Synthesis, Characterization, and Antimicrobial Evaluation of Random Poly(ester-Carbonate)s Bearing Pendant Primary Amine in the Main Chain.

Starting from primary amine bearing cyclic carbonate tert-butyl-(2-oxo-1,3-dioxan-5-yl) carbamate (TBODC) and caprolactone (CL), amphiphilic poly(caprolactone-ran-amino trimethyl carbonate)s (P(CL-ran-ATC)s) random copolymers with controlled molecular weight and composition were synthesized via ring opening polymerization (ROP) and deprotection, using stannous octoate (Sn(Oct)2) as catalyst and benzyl alcohol (BnOH) as initiator. Therefore, hydrophilic/lipophilic ratio (HLR) of the P(CL-ran-ATC)s copolymers can be finely adjusted by the feed ratio of TBODC and CL. The antimicrobial activity against Staphylococcus aureus (S. aureus) and Escherichia coli (E. coli) of P(CL-ran-ATC)s were proportional to HLR, and P(CL-ran-ATC)s presented more vigorous bactericidal activity towards S. aureus. The minimum inhibitory concentration (MIC) values of P(CL-ran-ATC 50.9%) are 2000 μg mL-1 and 3000 μg mL-1 for S. aureus and E. coli. While P(CL-ran-ATC 50.9%) exhibited deficient hemolytic activity as 1.41%. In addition, the P(CL-ran-ATC)s showed extremely low cytotoxicity towards fibroblast L929 cells.

1. Introduction

Antimicrobial n class="Chemical">peptides (n class="Chemical">AMPs) are promising antimicrobial agents originating from nature [1,2]. Despite its diverse origins, the basic structure of AMPs is an amphiphilic polypeptide containing cationic amino acid residues [3,4]. Unlike antibiotics that hindered pathogens’ metabolic pathways of [5], AMPs generally kill bacteria by membrane rupture mechanism [6,7]. Hence, it is difficult for the bacteria to develop resistance towards the AMPs. However, toxicity and low yield of the natural AMPs obstruct their application [8]. Additionally, AMPs quickly degraded in physiological environments, resulting in the loss of antibacterial effects [9].

Inspired by tn class="Chemical">he structure of n class="Chemical">AMPs, amphiphilic polymers bearing cationic segments which are stable to hydrolysis have been widely studied [10,11,12]. The synthetic polymers mimicking AMPs structure showed comparable antimicrobial efficiency towards pathogens. It has been extensively confirmed that the polymers’ hydrophilic/lipophilic ratio (HLR) significantly affected their toxicity and antibacterial ability [13,14,15,16]. Sophisticated control of HLR generally relied on the side chain’s design and the polymer’s main chain. Lipophilic side chain was commonly applied to alter HLR in the AMPs mimicking polymer [3,17]. Many studies have confirmed moderate length of the lipophilic alkyl side chain (5–7 C) was conducive to balance antimicrobial ability and toxicity [18]. Compared to HLR controlled by side chains, HLR controlled by the main chain lacks systematic study [19,20].

Tn class="Chemical">he positively charged cations in the AMPs mimics tended to interact with negatively charged bacteria and promoted the lipophilic section of tn class="Chemical">he AMPs mimics penetrating the cell wall causing the death of the bacteria [21]. Amines are widely applied in the AMPs mimics as they present a positive charge under the infection environment [15,22,23]. Compared to quaternary ammonium, which has been generally used in the AMPs mimicking polymers, primary amine showed better antimicrobial property [24,25] while more tendency to cause hemolysis [26].

Introducing biocompatible segments into AMPs mimicking polymers helped relieve toxicity [22,27,28,29,30,31]. Polycaprolactone (PCL) is a biocompatible material [32,33], and its lipophilic character can be used for adjusting HLR of the AMPs mimics [34]. In this research, primary amine bearing cyclic carbonate monomer TBODC was copolymerized with CL via ring opening polymerization (ROP) to get a series of AMP mimicking random copolymers. The protonated P(TBODC-ran-ATC)s were obtained via the deprotection process. HLR of P(TBODC-ran-ATC)s was adjusted by the initial feed ratio of TBODC to CL. The primary amine carrying precursor polymers and the protonated copolymers were characterized by nuclear magnetic resonance (NMR), gel permeation chromatography (GPC), differential scanning calorimetry (DSC) and thermogravimetric analyses (TGA). Antimicrobial activity of the protonated copolymers was evaluated against Gram-positive S. aureus and Gram-negative E. coli. Hemolytic activity and cytotoxicity were tested individually. The primary amine functionalized poly(ester-carbonate) with antimicrobial property has various potential applications, including wound dressings and antibiotics carriers.

2. Materials and Methods

2.1. Materials

n class="Chemical">Serinol, n class="Chemical">di-tert-butyl dicarbonate (n class="Chemical">Boc2O) were purchased from Meryer Chemical Technology (Shanghai, China). Trifluoroacetic acid (TFA) was purchased from Macklin Biochemical Co. Ltd (Shanghai, China). Ethyl chloroformate (>99.5%) was purchased from Xiya Reagent (Chengdu, China). Stannous octoate (Sn(Oct)2, 96%) was obtained from Alfa Aesar (Tianjin, China). Reagents mentioned above were used as received. Caprolactone (ε-CL) was purchased from Aladdin Biochemical Co. Ltd (Shanghai, China). and distilled over CaH2 before use. Triethylamine (Et3N) was successively treated by p-tosyl chloride and CaH2 to remove trace amounts of primary amine and H2O and stored with 4 Å molecular sieves. Dichloromethane (DCM), tetrahydrofuran (THF), toluene, and benzyl alcohol (BnOH) were dried over CaH2 and stored with 4 Å molecular sieves, respectively. All the reagents used in the research were of pure analytical grade.

2.2. Measurements

1H (400 MHz) and 13C NMR (100 MHz) spectra were obtained in deuterated chloroform (CDCl3, 99.5 atom % D with 0.03% v/v TMS), DMSO-d6 (D, 99.9% with 0.03% v/v TMS) using a AVANCE III HD 600 spectrometer (Bruker, Berlin, Germany).

Gel permeation chromatography (GPC) measurements were performed on a Waters 1525 binary high-pressure liquid chromatography (HPLC) pump equipped with 3 Ultra Styragel columns and a Waters 2414 refractive index detector (Waters Alliance GPC2000, Waters Corporation, Milford, MA, USA). To characterize the copolymers, THF was used as an eluent at a flow rate of 1 mL/min at 40 °C. The number-averaged molecular weight (Mn) and molar mass distribution (Ð) were calculated using Waters GPC Software, and narrowly dispersed polystyrenes (PS) were employed as calibration standards.

Tn class="Chemical">he n class="Chemical">copolymers’ tn class="Chemical">hermal properties were determined on a TA Instruments Q10 Differential Scanning Calorimeter (DSC, TA Instruments, New Castle, DE, USA). The enthalpy (cell constant) and temperature were calibrated by running high-purity indium and gallium standards under conditions identical to those used to measure the samples.

Zeta potential values were measured on Malvern Zetasizer Pro with He-Ne lamp at 633 nm (Malvern Instruments, Malvern, UK).

High-resolution mass spectrometry (HRMS) was determined on Waters G2-XS Qtof (Waters Corporation, Milford, MA, USA).

Tn class="Chemical">hermogravimetric analyses (TGA) were carried out using an STA 449 F3 Jupiter® simultaneous thermogravimetry-differential scanning calorimetry analyzer (NETZSCH-Gerätebau GmbH, Selb/Upper Franconia, Germany).

Organic elemental analyses (OEA) were conducted using a Vario EL cube analyzer (Elementar Analysensysteme GmbH, Frankfurt am Main, Germay).

2.3. Experimental Methodology

2.3.1. Synthesis of Cyclic Carbonates Bearing Potential Primary Amino Groups

n class="Chemical">TBODC was synthesized according to the previous report with some modifications [35]. Firstly, n class="Chemical">serinol (10.0 g, 11 mmol) was dissolved in 150 mL anhydrous ethanol, and Boc2O (30.3 mL, 13 mmol) was added dropwise. The mixture was stirred overnight at room temperature. Then ethanol was removed by rotary evaporation, and the residual was crystallized by a mixture of ethyl acetate/petroleum ether (v/v = 1/1). The white crystal was filtered to obtain intermediate tert-butyl (1,3-dihydroxypropan-2-yl)carbamate (Boc-serinol, 17.63 g). Yield: 83.5%. mp 90.8–92.7 °C. 1H NMR (400 MHz DMSO-d6, δ): 6.32 (s, 1H, -NHCOO-), 4.53–4.45 (t, 2H, -CH2OH), 3.43–3.33 (dm, 5H, -CH2CH- and -CH2CH-), 1.37 (s, 9H, -CH3).

n class="Chemical">Boc-serinol (15 g, 78 mmol) and ethyl chloroformate (14.9 mL, 156 mmol) were completely dissolved in 200 mL anhydrous THF. Tn class="Chemical">he mixture was cooled to 0 °C. Then, Et3N (27.1 mL, 195 mmol) was added dropwise, and white precipitation formed. The reaction was to lift to room temperature for another hour after the complete addition of Et3N. After filtration of the white precipitate, the filtrate was condensed by rotary evaporation, and then petroleum ether was added to obtain TBODC as white flakes (TBODC, 6.94 g). Yield: 58.5%. mp. 139.0–140.8 °C. HRMS: m/z calcd for C9H16NO5 208.1028, found 208.1019. 1H NMR (400 MHz, DMSO-d6, δ): 7.60 (s, 1H, -CONH-), 4.52 (dd, J = 3.5, 7.0 Hz, 2H, -OCH2-), 4.24 (dd, J = 3.5, 7.0 Hz, 2H, -OCH2-), 3.92 (s, 1H, -CH2CH-), 1.40 (s, 9H, -CH3). 13C NMR (100 MHz, DMSO-d6, δ): 155.38, 153.58, 78.55, 66.95, 41.80, 28.11. Anal. Calcd for C9H16NO5: C, 49.53; H, 7.39; N, 6.42; O, 36.66. Found: C, 49.27; H, 7.52; N, 6.63; O, 36.58.

2.3.2. Typical Synthesis of Random Copolymer Poly(ε-caprolactone-ran-tert-butyl (2-oxo-1,3-dioxan-5-yl)carbamate) (P(CL-ran-TBODC))

Syntn class="Chemical">hesis of n class="Chemical">P(CL-ran-TBODC) was conducted with the standard Schlenk technique under an atmosphere of nitrogen unless stated otherwise. For instance, 0.2 g TBODC (0.92 mmol), 920 μL CL (8.28 mmol), 9.6 μL BnOH (0.092 mmol), 14.9 μL SnOct2 (0.046 mmol) were added into a Schlenk flask. Then, 5 mL dry toluene was added into the flask, and the freezing–thawing cycle was conducted three times to remove oxygen and moisture. After the flask was charged with N2, polymerization was conducted at 100 °C. After polymerization for 24 h, 1H NMR monitored that conversion of both TBODC and CL exceeded 90%. Then the polymerization was stopped by cooling to room temperature, and the crude product was immediately precipitated by cold ethanol. Then, the crude polymer was dissolved and precipitated twice by THF and petroleum ether. The polymer was collected by filtration and dried in a vacuum oven for two days until constant weight. The polymer yield was over 90%.

2.3.3. Preparation of Poly(ester-carbonate)s Bearing Primary Amine

Deprotection of n class="Chemical">P(CL-ran-TBODC) was conducted as follows: 0.5 g n class="Chemical">P(CL-ran-TBODC) was completely dissolved in n class="Chemical">DCM. Then trifluoroacetic acid (TFA) was added dropwise at 0 °C. The deprotection was conducted for one hour to remove Boc groups. Then, deprotected polymer P(caprolactone-ran-amino trimethyl carbonate)s (P(CL-ran-ATC)s) were precipitated by diethyl ether. The product was dissolved-precipitated twice and dried in a vacuum oven till constant weight.

2.3.4. Antimicrobial Activity

Bacterial growth inhibition was evaluated by minimum inhibitory concentration (MIC) assay via the broth microdilution method. The MIC values of P(CL-ran-ATC)s were determined against S. aureus (ATCC No. 6538, Gram-positive) and E. coli (ATCC No. 8739, Gram-negative). Bacterial colonies were inoculated in Luria broth (LB) and left to grow overnight at 37 °C until the exponential phase while being shaken continuously. The overnight cultures of bacteria were adjusted to an optical density of 0.1 at 600 nm (OD600), equal to 108 CFU/mL. After washing in phosphate-buffered saline (PBS; NaH2PO4, K2HPO4, NaCl), the bacteria were diluted by Mueller–Hinton broth (MHB) to obtain a stock solution of 106 CFU/mL. The P(CL-ran-ATC)s were then diluted using the PBS buffer solution to bring the copolymers to the desired concentration range. After that, 40 μL of bacterial stock solution was added to each dilution and incubated at 37 °C for 24 h. The OD600 was then measured using a 96 well microplate reader. The minimum inhibitory concentrations (MIC) were later reported as the concentration at which no bacterial growth was observed.

2.3.5. Hemolysis

n class="Disease">Hemolysis caused by n class="Chemical">P(CL-ran-ATC)s was determined by n class="Chemical">hemoglobin release assay using the same P(CL-ran-ATC)s stock solutions used in the MIC test. Then, 1 mL of 4% (v/v) rabbit red blood cells (RBCs) was centrifuged at 1000 rpm for 5 min and after that washed with PBS solution of pH 7.4. The supernatants were then removed by pipetting. The RBCs were further washed with PBS twice. The RBCs were then diluted using PBS to provide 1% (v/v) RBCs assay stock. In a 96-well microplate, 90 μL of 1% (v/v) RBCs assay stock was mixed with 10 μL of the copolymer dilution. PBS with 5% (v/v) of DMSO was used as a negative control, while PBS with 0.1% (v/v) of Triton X-100 was used as a positive control. The microplate was sealed using a parafilm and incubated in an orbital shaker at a temperature of 37 °C at 180 rpm for 60 min. The microplate was then centrifuged at 1000 rpm for 10 min. In another microplate, 10 μL of supernatant was diluted in 90 μL of PBS. The absorbance at 415 nm was recorded using a microplate reader. Hemolysis fraction was then calculated using Equation (1). where OD415 is the absorbance of the test well, OD415 is the absorbance of negative control well, and OD415 is the absorbance of positive control well.

Tn class="Chemical">hepan> assay was performed in triplicates, with three replicates for each indepenpan>denpan>t experimenpan>t.

2.3.6. Cyto-Compatibility

Tn class="Chemical">he n class="Disease">cytotoxicity was cn class="Chemical">hecked on the first, second, and fourth days of culture using a cell counting kit-8 (CCK-8) assay. Fibroblast L929 suspension of 100 μL was seeded at a density of 1 × 103 cells/well and was pre-incubated at 37 °C for 4 h in a 5% CO2 incubator. The P(CL-ran-ATC)s copolymers were sterilized through filtration and diluted by PBS. Then, 10 μL of each diluted P(CL-ran-ATC)s copolymer was transferred to the cell seeding 96-well plate. The culture medium was changed every other day. Then, 10 μL of a CCK-8 solution was added to each well and incubated for 2 h according to the manufacturer’s instructions. After 2 h of incubation, the absorbance was measured at a wavelength of 450 nm using a microplate reader (Multiskan GO, Thermo Scientific, Waltham, MA, USA). The cell viability was calculated using Equation (2): where A is the absorbance of the test well, A is the absorbance of negative control well, and A is the absorbance of blank control well.

Tn class="Chemical">hepan> assay was performed in triplicates, with three replicates for each indepenpan>denpan>t experimenpan>t.

3. Results and Discussion

3.1. Synthesis of Cyclic Carbonate TBODC

n class="Chemical">TBODC, a n class="Chemical">cyclic carbonate monomer bearing potential primary n class="Chemical">amine groups, was synthesized by a two-step reaction starting from serinol (Scheme 1). Primary amine in serinol was protected by di-tert-butyl dicarbonate with high yield. The protection prevented interference with the ring closure reaction. The Boc-serinol intermediate was cyclocarbonated by ethyl chloroformate in the presence of triethylamine at 0 °C in THF. Finally, the cyclic carbonate TBODC was obtained with an overall yield of 50%. The structures of TBODC were characterized by 1H NMR and 13C NMR (Figures S1 and S2). Both appearance of the Boc signal and the signal shift of methylene indicated a successful synthesis of TBODC. In addition, the HRMS spectra and elemental analysis results confirmed the successful preparation of TBODC monomer.

Scheme 1

Synthesis of Boc-serinol and carbonate tert-butyl-(2-oxo-1,3-dioxan-5-yl) carbamate (TBODC).

3.2. Random Copolymerization of CL and TBODC

Tn class="Chemical">he semi-crystalline structure decreased the solubility of PCL [36,37,38]. n class="Chemical">Here, random copolymerization of TBODC and ε-CL was conducted to improve the copolymer’s solubility by disrupting the semi-crystalline region. The copolymerization was done in toluene using benzyl alcohol as initiator and SnOct2 as catalyst (Scheme 2).

Scheme 2

Synthesis of random copolymer P(CL-ran-TBODC) and deprotection.

Tn class="Chemical">he comonomer to initiator ratio was set at 100/1, and TBODC in monomer feed varied from 10%, 25%, to 50% (Table 1, entries 1–3). After 24 h, the polymerizations were stopped, and the conversion of both n class="Chemical">TBODC and ε-CL exceeded 90% (Figure S3). The initiator’s methylene hydrogen signal was selected to calculate the number average molecular weight (Mn) of the copolymers. P(CL-ran-TBODC X%) was short for the copolymers of TBODC and ε-CL, where X% stood for the percentage of TBODC segment in the copolymer. As shown in Table 1, TBODC ratio in the copolymers almost coincided with the monomer feed ratio, which suggested fine control of SnOct2 over the copolymerization. In addition, the protection of primary amine omitted possible interference on the ROP reaction. A typical 1H NMR spectrum of P(CL-ran-TBODC 22.8%) (Table 1, entry 2) is shown in Figure 1A. Signal of -OCH2- shifted from 4.55 ppm to 4.16 ppm indicated ring opening of TBODC. Furthermore, the presence of signals corresponding to PCL suggested that successful copolymerization of TBODC and CL. 13C NMR spectra also confirmed the synthesis of P(CL-ran-TBODC). As displayed in Figure 1B, peaks corresponding to P(CL-ran-TBODC 22.8%) were assigned. Signals of the carbonyl carbon of ester (j, 178.50–175.50 ppm) and carbonate (k, 138.30–136.40 ppm) split into two peaks as shown in the insert figure in Figure 1B. The signals were labeled as TT, TC, CT, and CC corresponding to TBODC-TBODC, TBODC-CL, CL-TBODC, and CL-CL dyads. The appearance of four dyads confirmed the preparation of random copolymers [39]. GPC curves indicated successful random copolymerizations were accomplished as uni-peaks showed up (Figure 2A). Meanwhile, low molar mass dispersities (Đ = 1.26 to 1.58) of the copolymer also revealed fine control of the copolymerization. DSC result confirmed that including TBODC segments can alter crystallinity of the copolymer. As shown in Figure 2B, the melting peak disappeared with an increase of TBODC ratio in the copolymer. In addition, the copolymer’s glass transition temperature (Tg) increased with a rise in TBODC ratio in the copolymer. It could ascribe to the bulky Boc groups hindered the chain segment’s movement, which caused a higher Tg.

Table 1

Ring opening polymerization of TBODC and ε- caprolactone (CL) catalyzed by SnOct2 a.

Entry	f TBODC/ε-CL b	1H NMR		GPC e		DSC
		F c	Mn/kDa d	Mn/kDa	Đ	Tg/°C	Tm/°C
1	10/90	7.1	8.3	8.7	1.26	−47.15	49.54
2	25/75	22.8	10.7	14.9	1.58	−40.73	36.53
3	50/50	50.9	3.9	17.7	1.30	−34.59	N/A
4	100/0	N/A	4.8	3.3	1.10	48.45	N/A
5	0/100	N/A	12.2	8.3	1.40	/f	63.50

a Polymerization conditions: [comonomer]/[BnOH]/[SnOct2] = 100/1/0.5, 100 °C, 24 h, 1 M in toluene; b feed ratio of TBODC to ε-CL in comonomer; c TBODC segment ratio in copolymers which is determined by 1H NMR via 0.5 × I4.14ppm/(0.5 × I4.14ppm + 0.5 × I2.31ppm); d molecular weight calculated by 1H NMR via 0.5 × I4.14 ppm × 217.22 + 0.5 × I2.31 ppm × 114.14 + 107.41; e THF used as elution; f Tg of PCL was not detected due to cooling depth limitation.

Figure 1

(A) 1H NMR spectrum of P(CL-ran-TBODC 22.8%) (400 MHz, CDCl3, 25 °C); (B) 13C NMR spectrum of P(CL-ran-TBODC 22.8%). Signals labeled TT, TC, CT, CC correspond to TBODC-TBODC, TBODC-CL, CL-TBODC, and CL-CL dyads (100 MHz, CDCl3, 25 °C).

Figure 2

(A) Gel permeation chromatography (GPC) curves of P(CL-ran-TBODC), (B) second heating scan of DSC traces of P(CL-ran-TBODC).

3.3. Deprotection of P(CL-ran-TBODC)

n class="Chemical">Boc groun class="Chemical">ps were removed by n class="Chemical">TFA to endow hydrophilicity and positive charge to the copolymers. 1H NMR was used to carefully monitor the deprotection progress to prevent excessive degradation of the copolymer. It was confirmed deprotection for 1 h was enough to remove Boc (Figure S4). The deprotected copolymer was obtained by adding diethyl ether, and the signal of Boc groups in carbonate segments almost disappeared. FT-IR results also confirmed the total removal of the Boc groups (Figure 3C). Peaks corresponding to Boc groups (1767 cm−1, 1265 cm−1, 1167 cm−1) disappeared after deprotection. The peak of primary amine showed up at 3438 cm−1. The deprotected copolymers were named after P(CL-ran-ATC x%), where ATC stood for carbonate segments after deprotection and x meant for carbonate ratio in the deprotected copolymers. Meanwhile, x was also exhibited as HLR in this study. Take deprotection of P(CL-ran-TBODC 7.1%) as an example, the methyl signal at 1.37 ppm disappeared and the signal at 3.65 ppm corresponding to freed amine shown up (Figure 3A). The NMR signal change indicated successful deprotection of Boc groups. Both NMR integration and uni-peak of GPC trace (Figure 3B) suggested no severe degradation occurred during deprotection. Compared to its precursor polymer P(CL-ran-TBODC 7.1%), an exothermic peak showed up at −29.01 °C in the second heating round of P(CL-ran-ATC 7.1%) (Figure 3C). As the bulky Boc groups were removed, the deprotected copolymer’s main chain was susceptible to undergoing a cold crystallization process. Hence, the melting point of P(CL-ran-ATC 7.1%) also decreased. TGA analysis confirmed that P(CL-ran-ATC 7.1%) tended to undergo pyrolytic degradation compared to its precursor P(CL-ran-TBODC 7.1%) (Figure 3D). It was due to the bare primary amine was not stable and can cause degradation of the copolymer.

Figure 3

(A) 1H NMR spectra of P(CL-ran-ATC 7.1%) and P(CL-ran-TBODC 7.1%) (DMSO-d6, 400 MHz); (B) GPC curves of P(CL-ran-ATC 7.1%) and P(CL-ran-TBODC 7.1%); (C) FT-IR spectra of P(CL-ran-ATC 7.1%) and P(CL-ran-TBODC 7.1%); (D) DSC traces of P(CL-ran-ATC 7.1%) and P(CL-ran-TBODC 7.1%); (E) TGA traces of P(CL-ran-ATC 7.1%) and P(CL-ran-TBODC 7.1%).

With tn class="Chemical">he increase of carbonate content in the n class="Chemical">copolymer, P(CL-ran-ATC)’s solubility in DI water increased after the deprotection process. Notably, P(CL-ran-ATC 50.9%) formed a homogeneous aqueous solution. P(CL-ran-ATC 50.9%) solution showed 38.3 ± 1.2 mV Zeta potential, while Zeta potential P(CL-ran-ATC 22.8%) was 25.8 ± 1.8 mV. Zeta potential determination of P(CL-ran-ATC 7.1%) was failed as poor solubility of P(CL-ran-ATC 7.1%) in DI water. Surprisingly, PATC showed a Zeta potential of 7.7 ± 0.7 mV, which was lower than P(CL-ran-ATC 50.9%) and P(CL-ran-ATC 22.8%). Different main chain structure of P(CL-ran-ATC) and homo-PATC might be responsible for the Zeta potential determination.

Tn class="Chemical">he deprotected primary n class="Chemical">amine in n class="Chemical">P(CL-ran-ATC)s tended to form -NH3+ammonium ions under physiological condition, which is responsible for amphiphilicity and positive Zeta potential of P(CL-ran-ATC)s. Principally, P(CL-ran-ATC)s were structural analogs of antimicrobial peptides (AMPs). In the following study, the relationship between the structure of P(CL-ran-ATC)s and their antimicrobial property was studied.

3.4. Antimicrobial Property, Hemolytic Activity, and Cytotoxicity

Tn class="Chemical">he antimicrobial property of P(CL-ran-ATC)s was studied by minimum inhibitory concentrations (MIC) test via the microdilution method. n class="Species">S. aureus (ATCC No. 6538) and E. coli (ATCC No. 8739) were applied as model Gram-positive and Gram-negative bacteria. P(CL-ran-ATC)s was dissolved into 5000 μg mL−1, and the concentration subsequently diluted until 1 μg mL−1. As demonstrated in Table 2, MICs of P(CL-ran-ATC)s generally decreased with the increase of HLR of the copolymers. The results showed that the increase in the content of hydrophilic carbonate segments in the random copolymer P(CL-ran-ATC)s is conducive to enhancing the antimicrobial property. P(CL-ran-ATC 7.1%) showed no antibacterial effect even at 5000 μg mL−1. It should ascribe to the low solubility of P(CL-ran-ATC 7.1%).

Table 2

Antimicrobial (MIC), hemolytic activities (HC4000), and Zeta potential of the polycationic copolymers.

Polymer	HLR a	MIC (μg mL−1)		Hemolytic Activity (H4000) b	Zeta Potential (mV)
		S. aureus (Gram +)	E. coli (Gram −)
P(CL-ran-ATC 7.1%)	7.1	NA c	NA c	2.16%	/d
P(CL-ran-ATC 22.8%)	22.8	3500	4000	1.53%	25.8 ± 1.8
P(CL-ran-ATC 50.9%)	50.9	2000	3000	1.41%	38.3 ± 1.2
PATC	/	4000	NA c	0.74%	7.7 ± 0.7

a Hydrophilic/lipophilic ratio (HLR) is protonated carbonate segment ratio in P(CL-ran-ATC). b H4000 is the hemolysis percentage at a concentration of 4000 μg mL−1. c NA indicates that no antibacterial effect was observed even at 5000 μg mL−1. d Undetectable.

As confirmed by MIC, tn class="Chemical">he n class="Chemical">P(CL-ran-ATC) copolymers showed a relatively more substantial antimicrobial effect towards Gram-positive S. aureus. The results are consistent with previously reported that amino-bearing polyesters have a better bactericidal effect on Gram-positive bacteria [30,31]. SEM images also confirmed the results of MIC (Figure 4). S. aureus significantly shrank after treatment with P(CL-ran-ATC 50.9%)s and rupture can be observed. E. coli showed a similar trend, but slight shrinkage was observed (arrow in Figure 4C). As confirmed by SEM, the morphological change of bacterial membrane accorded with the membrane rupture mechanism after treatment with AMPs.

Figure 4

SEM images of S. aureus incubated (A) in the presence of P(CL-ran-ATC 50.9%) (3000 μg mL−1), (B) in the absence of polymer; E. coli incubated (C) in the presence of P(CL-ran-ATC 50.9%) (3000 μg mL−1), (D) in the absence of polymer. The scale bar was 5 μm.

Surprisingly, homon class="Chemical">polymer PAn class="Chemical">TC presented a weaker antibacterial effect than P(CL-ran-ATC 22.8%) and P(CL-ran-ATC 50.9%). It reminded the lipophilic segment is necessary for promoting antimicrobial effect for poly(ester-carbonate)s. In addition, MICs of P(CL-ran-ATC)s were high when they were compared with other antimicrobial poly(ester-carbonate)s [40,41]. Cationic centers distributed on the main chain and the random structure of P(CL-ran-ATC)s may hinder interaction between the copolymer and the bacteria, which led to a high MIC value of P(CL-ran-ATC)s.

Previous literature reported that n class="Chemical">polymers containing primary amine groups are prone to hemolysis [27]. Here, rabbit red blood cells (rRBCs) were used to evaluate tn class="Chemical">he hemolytic activity of P(CL-ran-ATC)s (Table 2). The rRBCs remained a complete structure even when the concentration of P(CL-ran-ATC)s reached 4000 μg mL−1. The hemolysis rate was lower than 2.5% during the whole test. Moreover, hemolysis slightly increased with a decrease of HLR of P(CL-ran-ATC)s. The results indicated that the increase of hydrophobic PCL segments caused a decrease of HLR and slightly promoted hemolysis.

To furtn class="Chemical">hepan>r characterize tn class="Chemical">he n class="Disease">cytotoxicity of P(CL-ran-ATC)s, fibroblast L929 was co-cultivated with P(CL-ran-ATC)s. After culture for three days, Cell Counting Kit-8 (CCK-8) was used. As shown in Figure 5, cells proliferated well in all groups, indicating that the cytotoxicity of P(CL-ran-ATC)s can be ignored.

Figure 5

Cytotoxicity of P(CL-ran-ATC)s against fibroblast L929 cells.

4. Conclusions

In conclusion, primary bearing cyclic carbonate TBODC was copolymerized with CL to form random copolymers via ring opening polymerization. The random copolymers turned amphiphilic after the removal of Boc protecting groups. Hydrophilic/lipophilic ratio (HLR) of the protonated poly(ester-carbonate)s can be adjusted by the feed ratio of TBODC and CL. P(CL-ran-ATC 50.9%) exhibited higher antimicrobial activity than P(CL-ran-ATC 7.1%) and P(CL-ran-ATC 22.8%) due to higher HLR. All the P(CL-ran-ATC)s exhibited low hemolytic activity, and the hemolysis rate slightly increased with a decrease of HLR. P(CL-ran-ATC)s were proved to be free of cytotoxicity. Further study on block copolymer of TBODC and CL is under investigation. We anticipate that by altering polymer’s structure, the antibacterial ability of P(CL-co-ATC)s can be improved.