A Novel Disulfide-Containing Polycationic Amphiphile : 1 , 28-Di [ ( cholest-5-en-3 β-yl ) disulfanyl ]-4 , 25-dioxo-3 , 8 , 12 , 17 , 21 , 26-hexaazaoctacosane Tetrahydrochloride

The absence of highly effective delivery systems is a major challenge for gene therapy. Our work was aimed at the development of novel cationic liposomes possessing high transfection efficiency. For this purpose, a novel disulfide polycationic amphiphile 2S4 was synthesized. Cationic liposomes based on 2S4 and a helper lipid DOPE were formed by the thin film hydration method and exhibited effective plasmid DNA delivery into the HEK293 cells, with a transfection activity superior to that of the commercial agent Lipofectamine® 2000. Our results suggest that the polycationic amphiphile 2S4 is a promising candidate for in vitro nucleic acid delivery.


Introduction
Gene therapy is an attractive tool for the treatment of both inherited [1,2] and acquired diseases [3,4] and is based on the delivery of therapeutic nucleic acid (NA) into cells.Moreover, DNA delivery has been used for effective induction of both cellular and humoral immunity against the encoded antigen [5].Nucleic acid delivery requires a special vehicle to protect NA against nucleases and to help them pass through different intracellular and extracellular barriers.The most attractive and safe delivery vehicles are the non-viral ones, such as cationic liposomes (CLs).Despite their advantages, including safety, low cost, and the ability to be produced at scale, CLs have inadequate delivery (also called transfection) efficiency [6].This fact induces the development of novel liposomal systems.CLs are formed from cationic amphiphiles (CAs) and the structure of CAs has a crucial influence on delivery efficiency.Typical CAs consist of hydrophobic and hydrophilic domains, a connecting linker, and a spacer that maintains the steric arrangement of domains [6,7].In order to increase transfection efficiency, modification of the CA structure with labile stimuli-responsive groups may be performed.Intracellular stimuli cause CA degradation which, in turn, can enhance NA release from the liposomes/NA complexes and stimulate endosomal escape [8].For example, a disulfide linker is degradable by intracellular reducing agents such as glutathione (GSH) [9].
Recently, Zhao et al. designed disulfide CAs based on a polar amino acid head and tocopherol, with the disulfide bond introduced as a cystamine moiety [10].The transfection efficiency of these CAs with respect to HEK293 cells was comparable to that of the commercial agent Lipofectamine ® 2000.High transfection efficiency both in vitro and in vivo was demonstrated by a disulfide CA based on lysine and arginine [11].A number of disulfide CAs based on cholesterol have been synthesized and have demonstrated delivery efficiency comparable with that of commercial agents.CAs with a polyamine cationic domain (lysine or triethylenetetramine) were the most effective ones with respect to COS-7 cells [12].Redox-sensitive gemini CAs based on thiocholesterol with a flexible hydrophilic spacer and ether linkers were the most effective for hard-to-transfect HaCaT cells [13].Cationic lipophosphoramidates were also modified by disulfide linkers and demonstrated more effective NA delivery compared to Lipofectamine ® [14].It is also known that the location of a disulfide bond location have a strong effect on the transfection efficiency [15].Recently, we have developed a polycationic gemini amphiphile 2X3 with a hexamethylene spacer and a carbamoyl linker (Figure 1) and have demonstrated its remarkably high transfection efficiency, which is superior to that of Lipofectamine ® 2000 [16].Here we studied the influence of the disulfide groups incorporated into the CA molecule on the transfection efficiency of CLs containing such CA.
In this work, we designed and synthesized a novel polycationic gemini amphiphile 2S4 (Figure 1) with two disulfide linkers placed close to the hydrophobic domains of the CA.We believe that disulfide groups degradable in the presence of reducing agents should contribute to better NA release into the cytosol.We also evaluated the physicochemical properties and transfection efficiency of liposomes composed of 2S4 in comparison with non-redox-sensitive 2X3 CLs and Lipofectamine ® 2000.2000.High transfection efficiency both in vitro and in vivo was demonstrated by a disulfide CA based on lysine and arginine [11].A number of disulfide CAs based on cholesterol have been synthesized and have demonstrated delivery efficiency comparable with that of commercial agents.CAs with a polyamine cationic domain (lysine or triethylenetetramine) were the most effective ones with respect to COS-7 cells [12].Redox-sensitive gemini CAs based on thiocholesterol with a flexible hydrophilic spacer and ether linkers were the most effective for hard-to-transfect HaCaT cells [13].Cationic lipophosphoramidates were also modified by disulfide linkers and demonstrated more effective NA delivery compared to Lipofectamine ® [14].It is also known that the location of a disulfide bond location have a strong effect on the transfection efficiency [15].Recently, we have developed a polycationic gemini amphiphile 2X3 with a hexamethylene spacer and a carbamoyl linker (Figure 1) and have demonstrated its remarkably high transfection efficiency, which is superior to that of Lipofectamine ® 2000 [16].Here we studied the influence of the disulfide groups incorporated into the CA molecule on the transfection efficiency of CLs containing such CA.
In this work, we designed and synthesized a novel polycationic gemini amphiphile 2S4 (Figure 1) with two disulfide linkers placed close to the hydrophobic domains of the CA.We believe that disulfide groups degradable in the presence of reducing agents should contribute to better NA release into the cytosol.We also evaluated the physicochemical properties and transfection efficiency of liposomes composed of 2S4 in comparison with non-redox-sensitive 2X3 CLs and Lipofectamine ® 2000.

Synthesis of 2S4
To obtain the target amphiphile 2S4, we synthesized a hydrophilic component (4), a hydrophobic component (6) containing disulfide linker, and then combined them into a single molecule (Scheme 1).The hydrophilic component is a dicarboxylic derivative of spermine (4), which was obtained through a number of synthetic steps.Firstly, a regioselectively protected derivative of spermine (1) was synthesized as described previously [17].Alkylation of 1 was performed in the Fukuyama reaction conditions [18] with ethyl 4-bromobutyrate to give the compound 2, which was isolated by column chromatography with 76% yield.Desulfonylation of 2 performed by the treatment with thiophenol in the presence of potassium carbonate afforded amine 3 in 18% yield.To avoid side reactions and to facilitate purification in the following steps, secondary amino groups of 3 were blocked with Boc2O in the presence of TEA.The resulting fully protected diester was hydrolyzed with NaOH in the methanol-water solution.The desired dicarboxylic derivative of spermine 4 was isolated with 49% yield.
Synthesis of the hydrophobic component with the disulfide linker was performed via a thioldisulfide exchange reaction [19].Direct thiol-disulfide exchange often proceeds with a low yield of the desired disulfide.Therefore, a two-step synthesis through an appropriate intermediate disulfide is preferable.To realize this synthetic approach, we synthesized a 2-[(cholest-5-en-3βyl)disulfanyl]pyridine by reacting thiocholesterol (5) with 2,2′-dithiodipyridine [20].However, a subsequent reaction of the disulfide obtained with 2-aminoethanethiol did not lead to the desired disulfide 6. Intrigued by that, we performed a direct reaction between thiocholesterol (5) and

Synthesis of 2S4
To obtain the target amphiphile 2S4, we synthesized a hydrophilic component (4), a hydrophobic component (6) containing disulfide linker, and then combined them into a single molecule (Scheme 1).The hydrophilic component is a dicarboxylic derivative of spermine (4), which was obtained through a number of synthetic steps.Firstly, a regioselectively protected derivative of spermine (1) was synthesized as described previously [17].Alkylation of 1 was performed in the Fukuyama reaction conditions [18] with ethyl 4-bromobutyrate to give the compound 2, which was isolated by column chromatography with 76% yield.Desulfonylation of 2 performed by the treatment with thiophenol in the presence of potassium carbonate afforded amine 3 in 18% yield.To avoid side reactions and to facilitate purification in the following steps, secondary amino groups of 3 were blocked with Boc 2 O in the presence of TEA.The resulting fully protected diester was hydrolyzed with NaOH in the methanol-water solution.The desired dicarboxylic derivative of spermine 4 was isolated with 49% yield.
Synthesis of the hydrophobic component with the disulfide linker was performed via a thiol-disulfide exchange reaction [19].Direct thiol-disulfide exchange often proceeds with a low yield of the desired disulfide.Therefore, a two-step synthesis through an appropriate intermediate disulfide is preferable.To realize this synthetic approach, we synthesized a 2-[(cholest-5-en-3β-yl)disulfanyl]pyridine by reacting thiocholesterol (5) with 2,2 -dithiodipyridine [20].However, a subsequent reaction of the disulfide obtained with 2-aminoethanethiol did not lead to the desired disulfide 6. Intrigued by that, we performed a direct reaction between thiocholesterol (5) and cystamine dihydrochloride, which resulted in compound 6 with high yield.Thiol-disulfide exchange is a reverse reaction and the equilibrium Molbank 2018, 2018, M981 3 of 9 position appear to be depended from the nucleophilicity of starting and resulting thiols.We believe that the similar nucleophilicity of both 2-aminoethanethiol and pyridine-2-thiol in the first thiol-disulfide reaction did not favor the formation of the desire product 6.
A key step in the synthesis was the condensation of hydrophilic ( 4) and hydrophobic (6) components.The reaction was carried out in the presence of a coupling reagent EEDQ (2-ethoxy-1ethoxycarbonyl-1,2-dihydroquinoline) and resulted in compound 7, which was purified by column chromatography with 84% yield.The removal of Boc protecting groups by 3 M HCl in dioxane produced the target amphiphile 2S4 with 91% yield after recrystallization from ethanol and diethyl ether.
cystamine dihydrochloride, which resulted in compound 6 with high yield.Thiol-disulfide exchange is a reverse reaction and the equilibrium position appear to be depended from the nucleophilicity of starting and resulting thiols.We believe that the similar nucleophilicity of both 2-aminoethanethiol and pyridine-2-thiol in the first thiol-disulfide reaction did not favor the formation of the desire product 6.
A key step in the synthesis was the condensation of hydrophilic ( 4) and hydrophobic (6) components.The reaction was carried out in the presence of a coupling reagent EEDQ (2-ethoxy-1ethoxycarbonyl-1,2-dihydroquinoline) and resulted in compound 7, which was purified by column chromatography with 84% yield.The removal of Вос protecting groups by 3 М HCl in dioxane produced the target amphiphile 2S4 with 91% yield after recrystallization from ethanol and diethyl ether.

Cationic Liposomes and Their Transfection Efficiency
Based on the disulfide CA 2S4 and a zwitterionic helper lipid DOPE (1,2-dioleoyl-sn-glycero-3phosphoethanolamine), CLs were prepared at lipid molar ratio of 1:1 by the thin film hydration method.Nonredox-sensitive 2X3 based CLs was prepared in the same manner and used as a positive control (here and thereafter referred as 2S4 and 2X3 CLs).The hydrodynamic diameter and the polydispersity index (PI) of 2S4 CLs determined by dynamic light scattering was 440 nm and 0.254, respectively, while 2X3 CLs had the diameter of 104 nm and PI 0.313.CLs obtained were used for the delivery of a pEGFP-C2 plasmid, which encodes enhanced green fluorescent protein (EGFP), into HEK293 cells at various N/P ratios (number of polycationic amino groups of CAs per phosphate group of nucleic acids).After the CL/NA complexation the hydrodynamic diameter of 2S4 CLs decreased to 250 nm and that of 2X3 CLs (N/P 6/1) increased slightly to 120 nm.Furthermore, all CLs and their complexes with NA had a positive zeta-potential.
To estimate the cytotoxic effect of liposomes, HEK 293 cells were incubated with the liposomes under serum-free conditions.IC50 values for cationic liposomes 2X3 and 2S4 lied within the range of 30-40 μM.Preliminary data showed, that 80% of HEK 293 cells were viable at N/P ratios used for intracellular delivery of pEGFP-C2 plasmid.
Transfection experiments were performed in the presence of 10% fetal bovine serum (FBS) to mimic the in vivo conditions.As shown by flow cytometry, transfection efficiency increased with

Cationic Liposomes and Their Transfection Efficiency
Based on the disulfide CA 2S4 and a zwitterionic helper lipid DOPE (1,2-dioleoyl-sn-glycero-3phosphoethanolamine), CLs were prepared at lipid molar ratio of 1:1 by the thin film hydration method.Nonredox-sensitive 2X3 based CLs was prepared in the same manner and used as a positive control (here and thereafter referred as 2S4 and 2X3 CLs).The hydrodynamic diameter and the polydispersity index (PI) of 2S4 CLs determined by dynamic light scattering was 440 nm and 0.254, respectively, while 2X3 CLs had the diameter of 104 nm and PI 0.313.CLs obtained were used for the delivery of a pEGFP-C2 plasmid, which encodes enhanced green fluorescent protein (EGFP), into HEK293 cells at various N/P ratios (number of polycationic amino groups of CAs per phosphate group of nucleic acids).After the CL/NA complexation the hydrodynamic diameter of 2S4 CLs decreased to 250 nm and that of 2X3 CLs (N/P 6/1) increased slightly to 120 nm.Furthermore, all CLs and their complexes with NA had a positive zeta-potential.
To estimate the cytotoxic effect of liposomes, HEK 293 cells were incubated with the liposomes under serum-free conditions.IC 50 values for cationic liposomes 2X3 and 2S4 lied within the range of 30-40 µM.Preliminary data showed, that 80% of HEK 293 cells were viable at N/P ratios used for intracellular delivery of pEGFP-C2 plasmid.
Transfection experiments were performed in the presence of 10% fetal bovine serum (FBS) to mimic the in vivo conditions.As shown by flow cytometry, transfection efficiency increased with increasing N/P ratios (Figure 2).Both 2X3 and 2S4 CLs showed better transfection efficiency than Lipofectamine ® 2000.At lower N/P ratios (2/1 and 4/1), the 2S4 CLs mediated better percentage of transfected cells as well as higher mean fluorescence intensity than the 2X3 CLs.On the other hand, at higher N/P ratios, the percentage of transfected cells was similar for both 2X3 and 2S4 CLs, but mean fluorescence intensity was lower for 2S4 CLs.increasing N/P ratios (Figure 2).Both 2X3 and 2S4 CLs showed better transfection efficiency than Lipofectamine ® 2000.At lower N/P ratios (2/1 and 4/1), the 2S4 CLs mediated better percentage of transfected cells as well as higher mean fluorescence intensity than the 2X3 CLs.On the other hand, at higher N/P ratios, the percentage of transfected cells was similar for both 2X3 and 2S4 CLs, but mean fluorescence intensity was lower for 2S4 CLs.From the physicochemical point of view, the differences between the 2X3 and 2S4 CLs may be explained by the fact that CL/pEGFP-C2 complexes of 2S4 were larger (250 nm versus 120 nm) and more heterogeneous (PIs 0.369 and 0.143, respectively) as compared with CL/pEGFP-C2 complexes of 2X3 at N/P ratio of 6/1.
In this study, a novel disulfide polycationic amphiphile 2S4 was synthesized for plasmid DNA delivery.Transfection efficiency was evaluated by measuring the level of transgene expression in HEK293 cells.We demonstrated that the transfection efficiency of 2S4 CLs was higher than that of Lipofectamine ® 2000 and similar to that of nonredox-sensitive 2X3 CLs.Nevertheless, 2S4 CLs have a potential for in vitro transfection at low N/P ratios.In addition, we plan to continue the study of the redox-sensitive delivery vehicles and the influence of disulfide bond location within CA on transfection efficiency.
CH2Cl2, ТЕА, DIEA were refluxed with CaH2 and distilled prior to the reaction.EtOH was refluxed with magnesium turnings and iodine and distilled prior to the reaction.МеОН and DMF were kept over calcined molecular sieves 3 Å and 4 Å, respectively.
Column chromatography was carried out on silica gel Kieselgel 60 (0.040-0.063 mm, Merck). 1 Hand 13 C-NMR spectra were recorded on a Avance DPX-300 and Avance DRX-500 pulse Fourier transform spectrometers (Bruker, Karlsruhe, Germany) in CDCl3 unless otherwise stated.Chemical shifts were recorded in ppm on the δ scale relative to CHCl3 solvent residual peak (7.26 ppm for 1 H and 77.0 ppm for 13 C-NMR spectra).Coupling constants (J) are absolute values and recorded in Hz.Mass spectra were run on a Thermo Finnigan MAT 900XL-TRAP mass spectrometer and on a Orbitrap Fusion mass spectrometer (Thermo Scientific, Pittsburgh, PA, USA) with electrospray From the physicochemical point of view, the differences between the 2X3 and 2S4 CLs may be explained by the fact that CL/pEGFP-C2 complexes of 2S4 were larger (250 nm versus 120 nm) and more heterogeneous (PIs 0.369 and 0.143, respectively) as compared with CL/pEGFP-C2 complexes of 2X3 at N/P ratio of 6/1.
In this study, a novel disulfide polycationic amphiphile 2S4 was synthesized for plasmid DNA delivery.Transfection efficiency was evaluated by measuring the level of transgene expression in HEK293 cells.We demonstrated that the transfection efficiency of 2S4 CLs was higher than that of Lipofectamine ® 2000 and similar to that of nonredox-sensitive 2X3 CLs.Nevertheless, 2S4 CLs have a potential for in vitro transfection at low N/P ratios.In addition, we plan to continue the study of the redox-sensitive delivery vehicles and the influence of disulfide bond location within CA on transfection efficiency.
CH 2 Cl 2 , TEA, DIEA were refluxed with CaH 2 and distilled prior to the reaction.EtOH was refluxed with magnesium turnings and iodine and distilled prior to the reaction.MeOH and DMF were kept over calcined molecular sieves 3 Å and 4 Å, respectively.
Column chromatography was carried out on silica gel Kieselgel 60 (0.040-0.063 mm, Merck). 1 H-and 13 C-NMR spectra were recorded on a Avance DPX-300 and Avance DRX-500 pulse Fourier transform spectrometers (Bruker, Karlsruhe, Germany) in CDCl 3 unless otherwise stated.Chemical shifts were recorded in ppm on the δ scale relative to CHCl 3 solvent residual peak (7.26 ppm for 1 H and 77.0 ppm for 13 C-NMR spectra).Coupling constants (J) are absolute values and recorded in Hz.Mass spectra were run on a Thermo Finnigan MAT 900XL-TRAP mass spectrometer and on a Orbitrap Fusion mass spectrometer (Thermo Scientific, Pittsburgh, PA, USA) with electrospray ionization (ESI).Melting points were determined on a IA9100 digital melting point apparatus (Electrothermal, Stone, Great Britain).

Preparation of cationic liposomes (CLs).
CLs were prepared by hydrating of thin lipid films.Briefly, polycationic amphiphile and lipid helper 1,2-dioleoyl-sn-glycero-3-phosphoethanolamine (DOPE, Avanti Polar Lipids, Alabaster, AL, USA) were dissolved at a molar ratio of 1:1 in a mixture of CHCl 3 and CH 3 OH.Organic solvents were removed in vacuo.The lipid film obtained was dried for 4 h at 0.1 Torr to remove residual organic solvents.The dried lipid film was hydrated using deionized MilliQ water at 4 • C overnight, the resulting liposomal dispersion was sonicated for 15 min at 70-75 • C in a bath-type sonicator (Bandelin Sonorex Digitec DT 52H, Berlin, Germany), filtrated through a 0.45 µm pore polycarbonate membrane, flushed with argon and stored at 4 • C. The final polycationic amphiphile concentrations were 1 mM.
Preparation of CL/NA complexes.Prior to their use, the complexes of the CLs and NA were formed in a serum-free Opti-MEM medium (Invitrogen, Waltham, MA, USA) by vigorous mixing of nucleic acid (0.5 µg pEGFP-C2) and liposome suspensions taken at concentrations corresponding to

Figure 2 .
Figure 2. Transfection efficacy of CL/pEGFP-C2 complexes formed at different N/P ratios: (a) Percentage of transfected cells; (b) Mean fluorescence intensity of the cell population.Lf (Lipofectamine ® 2000) and 2X3 cationic liposomes (CLs) were used as positive control.Experiments were performed in the presence of 10% FBS, each in triplicate.Standard deviation did not exceed 7-9%.

Figure 2 .
Figure 2. Transfection efficacy of CL/pEGFP-C2 complexes formed at different N/P ratios: (a) Percentage of transfected cells; (b) Mean fluorescence intensity of the cell population.Lf (Lipofectamine ® 2000) and 2X3 cationic liposomes (CLs) were used as positive control.Experiments were performed in the presence of 10% FBS, each in triplicate.Standard deviation did not exceed 7-9%.