41 μmol); the obtained solution was stirred for 16 h at room temperature. Next, 10 mL water was added and the product was obtained after freeze-drying. Subsequently, the product was dissolved in 5 mL water and dialyzed against water for 2 days using a membrane with a molecular weight cut off of 3000. The product was obtained in a yield of 90%. The amount of cRGD conjugated to BCN-PEG-BCN was determined using 1H NMR analysis based on the peak intensity ratio of phenyl protons of the cRGD peptide (7.0–7.2 ppm) to ethylene protons of PEG (-CH2-CH2-, 3.4–3.6 ppm) (Fig. S6). The product was analyzed by SEC (Fig. S7) and the shift of the PEG peak to a slightly shorter retention time proved that a product with higher molecular weight was obtained and thus showed the successful conjugation of cRGD and BCN-PEG. It should be noted that the applied procedure resulted in the formation of a mixture of BCN-PEG-cRGD, cRGD-PEG-cRGD, and unreacted BCN-PEG-BCN.
Synthesis of p(HPMA-r-NAS) (pHN) by RAFT polymerization
Radical cross-coupling of pHN with C-V501-C (C-pHN)
The reaction process was based on previously published methods . p(HPMA-r-NAS) (400 mg, 40.5 μmol, calculated based on the Mn(theory) = 9800 g/mol) and C-V501-C (1238 mg, 1217 μmol) were dissolved in 4 mL dry DMF, and the solution purged with argon for 30 min. Subsequently, the flask was put into the preheated oil bath (70 °C) and incubated for 4 h. A control polymer without cholesterol modification was synthesized as follows: p(HPMA-r-NAS) (100 mg, 10.1 μmol, calculated based on the Mn(theory) = 9800 g/mol) and AIBN (50 mg, 304 μmol) were dissolved in 1 mL dry DMF and heated at 70 °C for 4 h under an argon atmosphere. The product was precipitated two times in a mixture of anhydrous acetone and diethyl ether (50/50, v/v), dried in vacuo prior to 1H NMR and GPC analysis (yield 65%).
Synthesis of cholesteryl p(HPMA-DMAE-r-AEDA) (C-pHDA)
The cholesteryl copolymer (C-pHN, 300 mg) (0.56 mmol of NAS, 1.44 mmol of HPMA) was dissolved in 3 mL dry DMSO and flushed with argon for 30 min. Next, 72 mg (0.40 mmol) of 2-((2-azidoethyl) disulfanyl) ethan-1-amine hydrochloride (AEDA) was added to this solution under argon purge. Then, 340 mg (3.36 mmol) of triethylamine was injected into the reaction vessel and the solution was stirred at 35 °C. After 48 h, 84 mg (1.2 mmol) of d,l-amino-2-propanol was injected into the reaction mixture and the solution was stirred for 16 h at room temperature. The modified polymer was precipitated twice into a mixture of anhydrous acetone and diethyl ether (50/50) and dried in vacuo to get the white-colored product C-pHNA (yield 63%). The resulting polymer was then dissolved in 2 mL dry DMSO. DMAE-CI (3.4 g, 14.4 mmol) was added and the solution was flushed with argon. After 72 h of reaction at room temperature, the solution was diluted with 20 ml of 5 mM ammonium acetate buffer (pH 5) and purified with the same buffer by ultrafiltration for 24 h using a membrane with MWCO of 3000. The resulting polymer solution was filtered with 0.2-μm filter and the polymer was obtained after freeze-drying (yield 94.7 mg).
Characterization of polymer
The copolymer composition of the different polymers was determined by 1H NMR analysis performed with a Gemini 400 MHz spectrometer (Varian Associates Inc., NMR Instruments, Palo Alto, CA). The polymers were dissolved in D2O or DMSO-d6. The molecular weights and molecular weight distributions of the synthesized copolymers pHN and C-pHN were determined by gel permeation chromatography (GPC) . For the polymer C-pHNA and C-pHDA, the molecular weights and molecular weight distributions were determined by GPC using a Viscotek-GPC max (Viscotek, Oss, The Netherlands) light scattering (λ = 670 nm, right (90°) and low (7°) angle)/viscometric detection system, using a ultrahydrogel 2000, 7.8 × 300 mm column in series with a ultrahydrogel 6.0 × 40 mm guard column (waters), 0.3 M NaAc, pH 4.4, and 30% acetonitrile as eluent . The flow rate was 0.6 mL/min and the run time was 50 min. PolyCAL™ PEO standard (Mn = 24 kDa, PDI = 1.01, Malvern) was used for calibration.
Preparation and characterization of polymer/siRNA polyplexes
siRNA polyplex preparation
siRNA duplexes for target genes were purchased from IDT (Coralville, IA, USA). The siRNA polyplexes preparation process consisted of 3 consecutive steps: complexation, pegylation, and lyophilization. Briefly, for complexation, four volumes of polymer and one volume of nucleic acid both dissolved in 10 mM NaOAc buffer, pH 5, at the desired N/P ratio, were mixed by vortexing with a final siRNA concentration of 50 μg/mL. For pegylation, BCN-PEG (BCN-PEG-COOH) or BCN-PEG-cRGD as added to the polyplexes at the amount of PEG equivalent to 60 mol% of an azide of the polymer used for preparing polyplexes and left to react for 2 h at room temperature. This ratio was selected based on our prior studies, in which we investigated the optimal post-PEGylation ratio for RNA polyplexes [25, 34]. For freeze-drying of the polyplexes, sucrose was added to the polyplex formulation to a final concentration of 5% before snap-freezing in liquid nitrogen. Frozen samples were freeze-dried overnight using an Alpha 1–2 LD plus freeze-dryer (Marin Christ, Osterode, Germany).
Particle size and zeta-potential measurements
Particle sizes of the polyplexes (10 μg/mL siRNA concentration) were measured with dynamic light scattering (DLS) using an ALV CGS-3 system (Malvern Instruments, Malvern, U.K.) equipped with a JDS Uniphase 22 mW He−Ne laser operating at 632.8 nm, an optical fiber-based detector, and a digital LV/LSE-5003 correlator at 25 °C. The zeta-potential of the polyplexes was measured at 25 °C using a Malvern Zetasizer Nano-Z (Malvern Instruments, Malvern, U.K.) in 10 mM HEPES buffer. To detach PEG from C-pHDA/siRNA polyplexes, the polyplexes were incubated with 10 mM DTT at room temperature before measurement.
Gel retardation assay
Polyplexes prepared at different N/P ratios were made by adding 5 μL of polymer solution (concentrations varying between 14 and 2400 μg/mL in 10 mM HEPES, pH 7.4) to 5 μL of siRNA solution (40 μg/mL in 10 mM HEPES, pH 7.4), followed by vortexing for 5 s and the dispersions were incubated for 30 min at room temperature. For release studies with heparin, the sample prepared at an N/P of 8 (10 μL) was mixed with of 5 μL heparin sodium salt (concentrations varying between 75 and 900 μg/mL). Next, 1 μL of sodium chloride (1.54 M) was added to get a final salt concentration of 150 mM, and the samples were incubated for 10 min at room temperature . Next, the gel was analyzed by a Gel Doc XR+ system (BioRad Laboratories Inc., Hercules, CA) with Image Labsoftware.
Transmission electron microscopy
Transmission electron microscopy (TEM) was carried out on an FEI Tecnai T10 microscope from FEI Company (Eindhoven, The Netherland). Twenty microliters of polyplex dispersion of 50 μg/mL siRNA in 10 mM HEPES, pH 7.4, were placed on a carbon-coated copper grid and left to dry. The samples were stained with 2% uranyl acetate. Scale bars were added with the help of ImageJ software.
In vitro cytotoxicity and cell transfection study
Human glioblastoma cells (line U87R-GFP; gift from Peter Forsyth, Moffitt Cancer Center, FL, USA) modified with luciferase were cultured in Dulbecco’s Modified Eagles Medium (DMEM) F12 supplemented with 10% fetal bovine serum and 200 μg/mL G418 as previously described . Cells were seeded at a density of 10,000 cells per well in 96-well plate 24 h prior to polyplex addition. Cells were cultured in (10% HI FBS,) before transfection, the medium was removed and replaced with opti-MEM or culture medium containing 10% FBS. siRNA polyplexes were then added to each well at a final siRNA concentration of 100 and 200 nM. lipofectamine 2000 (Invitrogen, Karlsruhe, Germany) (Lipo) was used as positive control (100 nM siRNA, Lipo/siRNA volume/weight ratio of 3/1), and formulations containing scrambled siRNA and PBS-treated cells were used as negative controls. After a 4-h incubation, the medium was replaced with culture medium containing 10% FBS.
To determine the cytotoxicity of the polyplexes the Alamar Blue cell viability assay (Invitrogen, Karlsruhe, Germany) was carried out. Forty-four hours following transfection, the cell medium was replaced with medium containing Alamar Blue (50 nM) and incubated for 4 h. Next, 80 μL of medium from each well was then transferred into a flat-bottom 96-well plate. The relative cell metabolic activity was calculated by normalizing the absorbance at 570 nm (reference wavelength of 630 nm) with the absorbance of PBS-treated cells.
Luciferase cellular expression was measured 48 h after transfection. Cells were washed with 100 μL cold PBS and lysed with 100-μL lysis buffer. Subsequently, 50-μL luciferase assay reagent (Promega) was added to 20-μL cell lysate using a microinjector, and luminescence measured after 2 s using a white microplate, using an FLUOstar OPTIMA equipped with a luminescence light guide (BMG LabTech, Germany). To normalize for transfection efficiency, the GFP intensity was also measured. The relative luciferase activity in each well was obtained by dividing the luminescence intensity by the corresponding GFP fluorescent intensity. This activity was then normalized against the PBS-treated control samples .
Cellular uptake of polyplexes studied by flow cytometry
U87R-GFP-Luc2 cells were seeded into a 96-well plate (30,000 cells/well) and incubated with polyplexes prepared as described above using Cy5-labeled siRNA (final siRNA concentration was 100 nM, N/P ratio of 8) for 4 h at 37 °C in medium with serum incomplete sentence). For the cRGD competition study, the cells were first treated for 1 h with 200 nM cRGD before addition of polyplexes. Cells were then washed twice with ice-cold PBS. To quench the fluorescence of polyplexes associated with the cell membrane, the cells were incubated with 0.4% trypan blue-containing PBS for 5 min and washed with PBS . Following trypsinization cells were collected and suspended in PBS. Cellular uptake of siRNA polyplexes was then examined through flow cytometry with help of Canto II (BD, USA).
Confocal laser scanning microscopy studies
U87R-GFP-Luc2 cells were seeded into 96-well μClear® black plates (20,000 cells/ well) and incubated for 24 h in full medium. Polyplexes with Cy5-labeled siRNA (final siRNA concentration was 100 nM, N/P ratio of 8) were added and the cells were subsequently incubated for another 4 h at 37 °C. For the cRGD competition study, the cells were first incubated with 200 nM cRGD for 1 h before adding the polyplexes. Prior to imaging, the medium was replaced with fresh full medium containing Hoechst33342 and Lysotracker Red (Molecular Probes, Oregon, USA) for staining the nuclei and lysosomes (incubation at 37 °C for 20 min). After washing with PBS, CLSM images were recorded using Yokogawa CV7000S imager (Yokogawa group, Tokyo, Japan) equipped with a 60× water immersion objective at an excitation wavelength of 405, 488, 561, and 646 nm for Hoechst33342, GFP, Lysotracker Red, and siRNA-Cy5, respectively.
p values were determined by Student’s test with two-tailed distribution performed with the software GraphPad Prism 5 (GraphPad Software Inc. La Jolla, California). p values < 0.05 were considered as statistically significant.
Results and discussion
Synthesis and characterization of random copolymers
Characteristics of synthesized random copolymers
HPMA (% mol)a
NAS (% mol)
Control polymer P(HPMA-DMAE-r-ADAE)
The chain transfer agent (CTA) used for the polymerization typically yields a dithioester or trithioester group at the ω-end of the polymer chain, which is available for further post-polymerization functionalization [45, 46]. A radical cross-coupling reaction  between the trithiocabonate chain end and a cholesterol modified azo-initiator was used to introduce a cholesterol moiety at the ω-end of pHN (Fig. 1b). The cholesterol modified initiator was synthesized using DCC-mediated esterification of the hydroxyl group of cholesterol and carboxylic acid of V501, yielding C-V501-C in 45% yield (Fig. 1a). 1H NMR spectrum (Fig. S1a) shows the disappearance of the signal at 3.51 ppm (assigned to the methine protons of cholesterol) and appearance of a new signal at 4.60 ppm (assigned to the methine protons of C-V501-C) suggests the formation of an ester bond between cholesterol and V501. The ester bond formation was further verified by the ATR-FTIR with its absorbance at a wavenumber of 1743 cm−1 (Fig. S1b). Radical cross-coupling of pHN and C-V501-C was performed at 70 °C in DMF for 4 h (Fig. 1b). 1H NMR analysis of the obtained polymer confirmed incorporation of the cholesterol moiety as evident by the appearance of peaks at 0.61 ppm (methyl protons of cholesterol) and 5.30 ppm (methylene protons of cholesterol) in the NMR spectrum (Fig. 2a). NMR analysis further showed that around 60% of pHN chains had a cholesterol terminus. The GPC chromatogram of pHN and C-pHN showed that there was no significant change in the molecular weight distribution (Fig. 1c) and polydispersity index (Table 1), and the decrease of the UV absorbance (90%) (Fig. S2) at 309 nm (thiocarbonylthio chromophore)  demonstrates again successful cross-coupling of cholesterol to the polymer. The resulting polymer C-pHN contained 27 mol% of NAS (calculated from NMR) demonstrated that these reactive esters were not hydrolyzed, due to possible presences of traces of water, during cholesterol modification and are therefore available for further post-polymerization modification.
Formation of C-pHDA polyplexes and in vitro siRNA delivery
The effect of the presence of cholesterol in the polyplexes on siRNA transfection efficiency was evaluated in the invasive U87R-GFP-Luc2 GBM cell line, which co-expresses green fluorescence protein (GFP) and luciferase (Luc) from a bicistronic transcript. To exclude the influence of serum, the polyplexes were incubated with the cells OPTI-MEM medium without serum, which favors stability of unshielded, cationic polyplexes, and lipoplexes made with commercial agent lipofectamine 2000 (Lipo). At an N/P 8, C-pHDA polyplexes containing anti-luciferase siRNA potently silenced around 50% of the expression of luciferase, which was significantly higher than observed for the polyplexes based on pHDA (10% silencing) (Fig. 4c). The improved gene-silencing efficacy of c-PHDA polyplexes compared to pHDA polyplexes is likely caused by the smaller size (37 vs 90 nm) and higher surface charge (25 vs 16 mV) of the polyplexes, as the size and zeta potential of polyplexes strongly influence the transfection efficiency . Moreover, polyplexes prepared by pHDA and C-pHDA showed minimal cytotoxicity to U87R cells (Fig. 4d). These data again demonstrate that p(HPMA-DMAE) has an excellent cytocompatibility, in agreement with a previous study using different cell lines . In conclusion, the introduction of cholesterol into the polymer enhanced the stability of formed siRNA polyplexes and leads to smaller particle size and higher gene-silencing efficacy.
Effect of post-PEGylation of C-pHDA polyplexes with PEG-cRGD on cellular uptake and transfection efficiency
Size and zeta potential of siRNA/C-pHDA polyplexes
Zeta potential (mV)
37 ± 1
25.0 ± 2.1
56 ± 2
9.4 ± 1.2
50 ± 3
8.7 ± 0.2
We have described the synthesis, preparation, characterization, and in vitro assessment of a novel cRGD-targeting and cholesterol stabilized polyplex system for siRNA delivery in GBM. Cholesterol moieties were introduced to the ω-end of polymer chain after RAFT polymerization, followed by conjugating with cationic charge amines and azide functional groups. The resultant polymer was able to condense siRNA to form small nanoparticles size around 40 nm with improved stability. Relative to pDHA polyplexes alone, these stable and targeted c-pHDA polyplexes demonstrate improved cellular uptake in targeted U87R-GFP-Luc2 cells and mediate an efficient gene-silencing effect with a low cytotoxicity profile. These data support further investigation of these polyplexes for in vivo delivery using clinically relevant GBM models.
Bo Lou was funded by the China Scholarship Council (CSC). This work was supported in part by a Science Foundation Ireland Technology Innovation Award (15/TIDA/2963). ATB is further supported by the “GLIOTRAIN” (http://www.gliotrain.eu) award, a Horizon 2020 Research and Innovation program funded under the Marie Skłodowska-Curie ETN initiative (Grant Agreement #766069).
- 5.Hou J, Diao Y, Li W, Yang Z, Zhang L, Chen Z, et al. RGD peptide conjugation results in enhanced antitumor activity of PD0325901 against glioblastoma by both tumor-targeting delivery and combination therapy. Int J Pharm. 2016;505:329–40. https://doi.org/10.1016/j.ijpharm.2016.04.017.CrossRefGoogle Scholar
- 7.Oe Y, Christie RJ, Naito M, Low SA, Fukushima S, Toh K, et al. Actively-targeted polyion complex micelles stabilized by cholesterol and disulfide cross-linking for systemic delivery of siRNA to solid tumors. Biomaterials. 2014;35:7887–95. https://doi.org/10.1016/j.biomaterials.2014.05.041.CrossRefGoogle Scholar
- 14.Funhoff AM, Van Nostrum CF, Janssen APCA, Fens MHAM, Crommelin DJA, Hennink WE. Polymer side-chain degradation as a tool to control the destabilization of polyplexes. Pharm Res. 2004;21:170–6. https://doi.org/10.1023/B:PHAM.0000012165.68765.e6.CrossRefGoogle Scholar
- 21.Takeda KM, Osada K, Tockary TA, Dirisala A, Chen Q, Kataoka K. Poly(ethylene glycol) crowding as critical factor to determine pDNA packaging scheme into polyplex micelles for enhanced gene expression. Biomacromolecules. 2017;18:36–43. https://doi.org/10.1021/acs.biomac.6b01247.CrossRefGoogle Scholar
- 25.Lou B, De Beuckelaer A, Dakwar GR, Remaut K, Grooten J, Braeckmans K, et al. Post-PEGylated and crosslinked polymeric ssRNA nanocomplexes as adjuvants targeting lymph nodes with increased cytolytic T cell inducing properties. J Control Release. 2018;284:73–83. https://doi.org/10.1016/J.JCONREL.2018.06.010.CrossRefGoogle Scholar
- 28.Kim HJ, Oba M, Pittella F, Nomoto T, Cabral H, Matsumoto Y, et al. PEG-detachable cationic polyaspartamide derivatives bearing stearoyl moieties for systemic siRNA delivery toward subcutaneous Bxpc3 pancreatic tumor. J Drug Target. 2012;20:33–42. https://doi.org/10.3109/1061186X.2011.632010.CrossRefGoogle Scholar
- 32.Liu L, Zheng M, Librizzi D, Renette T, Merkel OM, Kissel T. Efficient and tumor targeted siRNA delivery by polyethylenimine-graft-polycaprolactone-block-poly(ethylene glycol)-folate (PEI-PCL-PEG-Fol). Mol Pharm. 2016;13:134–43. https://doi.org/10.1021/acs.molpharmaceut.5b00575.CrossRefGoogle Scholar
- 33.Kim HJ, Miyata K, Nomoto T, Zheng M, Kim A, Liu X, et al. SiRNA delivery from triblock copolymer micelles with spatially-ordered compartments of PEG shell, siRNA-loaded intermediate layer, and hydrophobic core. Biomaterials. 2014;35:4548–56. https://doi.org/10.1016/j.biomaterials.2014.02.016.CrossRefGoogle Scholar
- 37.Moraes J, Simionca I-M, Ketari H, Klok H-A. Avoiding compositional drift during the RAFT copolymerization of N-(2-hydroxypropyl)methacrylamide and N-acryloxysuccinimide: towards uniform platforms for post-polymerization modification. Polym Chem. 2015;6:3245–51. https://doi.org/10.1039/C5PY00253B.CrossRefGoogle Scholar
- 39.Shi Y, van den Dungen ET a, Klumperman B, van Nostrum CF, Hennink WE. Reversible addition–fragmentation chain transfer synthesis of a micelle-forming, structure reversible thermosensitive diblock copolymer based on the N -(2-hydroxy propyl) methacrylamide backbone. ACS Macro Lett. 2013;2:403–8. https://doi.org/10.1021/mz300662b.CrossRefGoogle Scholar
- 47.Ming W, Xiaofeng Z, Xiaojiao R, Bailiang Y, Long C, Feizhuan L, et al. Efficacy and safety of first-line chemotherapy plus bevacizumab in patients with metastatic colorectal cancer: a met. Chin Med J. 2014;127:538–46. https://doi.org/10.3760/cma.j.issn.0366-6999.20132241.Google Scholar
- 48.Oba M, Miyata K, Osada K, Christie RJ, Sanjoh M, Li W, et al. Polyplex micelles prepared from ω-cholesteryl PEG-polycation block copolymers for systemic gene delivery. Biomaterials. 2011;32:652–63. https://doi.org/10.1016/j.biomaterials.2010.09.022.CrossRefGoogle Scholar
- 52.Shin S, Kim YS, Kim J, Kwon H-M, Kim D-E, Hah SS. Sniffing for gene-silencing efficiency of siRNAs in HeLa cells in comparison with that in HEK293T cells: correlation between knockdown efficiency and sustainability of sirnas revealed by FRET-based probing. Nucleic Acid Ther. 2013;23:152–9. https://doi.org/10.1089/nat.2012.0396.CrossRefGoogle Scholar
- 57.Shayakhmetov DM, Eberly AM, Li Z-Y, Lieber A. Deletion of penton RGD motifs affects the efficiency of both the internalization and the endosome escape of viral particles containing adenovirus serotype 5 or 35 fiber knobs. J Virol. 2005;79:1053–61. https://doi.org/10.1128/JVI.79.2.1053-1061.2005.CrossRefGoogle Scholar
- 58.Chávez A, Pujol M, Haro I, Alsina MA, Cajal Y. Membrane fusion by an RGD-containing sequence from the core protein VP3 of hepatitis A virus and the RGA-analogue: implications for viral infection. Biopolymers. 2001;58:63–77. https://doi.org/10.1002/1097-0282(200101)58:1<63::AID-BIP70>3.0.CO;2-L.CrossRefGoogle Scholar
Open Access This article is distributed under the terms of the Creative Commons Attribution 4.0 International License (http://creativecommons.org/licenses/by/4.0/), which permits unrestricted use, distribution, and reproduction in any medium, provided you give appropriate credit to the original author(s) and the source, provide a link to the Creative Commons license, and indicate if changes were made.