Stability and in vivo evaluation of pullulan acetate as a drug nanocarrier
Introduction Nanoparticles (NPs) have specic physicochemical properties diering from bulk materials of the same composition, and such properties make them very attrac- tive for commercial and medical development (Curtis et al., 2006; Lanone & Boczkowski, 2006; Medina et al., 2007). However, compared with conventional materials, NPs may have dierential toxicity proles due to their dierent chemical and structural properties (Vega-Villa et al., 2008). For example, the interaction between nano- materials and biological components, e.g. proteins and cells may lead to their unique bio-distribution, clearance, immune response, and metabolism, and therefore it is very necessary to study the in vivo toxicity of nanomateri- als (Fischer & Chan, 2007). Pullulan, a very important neutral and linear natural polysaccharide, has been used as a good biomaterial in drug and gene delivery, tissue engineering, and other elds (Leathers, 2003; Shingel, 2004; Rekha & Sharma, 2007). Many investigations (Akiyoshi et al., 1993; Jeong et al., 2006) have reported that some hydrophobized pullulan such as cholesterol-modied pullulan can form self-aggregated NPs to be used as the carrier for drug delivery. As one of the most conventional hydro- phobized pullulan derivatives (Jung et al., 2003; Na et al., 2003; 2004, Park et al., 2007), pullulan acetate (PA) and its modied materials can form self-aggregated NPs in Drug Delivery, 2010; 17(7): 552–558 Address for Correspondence: Qi-Qing Zhang, Institute of Biomedical Engineering, Chinese Academy of Medical Sciences, Peking Union Medical College, e Key Laboratory of Biomedical Material of Tianjin, Tianjin 300192, PR China. Tel/Fax: +86 22 87890868. E-mail: zhangqiq@126.com RESEARCH ARTICLE Stability and in vivo evaluation of pullulan acetate as a drug nanocarrier Hong-Bo Tang 1 , Lei Li 1 , Han Chen 1 , Zhi-Min Zhou 1 , Hong-Li Chen 1 , Xue-Min Li 1 , Ling-Rong Liu 1 , Yin-Song Wang 3 , and Qi-Qing Zhang 1,2 1 Institute of Biomedical Engineering, Chinese Academy of Medical Sciences, Peking Union Medical College, e Key Laboratory of Biomedical Material of Tianjin, Tianjin 300192, PR China, 2 Research Center of Biomedical Engineering, Department of Biomaterials, College of Materials, Xiamen University, Technology Research Center of Biomedical Engineering of Xiamen City, e Key Laboratory of Biomedical Engineering of Fujian Province, Xiamen 361005, PR China, and 3 College of Pharmacy, TianJin Medical University, Tianjin, 300070, PR China Abstract To develop pullulan acetate nanoparticles (PANs) as a drug nanocarrier, pullulan acetate (PA) was synthesized and characterized. Its acetylation degree determined by the proton nuclear magnetic resonance ( 1 H NMR) was 2.6. PANs were prepared by the solvent diffusion method and characterized by transmission electron microscope (TEM), size distribution, and ζ potential techniques. PANs had nearly spherical shape with a size range of 200–450 nm and low ζ potentials both in distilled water and in 10% FBS. The storage stability of PANs was observed in distilled water. PANs were stored for at least 2 months with no significant size and ζ potential changes. The safety of PANs was studied through single dose toxicity test in mice, and the result showed that PANs were well tolerated at the dose of 200 mg/kg in mice. Epirubicin-loaded PANs (PA/EPI) were also prepared and characterized in this study. Moreover, the in vivo pharmacokinetics of PA/EPI was investigated. Compared with the free EPI group, the PA/EPI group exhibited higher plasma drug concentration, longer half-life time (t 1/2 ) and the larger area under the curve (AUC). All results suggested that PANs were stable, safe, and showed a promising potential on improving the bioavailability of the loaded drug of the encapsulated drug. Keywords: Pullulan acetate; nanoparticles; pharmacokinetics; toxicity; epirubicin (Received 26 December 2009; revised 20 April 2010; accepted 28 April 2010) ISSN 1071-7544 print/ISSN 1521-0464 online © 2010 Informa Healthcare USA, Inc. DOI: 10.3109/10717544.2010.490250 http://www.informahealthcare.com/drd Drug Delivery 2010 17 7 552 558 26 December 2009 20 April 2010 28 April 2010 1071-7544 1521-0464 © 2010 Informa Healthcare USA, Inc. 10.3109/10717544.2010.490250 DRD 490250 Drug Delivery Downloaded from informahealthcare.com by University of Technology Sydney on 03/01/11 For personal use only. Stability and in vivo evaluation of pullulan acetate 553 aqueous media. e hydrophobic core of these self- assembled NPs formed by the hydrophobic interactions was considered to act as a reservoir of hydrophobic substances. In our previous report (Zhang et al., 2009), PANs prepared by the solvent diusion method had the potential to be used as a sustained release carrier for Epirubicin (EPI) in vitro. Some investigations (Gu et al., 1998; Na et al., 2004; Shimizu et al., 2008) showed that NPs of hydrophobized pullulans had good morphol- ogy, drug loading, and release properties in vitro, but the biological eects of hydrophobized pullulan NPs in vivo have not been investigated deeply up to date. Herein, based on our previous work, we studied the stability and toxicity of PANs, and further investigated the sustained release behavior in vivo of drug loading in PANs. PA was rstly synthesized and characterized by FT-IR and 1 H NMR, and then PANs with moderate size and low potential were prepared by the solvent diusion method. e storage stability of PANs was studied in the aqueous medium, and the acute toxicity of PANs was evaluated in mice. Morever, EPI was loaded into PANs and its pharmacokinetics was also assessed in rats to compare to the free drug. Methods Materials Pullulan (Mw = 200,000) was purchased from Hayashibara (Tokyo, Japan). Epirubicin·HCl (EPI·HCl) was purchased from Hisun Pharmaceutical Co. (Zhejiang, China). Poly (vinyl alcohol) (PVA) with an average molecular weight of 30,000–70,000 was obtained from Sigma-Aldrich (St. Louis, MO). All reagents for high performance liquid chromatography (HPLC) analysis, including acetonitrile and methanol, were HPLC grade. Other chemical reagents were of analytical grade and obtained from commercial sources. ICR mice and Wistar rats were purchased from the Institute of Radiology, Chinese Academy of Medical Science. All animal experiments were performed in compliance with the Institutional Animal Care and Use Committee (IACUC) guidelines. Synthesis and characterization of PA PA was synthesized according to the method described in previous literature (Jung et al., 2003; Zhang et al., 2009). Briey, pullulan (2 g) was suspended in 20 ml of formamide and dissolved by vigorous stirring at 54°C. Pyridine (6 ml) and acetic anhydride (5.5 ml) were added to the above solution, and the mixture was subsequently stirred at 54°C for 48 h. e reactant was precipitated with distilled water, and then washed with distilled water and methanol. e solid material was vacuum-dried at 50°C for 48 h. e nal product was identied by Fourier trans- form infrared (FT-IR) (ermo, Nicolet is10, Los Angeles, CA ) and 1 H NMR (Varian, Varian INOVA. 400 M NMR, Palo Alto, CA) spectrometry. e degree of substitution (DS) was dened as the number of acetyl groups per glucose unit of pullulan. It was determined by 1 H NMR (Zhang et al., 2009). e DS values are expressed by the following equations: DS = 10A/(3B + A), where A is the integration value of acetyl protons at 1.8–2.2 ppm and B is that of OH protons and H-1 to H-6 protons of pullulan moiety observed at more than 3.5 ppm. Preparation and characterization of PANs and PA/EPI Nanoparticles were prepared according to a solvent dif- fusion method (Fessi et al., 1989; Govender et al., 1999; Bilati et al., 2005; Zhang et al., 2009). Briey, PA (100 mg) was dissolved in 10 ml of N, N-Dimethylformamide (DMF). e solution was then added to 0.5% PVA aqueous solution through a syringe under moderate magnetic stirring. e produced PANs were collected with centrifugation (Beckman Coulter, Inc. Avanti J-25, Fullerton, CA) at 18,000 rpm for 15 min at 4°C. Subsequently, PANs were dispersed in the distilled water and 10% fetal bovine serum (FBS), respectively, with PA concentration of 1 mg/ml to carry out the later experiments. EPI-loaded PANs were prepared as follows: EPI·HCl (10 mg) was dissolved in DMF (2 ml) and then triethyl- amine (TEA) was added to this solution to remove hydrochloride. e mixed solution was stirred in the dark for 12 h. PA (100 mg) dissolved in 8 ml of DMF was added into this mixed solution. e PA/EPI were collected with centrifugation (Beckman Coulter, Inc. Avanti J-25, Fullerton, CA) at 18,000 rpm for 15 min at 4°C, then the supernatant removed and washed twice with distilled water, at last, dispersed in distilled water by sonication for several minutes with a probe-type sonier (Automatic Ultrasonic Processor UH-500A, China) at 100 W. e particle size and ζ potential were determined by dynamic light scattering (Malvern Instruments Ltd., Zeta sizer 2000, Worcestershire, UK). e morphology of NPs was observed using TEM (FEI, TECNAI G2F-20, Eindhoven, Holland). e stability of PANs in water In order to study the stability of PANs, the above disper- sions were stored for 2 months at 4°C. Macroscopic char- acteristics of NPs dispersions such as opalescence and precipitation were observed from time to time. Moreover, the size and ζ potential of PANs were also determined by dynamic light scattering method once a month, and all measurements were performed in triplicate. Drug Delivery Downloaded from informahealthcare.com by University of Technology Sydney on 03/01/11 For personal use only. 554 H.-B. Tang et al. In vivo toxicity e toxicity of PANs was evaluated in vivo according to the previous reported method (Yoksan & Chirachanchai, 2008; Sonaje et al., 2009). Adult male and female ICR mice (18–22 g) were randomly divided into two groups, each with 10 mice. e experimental group received a single intravenous (i.v.) dose of blank PANs (200 mg/kg); the other group was treated with a single i.v. dose of normal saline. All animals were fed with normal diet, and water was provided ad libitum. Animals were observed care- fully for the onset of any signs of toxicity and monitored for changes in food intake and body weight at 1, 8, and 15 days. After being sacriced at 15 days, internal organs of each animal were harvested and observed grossly. For histological examinations, specimens of major organs such as heart, liver, spleen, lung, and kidney were xed in 10% phosphate buered formalin, embedded in paraf- n, sectioned, and stained with hematoxylin and eosin (H&E). In vivo pharmacokinetics and bioavailability In vivo pharmacokinetic study was conducted by the routine method (Mross et al., 1988; Bibby et al., 2005; Cao & Feng, 2008; Devalapally et al., 2008). e drug content of the PA/EPI was determined according to our previous study (Zhang et al., 2009) and PA/EPI with 3.34% was selected to carry out the pharmacokinetics studies. Female Wistar rats of 180~250 g and 4~6 weeks old were held in an air-conditioned facility, provided with standard food and ltered water. Animals were ran- domly assigned to two groups, each with six rats, which received an i.v. injection via the tail vein of free EPI and the PA/EPI solution in saline at 10 mg/kg equivalent dose, respectively. All animals were observed for mortal- ity, general condition, and potential clinical signs. e blood samples were collected with heparinized tube at 0 (pre-dose), 0.0167, 0.0833, 0.167, 0.5, 1, 2, 4, 8, 12, 24, and 48 h post-treatment. Plasma samples were harvested by centrifugation at 3000 rpm for 15 min and stored at −20°C until analysis. Liquid–liquid extraction was performed prior to the HPLC analysis. Briey, the plasma (100 µl) was mixed with dichloromethane-meth- anol (4:1, v/v) on a vortex-mixer for 3 min to extract the drug. Upon centrifugation at 10,000 rpm (15,000 g) for 15 min, the upper aqueous layer was removed by aspi- ration and the organic layer was transferred to a tube and evaporated under nitrogen at 50°C. e residue was dissolved in 100 µl of anhydrous methanol by vortex. For the HPLC analysis, the C-18 column was used and the mobile phase (0.02 M KH 2 PO 4 /CH 3 CN/CH 3 OH = 49:17:34 v/v/v) was delivered at a rate of 1 ml/min. Sample (20 μl) was injected and the column euent was detected with a UV detector at 232 nm. e main pharmacokinetic parameters were calculated by DAS 1.0 (Anhui, China) program. Bioavailability (BA) is a measurement of the rate and extent of a therapeutically active drug that reaches the systemic circulation and is available at the site of action. When a medication is administered intravenously, its bioavailability is 100%. When the standard consists of intravenously administered drug, this is known as relative bioavailability (BA R ). e BA R of PA/EPI after administra- tion was calculated using the following formula (Sonaje et al., 2009): BA (AUC )Dose (AUC )Dose 100 R AB BA = × × ×% () () where AUC is the area under the curve. Statistical analysis All data are presented as a mean value with its stand- ard deviation indicated (mean ± SD). Statistical analysis was conducted using the Student’s t-test. Dierences were considered to be statistically signicant when the p-values were less than 0.05. Results and discussion Characterization of PA Pullulan has three free hydroxyl groups on each glucose unit. It is easy to synthesize hydrophobic pullulan deriva- tive, PA, by means of replacing the hydroxyl groups of the glucose unit with acetate groups. Figure 1 shows FT-IR spectra of pullulan and PA, which were similar to our previous literature (Zhang et al., 2009). Figure 2 shows 1 H NMR spectra of pullulan and PA in DMSO-d 6 . e acetylation degree of PA calculated by 1 H NMR method was 2.6, which is smaller than 2.7 reported by Zhang et al. (2009). Based on our previous report, PA with lower DS may form smaller NPs in size. Moreover, Li and Huang 3500 3000 2500 2000 1500 1000 500 Wavenumber (cm −1 ) a b Figure 1. FT-IR spectra of PA (a) and pullulan (b). Drug Delivery Downloaded from informahealthcare.com by University of Technology Sydney on 03/01/11 For personal use only. Stability and in vivo evaluation of pullulan acetate 555 (2008) also reported that the smaller size of NPs may be in favor of longer circulation time in vivo. erefore, PA with acetylation degree of 2.6 was used to prepare PANs and PA/EPI in our study. Characterization of PANs and PA/EPI e self-assembled NPs were prepared by solvent dif- fusion method. is method had several advantages such as a rapid and simple preparation procedure, great potential for large industrial scale production, and easy control of the particle size (Zhang et al., 2009). e size and the size distributions of PANs and PA/EPI in distilled water were measured by DLS. e morphological char- acteristics were observed by TEM at the same time. As shown in Table 1, the mean diameters of PANs and PA/ EPI were 247.6 ± 34.8 nm and 343.4 ± 87.7 nm, with the narrow size distributions (the polydispersity indexes (PDI) < 0.3, Figure 3). Under TEM observations (Figure 4), PANs and PA/EPI were nearly spherical in shape and uni- form sized. ζ potential of NPs in dierent media e ζ potentials of PANs and PA/EPI in distilled water were −3.353 ± 1.296 mV and −3.297 ± 1.025 mV. To model the circulation in vivo, we observed the ζ potentials of NPs in 10% FBS, which had a composition very similar to the body liquids. e ζ potentials of PANs and PA/EPI in 10% FBS were −1.460 ± 0.297 and −1.902 ± 1.112 mV. According to the previous report (Levchenko et al., 2002; Alexis et al., 2008), neutral NPs would exhibit a decreased rate of macrophage phagocytosis system (MPS) uptake. However, MPS is the major contributor for the clearance of NPs, thus the reducing rate of MPS uptake could be considered as the best strategy for prolonging the cir- culation of NPs (Li & Huang, 2008). erefore, PA/EPI prepared in this study would exhibit the longer blood circulation time than free EPI in vivo. e storage stability of PANs Stability is an important facet of preparation and a neces- sary step in the development process, it will indicate the potentiality of industry production. e possibilities of modulating the loaded drug’s pharmacokinetic param- eters are dependent on physicochemical properties such as stability, size, and surface characteristics (Lourenco et al., 1996). PANs dispersions maintained slight opal- escence within 2 months. As shown in Table 2, the size, size distribution, and ζ potential of PANs showed no sig- nicant changes during 2 months. erefore, it could be concluded that PANs in aqueous media were stable for at least 2 month at 4°C. Stabilization of colloidal systems is traditionally viewed as arising from either electrostatic or steric eects (Lourenco et al., 1996). A ζ potential of at least −30 mV for electrostatic stabilized systems is desired to obtain a physically stable suspension according to the literature (Müller & Jacobs., 2002). e higher zeta poten- tial value indicates the better stability (Dai et al., 2010). e absolute value of ζ potential was lower than 5 mV in our study. e result showed that electrostatic stabi- lization was not provided eciently in the suspension; 5.0 a b ppm (t1) 4.0 3.0 2.0 Figure 2. 1 H NMR spectra of pullulan (a) and PA (b) (DMSO-d6). 1000100 Size (d.nm) Size Distribution by intensity Intensity (%) 101 20 a 15 10 5 0 10000 Undersize 100 80 60 40 20 0 1000100 Size (d.nm) Size Distribution by intensity Intensity (%) 101 20 b 15 10 5 0 10000 Undersize 100 80 60 40 20 0 Figure 3. Diameter distributions of PANs (a) and PA/EPI (b). Table 1. Size and PDI of PANs and PA/EPI ( ± s, n = 6). NPs Diameter (nm) PDI PANs 247.6 ± 34.8 0.179 ± 0.057 PA/EPI 343.4 ± 87.7 0.195 ± 0.069 Drug Delivery Downloaded from informahealthcare.com by University of Technology Sydney on 03/01/11 For personal use only. 556 H.-B. Tang et al. therefore, a steric stabilization may occur and provide the stability of the PANs. It may also be important information for developing a new nanosuspension liquid formulation about pullulan acetate. In vivo toxicity To evaluate whether i.v. administration (at dose of 200 mg/kg) of PANs was associated with any toxicity in vivo, animals were treated with a single dose of empty NPs. No signicant dierences between the PANs group and the control group in clinical signs, e.g. diarrhea, fever, and other systemic symptoms, and no mortality occurred throughout the entire study course. Additionally, there were no signicant dierences in body weight and food intake for both male and female mice between the two studied groups (Tables 3 and 4). Figure 5 shows the microscopic examination of major organs including heart, liver, spleen, lung, and kidney sections stained with H&E. Pathological changes in the major organs including heart, liver, spleen, lung, kidney, stomach, and intestinal segments were scarcely observed at 15 days. Moreover, no evidence of inammatory reactions was observed in the experimental group. All the above results indicated that no apparent toxicity of the PANs was found in the experimental animals after i.v. at a dose of 200 mg/kg. In vivo pharmacokinetics e plasma levels of EPI were determined following a sin- gle i.v. injection of EPI or PA/EPI (10 mg/kg EPI equiv.) in female Wistar rats. e plasma levels over 48 h are shown in Figure 6 and the PK parameters are summarized in Table 5. e peak concentration of total EPI in plasma was 14.65 mg/L at 1 min after injection and then decreased to nearly undetectable levels after 24 h. e maximum con- centration (C max ) of PA/EPI at 5 min was 9.80 mg/L, which was obviously lower than that of EPI because of sustained release from NPs. According to the previous report (Mross et al., 1988; Jakobsen et al., 1991; 1994), free EPI rapidly Table 2. Diameter and ζ potential of PANs ( ± s, n = 3). Time Diameter (nm) PDI ζ potential (mV) Day 0 260.4 ± 8.03 0.180 ± 0.025 −3.353 ± 1.296 1 month 242.4 ± 27.15 0.162 ± 0.073 −2.058 ± 1.987 2 month 229.5 ± 17.78 0.136 ± 0.085 −1.580 ± 2.153 Table 3. Body weight of PANs i.v. injected in mice at 200 mg/kg dose ( ± s, g). Group Sex n Day 1 Day 8 Day 15 Control 5 18.46 ± 0.81 23.12 ± 1.51 24.90 ± 1.04 5 18.64 ± 1.17 25.68 ± 2.81 30.02 ± 2.25 PANs 5 18.14 ± 0.68 22.85 ± 1.12 24.96 ± 0.88 5 18.68 ± 0.51 26.30 ± 0.80 30.06 ± 1.48 Table 4. Food intake of PANs i.v. injected in mice at 200 mg/kg dose ( , g). Group Sex n Day 8 Day 15 Control 5 4.97 5.12 5 5.62 6.50 PANs 5 4.57 5.26 5 5.53 6.40 ab Liver Spleen Kidney Lung Heart Figure 5. Representative photomicrographs of the heart, liver, spleen, lung, and kidney sections (H&E staining) of mice of control group (a) and treated with test NPs (b). a 100 nm 0.2 µm b Figure 4. Transmission electron micrographs (TEM) of (a) PANs and (b) PA/EPI. Drug Delivery Downloaded from informahealthcare.com by University of Technology Sydney on 03/01/11 For personal use only. Stability and in vivo evaluation of pullulan acetate 557 disappeared from the circulation due to its short half-life. In this study, the terminal elimination half-life of free EPI was 8.129 h (Table 5), which was consistent with that of 7.3 h of doxorubucin (Gustafson et al., 2002; Bibby et al., 2005). In contrast, PA/EPI showed a much longer circula- tion time and its elimination half-life time was 17.231 h, 2.12-times that of free EPI. e clearance of EPI loaded in NPs was 0.104 L/h, which is 3.16-times smaller than free EPI. Moreover, the mean residence time (MRT) of PA/ EPI in the plasma was 15.854 h, 1.9-times that of free EPI. Altogether, PA/EPI had the longer t 1/2 and MRT, lower V d and CL than the free drug in rats. At the same time, the AUC of EPI and PA/EPI from 0–24 h were 48,128.269 and 91,006.508 µg h/L, respectively. e bioavailability of free EPI was 100%, the BA R of PA/EPI calculated through the equation above by the AUC 0–24h was 189%, much higher than the free drug. According to the previous report (Li & Huang, 2008), we believed that the longer t 1/2 of PA/EPI in plasma may be due to its low ζ potential and moder- ate size. As prolonged plasma circulation is the driving force for increased tumor targeting (Seymour et al., 1995), Tsuchihashi et al. (1999) prepared long circulating lipo- somes to improve therapeutic ecacy of doxorubicin. In this study, the slow release of EPI from PANs in the blood suggested that the bioavailability of EPI improved when it was loaded into PANs. However, whether it could enhance the uptake of passive permeability in targeting tumor tissues or not needs to be further proved by the experiments such as bio-distribution study and pharma- codynamic test. Conclusions In this study, PA with the DS of 2.6 was synthesized and characterized. PANs and PA/EPI with moderate size and low potential were prepared by the solvent diusion method. e nanoparticles were stable in aqueous media for at least 2 months in vitro, furthermore, PANs were safe in mice at 200 mg/kg and showed the potential to improve the bioavailability of the loaded drug in vivo. Declaration of interest is work was supported by the Major State Basic Research Program of China (No. 2006 CB933300). References Akiyoshi, K., Moriguchi, N., Yamaguchi, S., Sunamoto, J. (1993). Self-aggregates of hydrophobized polysaccharides in water. Formation and characteristics of nanoparticles. Macromolecules. 26:3062–8. Alexis, F., Pridgen, E., Molnar, L.K., Farokhzad, O.C. (2008). Factors aecting the clearance and biodistribution of polymeric nano- particles. Mol Pharm. 5:505–15. Bibby, D.C., Talmadge, J.E., Dalal, M.K., Kurz, S.G., Chytil, K.M., Barry, S.E., Shand, D.G., Steiert, M. (2005). Pharmacokinetics and biodistribution of RGD-targeted doxorubicin-loaded nanoparti- cles in tumor-bearing mice. Int J Pharm. 293:281–90. Bilati, U., Allemann, E., Doelker, E. (2005). Development of a nano- precipitation method intended for the entrapment of hydrophilic drugs into nanoparticles. Eur J Pharm Sci. 24:67–75. Cao, N., Feng, S.S. (2008). Doxorubicin conjugated to D-alpha- tocopheryl polyethylene glycol 1000 succinate (TPGS): conjuga- tion chemistry, characterization, in vitro and in vivo evaluation. Biomaterials. 29:3856–65. Curtis, J., Greenberg, M., Kester, J., Phillips, S., Krieger, G. (2006). Nanotechnology and nanotoxicology: a primer for clinicians. Toxicol Rev. 25:245–60. Dai, W., Zhang, D., Duan, C., Jia, L., Wang, Y., Feng, F., Zhang, Q. (2010). Preparation and characteristics of oridonin-loaded nanostructured lipid carriers as a controlled-release delivery system. J Microencapsul. 27:234–41. Devalapally, H., Rajan, K.S., Akkinepally, R.R., Devarakonda, R.K. (2008). Safety, pharmacokinetics and biodistribution stud- ies of a beta-galactoside prodrug of doxorubicin for improve- ment of tumor selective chemotherapy. Drug Dev Ind Pharm. 34:789–95. Fessi, H., Puisieux, F., Devissaguet, J.P., Ammoury, N., Benita, S. (1989). Nanocapsule formation by interfacial deposition follow- ing solvent displacement. Int J Pharm. 55:R1–R4. Fischer, H.C., Chan, W.C. (2007). Nanotoxicity: the growing need for in vivo study. Curr Opin Biotechnol. 18:565–71. Govender, T., Stolnik, S., Garnett, M.C., Illum, L., Davis, S.S. (1999). PLGA nanoparticles prepared by nanoprecipitation: drug load- Table 5. Pharmacokinetic parameters of EPI and PA/EPI i.v. injected in rats at the equivalent 10 mg/kg dose. Parameters EPI PA/EPI t 1/2 (h) 8.129 17.231 AUC 0–24 (µg h/L) 48,128.269 91,006.508 AUC 0–∞ (µg h/L) 50,720.404 100,500.955 MRT 0–24 (h) 8.356 15.854 MRT 0–∞ (h) 9.64 20.539 Vd (L/kg) 3.822 2.595 CL (L/h/kg) 0.33 0.104 t 1/2 : half-life time; AUC 0–24 : area-under-the-curve from time 0 to 24 h; AUC 0–∞ : area-under-the-curve from time 0 to innity; MRT 0–24 : mean residence time from time 0 to 24 h; MRT 0–∞ : mean residence time from time 0 to innity; Vd: volume of distribution; CL: total body clearance. Time (h) Con (µg/L) 10 15 20 25 30 35 EPI 10 PA/EPI 10 40 45 5050 0 00.5 11.5 2 2000 4000 6000 8000 10000 12000 14000 16000 0 2000 4000 6000 8000 10000 12000 14000 16000 Figure 6. Plasma drug concentration of EPI and PA/EPI after i.v. injec- tion in rats at a single equivalent dose of 10 mg/kg. Drug Delivery Downloaded from informahealthcare.com by University of Technology Sydney on 03/01/11 For personal use only. 558 H.-B. Tang et al. ing and release studies of a water soluble drug. J Contr Rel. 57:171–85. Gu, X.G., Schmitt, M., Hiasa, A., Nagata, Y., Ikeda, H., Sasaki, Y., Akiyoshi, K., Sunamoto, J., Nakamura, H., Kuribayashi, K., Shiku, H. (1998). A novel hydrophobized polysaccharide/oncoprotein complex vaccine induces in vitro and in vivo cellular and humoral immune responses against HER2-expressing murine sarcomas. Cancer Res. 58:3385–90. Gustafson, D.L., Rastatter, J.C., Colombo, T., Long, M.E. (2002). Doxorubicin pharmacokinetics: macromolecule binding, metabolism, and excretion in the context of a physiologic model. J Pharm Sci. 91:1488–501. Jakobsen, P., Sorensen, B., Bastholt, L., Mirza, M.R., Gjedde, S.B., Mouridsen, H.T., Rose, C. (1994). e pharmacokinetics of high- dose epirubicin and of the cardioprotector ADR-529 given together with cyclophosphamide, 5-uorouracil, and tamoxifen in meta- static breast-cancer patients. Cancer Chemoth Pharm. 35:45–52. Jakobsen, P., Steiness, E., Bastholt, L., Dalmark, M., Lorenzen, A., Petersen, D., Gjedde, S.B., Sandberg, E., Rose, C., Nielsen, O.S., et al. (1991). Multiple-dose pharmacokinetics of epirubicin at four dierent dose levels: studies in patients with metastatic breast cancer. Cancer Chemoth Pharma. 28:63–8. Jeong, Y.I., Na, H.S., Oh, J.S., Choi, K.C., Song, C.E., Lee, H.C. (2006). Adriamycin release from self-assembling nanospheres of poly(DL- lactide-co-glycolide)-grafted pullulan. Int J Pharm. 322:154–60. Jung, S.W., Jeong, Y.I., Kim, S.H. (2003). Characterization of hydro- phobized pullulan with various hydrophobicities. Int J Pharm. 254:109–21. Lanone, S., Boczkowski, J. (2006). Biomedical applications and poten- tial health risks of nanomaterials: molecular mechanisms. Curr Mol Med. 6:651–63. Leathers, T.D. (2003). Biotechnological production and applications of pullulan. Appl Microbiol Biotechnol. 62:468–73. Levchenko, T.S., Rammohan, R., Lukyanov, A.N., Whiteman, K.R., Torchilin, V.P. (2002). Liposome clearance in mice: the eect of a separate and combined presence of surface charge and polymer coating. Int J Pharm. 240:95–102. Li, S.D., Huang, L. (2008). Pharmacokinetics and biodistribution of nanoparticles. Mol Pharm. 5:496–504. Lourenco, C., Teixeira, M., Simoes, S., Gaspar, R. (1996). Steric stabili- zation of nanoparticles: size and surface properties. Int J Pharm. 138:1–12. Medina, C., Santos-Martinez, M.J., Radomski, A., Corrigan, O.I., Radomski, M.W. (2007). Nanoparticles: pharmacological and toxicological signicance. Br J Pharmacol. 150:552–8. Mross, K., Maessen, P., van der Vijgh, W.J., Gall, H., Boven, E., Pinedo, H.M. (1988). Pharmacokinetics and metabolism of epi- doxorubicin and doxorubicin in humans. J Clin Oncol. 6:517–26. Müller, R.H., Jacobs, C. (2002). Buparvaquone mucoadhesive nano- suspension: preparation, optimisation and long-term stability. Int J Pharm. 237:151–61. Na, K., Bum Lee T., Park, K.H., Shin, E.K., Lee, Y.B., Choi, H.K. (2003). Self-assembled nanoparticles of hydrophobically-modied polysaccharide bearing vitamin H as a targeted anti-cancer drug delivery system. Eur J Pharm Sci. 18:165–73. Na, K., Lee, K.H., Bae, Y.H. (2004). pH-sensitivity and pH-dependent interior structural change of self-assembled hydrogel nanopar- ticles of pullulan acetate/oligo-sulfonamide conjugate. J Cont Rel. 97:513–25. Park, K.H., Song, H.C., Na, K., Bom, H.S., Lee, K.H., Kim, S., Kang, D., Lee, D.H. (2007). Ionic strength-sensitive pullulan acetate nano- particles (PAN) for intratumoral administration of radioisotope: ionic strength-dependent aggregation behavior and (99m) Technetium retention property. Colloids Surf B Biointerfaces. 59:16–23. Rekha, M.R., Sharma, C.P. (2007). Pullulan as a promising biomaterial for biomedical applications: a perspective. Trends Biomater Artif Organs. 20:116–21. Seymour, L.W., Miyamoto, Y., Maeda, H., Brereton, M., Strohalm, J., Ulbrich, K., Duncan, R. (1995). Inuence of molecular weight on passive tumour accumulation of a soluble macromolecular drug carrier. Eur J Cancer. 31:766–70. Shimizu, T., Kishida, T., Hasegawa, U., Ueda, Y., Imanishi, J., Yamagishi, H., Akiyoshi, K., Otsuji, E., Mazda, O. (2008). Nanogel DDS enables sustained release of IL-12 for tumor immuno- therapy. Biochem Biophys Res Commun. 367:330–5. Shingel, K.I. (2004). Current knowledge on biosynthesis, biological activity, and chemical modication of the exopolysaccharide, pullulan. Carbohydr Res. 339:447–60. Sonaje, K., Lin, Y.H., Juang, J.H., Wey, S.P., Chen, C.T., Sung, H.W. (2009). In vivo evaluation of safety and ecacy of self-assembled nanoparticles for oral insulin delivery. Biomaterials. 30:2329–39. Tsuchihashi, M., Harashima, H., Kiwada, H. (1999). Development of a pharmacokinetic/pharmacodynamic (PK/PD)-simulation sys- tem for doxorubicin in long circulating liposomes in mice using peritoneal P388. J Contr Rel. 61:9–19. Vega-Villa, K.R., Takemoto, J.K., Yanez, J.A., Remsberg, C.M., Forrest, M.L., Davies, N.M. (2008). Clinical toxicities of nanocar- rier systems. Adv Drug Deliv Rev. 60:929–38. Yoksan, R., Chirachanchai, S. (2008). Amphiphilic chitosan nano- sphere: studies on formation, toxicity, and guest molecule incor- poration. Bioorg Med Chem. 16:2687–96. Zhang, H.Z., Gao, F.P., Liu, L.R., Li, X.M., Zhou, Z.M., Yang, X.D., Zhang, Q.Q. (2009). Pullulan acetate nanoparticles prepared by solvent diusion method for epirubicin chemotherapy. Colloids Surf B Biointerfaces. 71:19–26. Drug Delivery Downloaded from informahealthcare.com by University of Technology Sydney on 03/01/11 For personal use only. . studied the stability and toxicity of PANs, and further investigated the sustained release behavior in vivo of drug loading in PANs. PA was rstly. pullulan acetate nanoparticles (PANs) as a drug nanocarrier, pullulan acetate (PA) was synthesized and characterized. Its acetylation degree determined by the