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Transferrin receptor targeted PLA-TPGS micelles improved efficacy and safety in docetaxel delivery
Accepted Manuscript Title: Transferrin receptor targeted PLA-TPGS micellesimproved efficacy and safety in docetaxel delivery Author: Rahul Pratap Singh Gunjan Sharma Sonali Poornima Agrawal Bajarangprasad L. Pandey Biplob Koch Madaswamy S. Muthu PII: DOI: Reference:
S0141-8130(15)30177-X http://dx.doi.org/doi:10.1016/j.ijbiomac.2015.11.081 BIOMAC 5586
To appear in:
International Journal of Biological Macromolecules
Received date: Revised date: Accepted date:
17-10-2015 26-11-2015 27-11-2015
Please cite this article as: R.P. Singh, G. Sharma, P. Agrawal, B.L. Pandey, B. Koch, M.S. Muthu, Transferrin receptor targeted PLA-TPGS micellesimproved efficacy and safety in docetaxel delivery, International Journal of Biological Macromolecules (2015), http://dx.doi.org/10.1016/j.ijbiomac.2015.11.081 This is a PDF file of an unedited manuscript that has been accepted for publication. As a service to our customers we are providing this early version of the manuscript. The manuscript will undergo copyediting, typesetting, and review of the resulting proof before it is published in its final form. Please note that during the production process errors may be discovered which could affect the content, and all legal disclaimers that apply to the journal pertain.
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Transferrin receptor targeted PLA-TPGS micelles
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improved efficacy and safety in docetaxel delivery
3
Rahul Pratap Singha, Gunjan Sharmac,
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Sonalia, Poornima Agrawala, Bajarangprasad L. Pandeya,
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Biplob Kochc, Madaswamy S. Muthua, b*
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Department of Pharmacology, Institute of Medical Sciences, Banaras Hindu University, Varanasi 221005, U.P., India
b
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Department of Pharmaceutics, Indian Institute of Technology, Banaras Hindu University, Varanasi – 221005, India
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Department of Zoology, Faculty of Science, Banaras Hindu University, Varanasi 221005, U.P., India
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_______________________________________ *
Corresponding author: Department of Pharmacology, Institute of Medical Sciences, Banaras Hindu University, Varanasi – 221005, India Tel.: +91 9235195928; Fax: +91 542 2367568; E-mail: [email protected] (Madaswamy S. Muthu).
Singh et al: Revised submission to Int. Journal of Biological Macromolecules (26 Nov 2015) 1
Page 1 of 40
ABSTRACT
2
The aim of this work was to develop targeted polymeric micelles of poly-lactic acid-D-
3
α-tocopheryl polyethylene glycol 1000 succinate (PLA-TPGS), which are assembled along with
4
D-alpha-tocopheryl polyethylene glycol 1000 succinate-transferrin conjugate (TPGS-Tf), and
5
loaded docetaxel (DTX) as a model drug for enhanced treatment of lung cancer in comparison to
6
non-targeted and DTX injection (DocelTM). A549 human lung cancer cells were employed as an
7
in-vitro model to access cytotoxicity study of the DTX loaded polymeric micelles. The safety of
8
DTX formulations were studied by the measurement of alkaline phosphatase (ALP), lactate
9
dehydrogenase (LDH) and total protein levels in bronchoalveolar lavage (BAL) fluid of rats after
10
the treatments. The IC50 values demonstrated that the non-targeted and transferrin receptor
11
targeted polymeric micelles could be 7 and 70 folds more effective than DocelTM after 24 h
12
treatment with the A549 cells. Results suggested that transferrin receptor targeted polymeric
13
micelles have showed better efficacy and safety than the non-targeted polymeric micelles and
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DocelTM.
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Key words: Cytotoxicity, Lung cancer, Nanomedicine, Nanotechnology, Polymeric micelles,
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Safety, Transferrin conjugation
18 19 20 21 22 23 24 25
1. Introduction Lung cancer is one of the top most deaths causing disease in the world in both sexes (men Singh et al: Revised submission to Int. Journal of Biological Macromolecules (26 Nov 2015) 2
Page 2 of 40
and women). Based on lethality, the lung cancer is further categorized in two major classes
2
including small cell lung cancer (13%) or non-small cell lung cancer (83%) for the purposes of
3
treatment. The 1 and 5 year relative survival rates for lung cancer are 44% and 17%, respectively.
4
The lung cancer treatment includes surgery, radiation therapy, chemotherapy, and/or targeted
5
therapies. The lung cancer patients are usually treated by chemotherapy and targeted drugs [1].
6
Presently, various receptor targeted drug delivery systems have showed the possibilities to provide
7
effective treatments to cancer cells which may minimize the adverse effects of drugs to the healthy
8
cells [2].
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The nanomedicine is the application of nanotechnology to medicine, which is highly
10
capable to develop nanoparticles drug delivery system [3]. These nano drug deliveries are enable
11
to target cancer cells in highly effective manner by enhanced permeability and retention (EPR)
12
effects, which is an important feature to make cancer targeting drug delivery system [4-10]. The
13
several
14
(D,L-lactide-co-glycolide) (PLGA) nanoparticles, carbon nanotubes and polymeric micelles
15
[11-22]. Among these, polymeric micelles are drug delivery systems, which are widely applied in
16
the lipophilic or poorly soluble drugs [17,23-25].
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systems
have
been
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delivery
developed
such
as
liposomes,
poly
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drug
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The polymeric micelles are formed through the multimolecular assembly of block
18
copolymers as novel core-shell typed nano carriers for drug targeting [26,27]. The polymeric
19
micelles outer corona made up by using the hydrophilic polymer segments, which act as a
20
stabilizing interface between the hydrophobic drug and the external medium and maintains the
21
aqueous solubility of polymeric micelles [28-30].
22
Polymeric micelles are emerging polymeric nano carriers, which act as a highly integrated
23
nanoplatform for cancer targeting (passive as well as active targeting), drug delivery and tumor
Singh et al: Revised submission to Int. Journal of Biological Macromolecules (26 Nov 2015) 3
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imaging applications [31-33]. It have several extraordinary properties including biocompatibility,
2
high stability in both in-vitro and in-vivo, and also have capacity to effectively solubilize a variety
3
of poorly soluble drugs, changing the release profile of the incorporated pharmaceutical agents,
4
and the ability to accumulate in the target zone based on the EPR effects [34-35]. These polymeric
5
micelles can be used as targeted drug delivery systems in lung cancer treatment [17, 36]. Also, it
6
can be conjugated with different biomolecules including targeting ligand, antibody,
7
P-glycoprotein (P-gp) inhibitor and diagnostic agents, which are highly beneficial to multiple drug
8
resistance (MDR) types of lung cancer treatment [37-39]. Also, polymeric micelles are highly
9
effective to increase EPR effect in cancer treatment. The polymeric micelles are frequently using
10
in the several cancer treatment including glioma, renal, stomach, lung, and pancreatic cancer at
11
phase I and phase II clinical trials. [28, 40, 41].
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Poly-lactic acid (PLA) is a biodegradable and biocompatible polymer, which is widely
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using in the biomedical for making safe and biodegradable nano carriers for cancer treatment. The
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United States Food and Drug Administration (US FDA) has approved their uses in drug delivery
15
systems. The monomer of PLA i.e., L-lactic acid (L-LA), which can be efficiently produced by
16
fermentation from renewable resources such as starchy materials and sugars. The PLA degrades to
17
its monomer, L-LA, which is a normal metabolite of the human [13]. D-α-tocopheryl polyethylene
18
glycol 1000 succinate (TPGS) mostly studied in liposomes and polymeric nanoparticles which
19
enhanced cellular uptake, cytotoxicity and showed prolonged circulation time [14,15]. TPGS is
20
simply known as vitamin E, which is provides better permeation effects of hydrophilic and
21
hydrophobic drug molecules. It is FDA approved water-soluble derivative of natural Vitamin E
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(PEGylated vitamin E). TPGS is a derivative of the natural vitamin E (alpha-tocopherol) and
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polyethylene glycol 1000. It is also non-ionic and highly hydrophilic, is used as solubilizer,
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absorption enhancer and a vehicle for various formulations [13,15,22]. PLA-TPGS is a block
2
copolymer of L-LA and TPGS. The PLA-TPGS block-copolymer was prepared by using ring
3
opening polymerization method. It has been used in the fabrication of nano drug delivery systems
4
because of its safety, stealth effect, targeting feasibility, multifunctional capability,
5
biocompatibility, size tunability and ease of preparation of nanoparticles. In recent study, de
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Melo-Diogo et al., has prepared a highly effective drug delivery of triple multiple drugs
7
(crizotinib–palbociclib–sildenafil) loaded PLA-TPGS micelles and improved lung cancer
8
treatment
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(Crizotinib–Palbociclib) loaded micelles treatment [17]. The polymeric micelles of PLA-TPGS
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can be prepared at the critical micelles concentration (CMC) of 0.016 mg/mL [17]. Further,
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targeting can be achieved via the EPR into the areas with the compromised vasculature and by
12
attaching specific targeting ligand molecules to the micelle surface [13, 42-44].
A549
cells
in
comparison
to
single
(Crizotinib)
and
dual
drug
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In this study, docetaxel (DTX) was used as anticancer model drug for the lung cancer
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treatment. DTX (N-debenzoyl-N-tertbutoxycarbonyl-10-deacetyl-paclitaxel) is a semisynthetic
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derivative of the taxoid family of antineoplastic agents. It is an analog of paclitaxel, which is
16
extracted from the needles of the European yew tree (Taxus baccata L). DTX has been found to be
17
more effective than paclitaxel against breast, ovarian, lung, brain and neck cancers [15, 16]. To
18
overcome the poor solubility of DTX and to reduce the systemic toxicity, conventional and various
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novel formulations have been developed [20, 22, 45]. However, there is a problem that needs to be
20
solved to meet the requirements for its clinical use i.e., targeted delivery of DTX to cancer cells.
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Transferrin receptor is a cell membrane-associated glycoprotein on the surface of the cells. It
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plays an important role in iron homeostasis and the regulation of cell growth in cells. The
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transferrin receptor expression on cancer cells can be up to 100-fold higher than the average
Singh et al: Revised submission to Int. Journal of Biological Macromolecules (26 Nov 2015) 5
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expression in normal cells owing to their rapid proliferation rate and iron demand, thereby
2
transferrin has been explored as a targeting ligand for nanocarriers to deliver therapeutic and
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diagnostic agent into cancer cells [46,47]. This approach shows the advantage of continuous
4
recycling of the transferrin receptor from the surface to the endosomal compartment to make it
5
efficient route for the internalization of nanoplatforms [20]. In one study, it was reported that
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among the primary lung cancer cases, 19% of adenocarcinomas showed positive results for
7
transferrin receptor overexpression which showed the possibility of transferrin receptor targeted
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delivery of micelles for lung cancer therapy [48].
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In this study, PLA-TPGS (block copolymer of L-LA and TPGS) was used to make polymeric
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micelles. DTX was loaded into polymeric micelles by using solvent displacement method.
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Transferrin was conjugated to activated TPGS-COOH, which serve as targeting agent to transport
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DTX into the human lung cancer cells (A549). The targeting effects of transferrin conjugated
13
polymeric micelles (targeted) were compared closely with non-targeted polymeric micelles and
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clinical DocelTM (DTX injection). In-vitro cytotoxicity of A549 cells was assessed and the IC50
15
value at 24 h was assessed to evaluate the therapeutic effect of the DTX loaded PLA-TPGS
16
polymeric micelles with or without targeting function. Further, PLA-TPGS micelles were tested
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in-vivo on rats model for safety applications i.e., alkaline phosphatase (ALP), lactate
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dehydrogenase (LDH), and total protein levels in bronchoalveolar lavage (BAL) fluid of lung
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tissue after intravenous (i.v.) administrations.
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2. Materials and methods
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2.1. Materials
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Docetaxel (DTX) of purity 99.56% was obtained from Neon Laboratories Ltd, Mumbai, India
Singh et al: Revised submission to Int. Journal of Biological Macromolecules (26 Nov 2015) 6
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as gift sample. D-alpha-tocopheryl polyethylene glycol 1000 succinate (TPGS) was obtained from
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Antares Health Products., St. Charles, U.S.A. as gift sample. Dialysis membrane (Spectra/Por7®)
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of 1 KDa molecular weight cut off was purchased from Spectrum Laboratories Inc., Rancho
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Dominguez, CA, U.S.A. Clinical formulation DocelTM was purchased from RPG Life Sciences
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Limited, Mumbai, India. L-Lactide (L-LA) monomer (3,6-Dimethyl-1,4-dioxane-2,5-dione),
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stannous octoate (Sn(Oct)2), transferrin (Molecular weight of 80 kDa), ethanol and phosphate
7
buffer saline (PBS) were purchased from Sigma–Aldrich, St. Louis, MO, USA. Anhydrous
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toluene, dichloromethane and methanol were purchased from Loba Chemie Pvt. Ltd, New Delhi,
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India. Human lung cancer cell lines (A549) were provided by National Centre for Cell Science,
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Pune, India. Dulbecco's Modified Eagle’s Medium (DMEM), fetal bovine serum (FBS),
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streptomycin, penicillin, L-glutamine and trypsin-EDTA were purchased from Genetix Biotech
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Asia Pvt. Ltd., Mumbai, India. T-25 culture flask and 96-well culture plates purchased from
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Tarsons
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5-diphenyltetrazoliumbromide (MTT) were purchased from Himedia Laboratories, Mumbai,
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India. All other chemicals were of analytical grade.
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2.2. Methods
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2.2.1. Synthesis of PLA-TPGS copolymer
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Ltd.,
Kolkata,
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Pvt.
India.
3-(4,
5-dimethylthiazolyl-2-yl)-2,
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Products
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The PLA-TPGS copolymer was synthesized by ring opening polymerization (ROP) of
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L-LA with TPGS in the presence of stannous octoate [Sn(Oct)2] as catalyst. Briefly, L-LA and
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TPGS (1:1 ratio) were added to a round bottom flask (RBF). The system was purged with nitrogen
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and anhydrous toluene (25 mL per gram of L-LA) was added. Subsequently Sn(Oct)2 (0.5% w/v)
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was added and the ROP reaction was carried out at 120 0C for 4 h, under nitrogen (N2) atmosphere.
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At the end of polymerization, the toluene was evaporated by using rotary evaporator (Buchi R-210
Singh et al: Revised submission to Int. Journal of Biological Macromolecules (26 Nov 2015) 7
Page 7 of 40
Advanced, Switzerland) at 37 0C and the resulting product was dissolved in dichloromethane
2
(DCM) and precipitated in cold methanol. The recovered precipitate was dialyzed for 2 days
3
against acetone and 3 days against distilled water. Finally, the diblock copolymer was lyophilized
4
and a white powder was obtained [11,17,41,47,49]. The schematic diagram of PLA-TPGS
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copolymer synthesis resents in Fig. 1A.
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2.2.2. Synthesis of TPGS-COOH (activation of TPGS) and its conjugate
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For the synthesis of TPGS and transferrin conjugate, TPGS was first activated (i.e.,
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TPGS-COOH) by succinic anhydride through ring-opening reaction in the presence of DMAP
9
[20]. In brief, TPGS (0.77 g, 0.5 mM), succinic anhydride (0.10 g, 1 mM) and DMAP (0.12 g, 1
10
mM) were mixed and heated at 100 0C under nitrogen atmosphere for 24 h. The mixture was
11
cooled to room temperature, dissolved in 5 ml of cold dichloromethane, filtered to remove
12
excessive succinic anhydride and then precipitated in 100 ml of diethyl ether at -10 0C overnight.
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The white TPGS-COOH precipitate was filtered and dried in vacuum [19,20,22]. The schematic
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diagram of synthesis of TPGS-COOH (activation of TPGS) resents in Fig. 1B (i).
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Further, TPGS-COOH carboxyl group was conjugated to the transferrin by carbodiimide
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chemistry with the help of EDC and NHS in phosphate buffer saline (pH 5.5) [20]. In brief, for
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conjugation of transferrin to TPGS-COOH, 1-ethyl-3-(3- dimethylaminopropyl) carbodiimide
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(EDC) and N-hydroxysuccinimide (NHS) (both are catalyst) were added into TPGS-COOH with a
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molar ratio of 1:5 (TPGS-COOH : EDC or NHS) in phosphate buffer saline (pH 5.5). In brief,
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TPGS-COOH (200 mg), EDC (96 mg) and NHS (74 mg) were mixed in 2 ml of phosphate buffer
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saline (pH 5.5) at 25 0C for 5 h, stored in a refrigerator at 4 0C over 24 h, mixed with 1 ml of 0.2 %
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(w/v) transferrin and stirred at 4 0C over 8 h. The resulted product was then dialyzed using a
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dialyzing membrane (MWCO: 12 kDa) against phosphate buffer saline (pH 5.5) for 48 h in order
Singh et al: Revised submission to Int. Journal of Biological Macromolecules (26 Nov 2015) 8
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to remove excess TPGS-COOH, NHS and EDC. The dialyzed product (i.e., TPGS-Tf) was freeze
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dried and used for micelle formation [20,22]. The schematic diagram of synthesis of TPGS-Tf
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resents in Fig. 1B (ii).
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2.2.3. Preparation of PLA-TPGS polymeric micelles using solvent displacement (SD) method
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Briefly, for DTX loaded polymeric micelles formulation, 3 mg DTX and 25 mg
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PLA-TPGS copolymer were dissolved in 5 ml of DCM/methanol (1:1 v/v). After that, the solvent
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was evaporated by using rotary evaporator (Buchi R-210 Advanced, Switzerland) at 37 0C and
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then film was hydrated with 10 ml of 1mM phosphate buffer saline (PBS), pH 7.4. After that the
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mixture was incubated in an orbital water bath shaker at 37 0C for 48 h. The excess
10
non-incorporated DTX was separated by filtration (using a 0.22-µm filter) before characterization.
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The targeted polymeric micelles were prepared with the addition of 10 mg of TPGS-Tf at 4 0C to
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obtain higher drug encapsulation, drug controlled release and drug targeting effects on cancer cell
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lines (Table 1). For the preparation of placebo polymeric micelles, the formulation process used
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was the same as previously described but without the inclusion of DTX [16,17]. The schematic
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diagram of preparation of non-targeted and targeted polymeric micelles resents in Fig. 1C (i) and
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(ii), respectively.
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2.2.4. Fourier transform infrared (FTIR) spectroscopy
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The FTIR spectroscopy for L-LA, TPGS, PLA-TPGS copolymer, TPGS-COOH and
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TPGS-Tf were performed using compressed KBr pellet method in Perkin Elmer FTIR
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spectrophotometer (Perkin Elmer Spectrum Two, Waltham, Massachusetts, U.S.A). The scanning
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range was 400-4000 cm-1.
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2.2.5. Particle size, polydispersity and zeta potential of polymeric micelles
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Size, polydispersity and zeta potential of the PLA-TPGS (placebo micelles),
Singh et al: Revised submission to Int. Journal of Biological Macromolecules (26 Nov 2015) 9
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DTX-PLA-TPGS (non-targeted micelles) and DTX-PLA-TPGS-Tf (targeted micelles) were
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measured by PCS using a Zetasizer ver. 7.03, Malvern instruments Ltd, Malvern, UK [16].
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2.2.6. Determination of encapsulation efficiency and drug loading of polymeric micelles The DTX encapsulation efficiency of non-targeted and targeted polymeric micelles were
5
determined by UV spectrophotometer (Shimadzu 1800, Tokyo, Japan). Briefly, 2 ml aliquots of
6
polymeric micelles were evaporated to dryness by rotary evaporator under reduced pressure at 35
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0
8
h at 37 0C to fully leach out the DTX. Then, the solution was centrifuged at 10,000 rpm for 10 min
9
at 4 0C, and the supernatant was collected. The supernatant (500 µl) was further diluted to 2 ml of
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methanol. Then light absorption was measured at 229 nm using spectrophotometer. The drug
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encapsulation efficiency was defined as the ratio between the amount of DTX encapsulated in the
12
polymeric micelles and that added in the polymeric micelles preparation process. The drug loading
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was calculated as the weight of drug (µg) per one mg of the drug-loaded polymeric micelles
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[20,22]. All samples were done in triplicate.
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2.2.7. In-vitro drug release studies
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The release patterns of DTX from DTX-PLA-TPGS and DTX-PLA-TPGS-Tf were studied
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by using dialysis bag diffusion technique [15,22]. The formulation of a volume equivalent to 300
18
µg of DTX were placed in the dialysis bag (cellulose membrane, molecular weight cut off 1 kDa),
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hermetically sealed and immersed into 100 ml of PBS (pH 7.4). The entire system as kept at 37 ±
20
0.5 0C with continuous shaking at 100 rpm/min. Then, 5 ml samples were withdrawn from the
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receptor compartment at predetermined time intervals and replaced by fresh medium. The samples
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were filtered through 0.45 mm syringe filter before analysis. The DTX content in the samples was
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determined by using UV spectrophotometer (Shimadzu 1800, Tokyo, Japan). Then drug release
Singh et al: Revised submission to Int. Journal of Biological Macromolecules (26 Nov 2015) 10
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profiles were calculated [20, 50].
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2.2.8. Cell culture A549 human lung cancer cell lines were grown in DMEM supplemented with 10% FBS,
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100 units/mL penicillin and 100 µg/mL streptomycin solutions. The cell lines were grown at 37 °C
5
in the presence of 5% CO2.
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2.2.9. Cytotoxicity of PLA-TPGS polymeric micelles
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The cytotoxicity of DTX formulations i.e., DTX-PLA-TPGS, DTX-PLA-TPGS-Tf and
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DocelTM (DTX injection) were performed on A549 human lung cancer cell lines by standard MTT
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assay. A549 cell lines were seeded into 96 well culture plates (Tarsons Products Pvt. Ltd.) at the
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density of 1×104 viable cells/well with DMEM and incubated at least overnight to allow cell
11
attachment. The spent medium was discarded and the cells were incubated with both
12
DTX-PLA-TPGS and DTX-PLA-TPGS-Tf, and their cytotoxicity was assessed in comparison
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with DocelTM at 0.025, 0.25, 2.5 and 25 µg/ml equivalent drug concentrations for 24 h. After 24 h,
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medium was removed and 100 µL medium and 10 µL of 5 mg/mL MTT in PBS, pH 7.4 was added
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to each well of the plate. The plates were further incubated for 2 h at 37 0C in the incubator. Then
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the medium and MTT were removed and 100 µL of DMSO was added to dissolve the MTT
17
formazan crystals. The absorbance of samples was measured at 570 nm by microplate reader [23].
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Cytotoxicity was calculated as the percentage of treated cells relative to untreated cells at 570 nm.
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The percent of the cell viability was calculated using the equation:
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Cell viability (%) = Absorbance of treated cells/Absorbance of control cells) X 100 2.2.10. In-vivo safety using bronchoalveolar lavage (BAL) fluids of rats
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The animal caring, handling, husbandry and the protocols were approved by the Institute of
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Medical Sciences (IMS), Banaras Hindu University (BHU), Varanasi, India. Both sexes (male and
Singh et al: Revised submission to Int. Journal of Biological Macromolecules (26 Nov 2015) 11
Page 11 of 40
female) rats of 150-200 gm (or 4–5 weeks old) were supplied by the Central Animal House of
2
IMS, BHU and maintained at animal room of the Department of Pharmacology of IMS, BHU,
3
Varanasi, India. The animals were acclimatized at a temperature of 25 ± 2 0C and a relative
4
humidity of 50–60% under natural light/dark conditions and given aseptic full-price nutritional
5
pellet feed and sterile water available ad libitum for 4–5 days before experiments. The study
6
protocol was follow guideline of Committee for the Purpose of Control and Supervision on
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Experiments on Animals (CPCSEA; Guidelines for Laboratory Animal Facility) Registration No.
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Dean/2015/CAEC/1262 of Banaras Hindu University, Varanasi (U.P.), India.
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The animals were randomly divided into 5 (4 treatment groups + 1 control group) groups
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with approximately 4 rats per group (n=4). One week after the initiation of acclimatization, all rats
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(except control animal) were treated with plain PLA-TPGS (placebo micelles), DTX-PLA-TPGS
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(5 mg/kg of DTX), DTX-PLA-TPGS-Tf (5 mg/kg of DTX) and DocelTM (5 mg/kg of DTX) and
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one control group was treated with normal saline (0.9% NaCl) solution via the i.v. route. Drinking
14
water was available ad libitum. During the treatment, the health conditions of rats were monitored
15
every day. At the indicated time of interval 7, 15 and 30 days of polymeric micelles and DocelTM
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formulation administrations. The rats were sacrificed with an intraperitoneal (i.p.) injection of
17
urethane (1.5 g/kg rats). The thorax was opened and the lung perfused with normal saline solution
18
(26.5 ml/kg rats). Further trachea was then cannulated and BAL fluid was performed by injecting
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approximately 4 mL of normal saline solution and thorough rinsing of the lung. The BAL fluid
20
was recovered and centrifuged at 400×g at 4 0C for 10 min and then stored at -20 0C until analysis
21
[50]. All biochemical assays were performed on BAL fluids such as estimation of ALP (Span
22
Diagnostics Ltd., Surat, India), LDH and total protein count (Crest Biosystems, Goa, India) by
23
using respective diagnostic kits according to the manufacturer’s instructions. ALP activity is a
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measure of type II alveolar epithelial cell secretory activity, and increased ALP activity in BAL
2
fluids is considered to be an indicator of type II cell toxicity. LDH is a cytoplasmic enzyme and is
3
used as an indicator of cell injury. Increases in BAL fluid protein concentrations generally were
4
consistent with enhanced permeability of vascular proteins into alveolar regions [51, 52].
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2.2.11. Statistical analysis
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Results are given as mean ± standard deviation (S.D). Mean values of particle size,
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encapsulation efficiency, in-vitro and in-vivo data were compared using the Student’s t-test.
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Differences are considered significant at a level of P<0.05.
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3. Results and discussions
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3.1. Preparation of different block-copolymer, TPGS-Tf and polymeric micelles
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Fig. 1A shows the schematic production of PLA-TPGS block-copolymer, that was
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prepared by using ring opening polymerization method in presence of stannous octoate (Sn(oct)2)
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as catalyst in the reaction under nitrogen gas environment at 120 0C for 4 h [17,48]. In the
15
polymerization reaction hydroxyl terminus (-OH) of TPGS was used as initiator. Further, this
16
amphiphilic copolymer of PLA-TPGS was used to prepared polymeric micelles. Fig. 1B (i) shows
17
the activation TPGS in to TPGS-COOH in the presence of succinic anhydride and DMAP at 100
18
0
19
attached to the activated TPGS (TPGS-COOH) by carbodiimide chemistry with the help of EDC
20
and NHS in phosphate buffer saline (pH 5.5) [20]. Fig. 1C (i and ii) clearly shows the preparation
21
DTX loaded polymeric micelles. The DTX was loaded using solvent displacement (SD) method.
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C under nitrogen atmosphere for 24 h [22]. Fig. 1B (ii) shows that transferrin was covalently
22 23
Table 1 (approximate position)
Singh et al: Revised submission to Int. Journal of Biological Macromolecules (26 Nov 2015) 13
Page 13 of 40
1
Fig. 1 (approximate position)
2 3
3.2. Characterization of L-LA, TPGS, PLA-TPGS, TPGS-COOH and TPGS-Tf by FTIR Fig.2A shows the FTIR spectra of L-LA, TPGS and PLA-TPGS, which is clearly revealed
5
the successful polymerization of L-LA and TPGS in to PLA-TPGS block-copolymer. In the
6
spectra, the C-H stretching is clearly appearing, which is due to methyl group vibrations from
7
L-LA (2925.55 cm-1), TPGS (2870.67 cm-1) and PLA-TPGS (2926.62 cm-1). The carbonyl
8
vibration peak was also present in all the spectra. The carbonyl band shift from TPGS to the
9
synthesized diblock-copolymer (PLA-TPGS) was also visible (TPGS: 1737.75 cm-1; PLA-TPGS:
10
1755.73 cm-1; L-LA: 1766.55 cm-1). Another important peak for -C-C- stretching is aromatic ring
11
was appeared in both TPGS and PLA-TPGS copolymer peak at 1465.06 and 1455.21 cm-1,
12
respectively. The peak at 1382.4 cm-1for -CH2 group of PEG chain was observed in PLA-TPGS
13
copolymer. In TPGS and PLA-TPGS FTIR spectra, the C-O stretch band is also present at peak
14
951.46 and 1252.4 cm-1, respectively. Finally at peak 3425.51 cm-1 band is assigned to the terminal
15
hydroxyl group of the PLA chain.
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Fig.2B shows FTIR spectra of TPGS-COOH and TPGS-Tf. In FTIR spectra of
17
TPGS-COOH, the –C=O stretching was clearly appeared peaks at 1736.47 cm-1, which is clearly
18
indicating a successful synthesis of TPGS-COOH. In transferrin conjugated TPGS, the linkage
19
between -COOH group of TPGS and -NH2 group of transferrin was confirmed by the amide
20
(-CO-NH-) stretching peak at 1634.02 cm-1. In both TPGS and TPGS-COOH, the absorption
21
bands at 3450.04 and 3452.3 cm-1 were due to the terminal hydroxyl group.
22 23
Figure 2 (approximate position)
Singh et al: Revised submission to Int. Journal of Biological Macromolecules (26 Nov 2015) 14
Page 14 of 40
1 2
3.3. Particle size, polydispersity and zeta potential of polymeric micelles The mean particle size and polydispersity of PLA-TPGS (placebo micelles),
4
DTX-PLA-TPGS and DTX-PLA-TPGS-Tf were listed in Table 2. PCS measurements were
5
undertaken in multimodal analysis to get a true reflection of particle size distribution. The particle
6
size distribution curves for all the samples were unimodal. The mean sizes of PLA-TPGS,
7
DTX-PLA-TPGS, and DTX-PLA-TPGS-Tf were 84.09 ± 7.3, 135 ± 6.5 and 184 ± 9.92 nm,
8
respectively (Fig.3A to C). The PLA-TPGS polymeric micelles were observed in very small size,
9
which are suitable for therapeutic application in cancer treatment [14,16]. The particle size results
10
indicate that incorporation of DTX and targeting ligand (transferrin) conjugation on the surface of
11
targeted polymeric micelles (DTX-PLA-TPGS-Tf) leads to significant (P < 0.05) increase in the
12
size in comparison to DTX-PLA-TPGS and PLA-TPGS. The size of non-targeted and targeted
13
polymeric micelles were bigger that the placebo polymeric micelles. This results may be due the
14
packaged micelles contained the more hydrophobic drugs in their cores, thus increasing the
15
diameter of the micelles in aggregation. It was reported that polymeric micelles size typically in
16
the range of ˂200 nm are suitable for drug delivery in cancer therapy. The polydispersity of all the
17
batches of polymeric micelles showed quite narrow size distribution, which is nearer to 0.5
18
(Fig.3B). The zeta potential of all the polymeric micelles were found to be negatively charged
19
except for the transferrin conjugated polymeric micelles (Table 2). The negative zeta potential of
20
plain was found to be higher than that of DTX loaded polymeric micelles owing to the better
21
packing of -OH on the surface of polymeric micelles. Also the raise in positive charge on the
22
transferrin conjugated polymeric micelles was due to the presence of amino ends on the surface
23
[20].
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Page 15 of 40
1
3.4. Determination of encapsulation efficiency and drug loading of polymeric micelles Drug encapsulation efficiency was calculated as the percentage ratio between amount of
3
drug loaded in polymeric micelles and amount of the drug added during fabrication of polymeric
4
micelles [28,41,45]. Fig.3D shows the drug encapsulation efficiency of the DTX-PLA-TPGS and
5
DTX-PLA-TPGS-Tf were 71.14 ± 6.7 and 86.63 ± 4.2%, respectively (Table 2). The targeted
6
polymeric micelles (DTX-PLA-TPGS-Tf) showed significant increase (P<0.05) in the drug
7
encapsulation in comparison to non-targeted polymeric micelles (DTX-PLA-TPGS). This may be
8
because of the influence of TPGS-Tf conjugate to surface of polymeric micelles that leads to
9
enhance drug encapsulation efficiency. Drug loading is defined as the weight of drug (µg) per mg
10
of the drug loaded polymeric micelles. The drug loading of the non-targeted polymeric micelles
11
(DTX-PLA-TPGS) was 37.23±3.2 µg/mg. The drug loading of the targeted (DTX-PLA-TPGS-Tf)
12
polymeric micelles was 39.69 ± 2.4 µg/mg (Table 2). As mentioned earlier, addition of TPGS-Tf
13
into the micelle formation might lead to slight increase (P < 0.05) in drug loading and drug
14
encapsulation efficiency for DTX-PLA-TPGS-Tf comparison to DTX-PLA-TPGS.
16 17 18 19
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Table 2 (approximate position)
Figure 3 (approximate position)
3.5. In-vitro drug release studies
20
Fig. 4 shows the accumulated percentage release of DTX from polymeric micelles and
21
DocelTM in the medium of PBS (pH 7.4) under sink condition. The DTX-PLA-TPGS and
22
DTX-PLA-TPGS-Tf showed a sustained release for 72 h without any burst release in comparison
23
to DocelTM. After 72 h of dialysis in PBS (pH 7.4), the percentage of DTX released from the
Singh et al: Revised submission to Int. Journal of Biological Macromolecules (26 Nov 2015) 16
Page 16 of 40
preparations were 90.35, 66.72 and 58.23% for the DocelTM, DTX-PLA-TPGS, and
2
DTX-PLA-TPGS-Tf, respectively. The DTX-PLA-TPGS showed sustained drug release effects
3
due to a strong interaction between the DTX and polymeric micelles in comparison to DocelTM.
4
There was a significant (P<0.05) decrease in the in vitro drug release from the
5
DTX-PLA-TPGS-Tf comparison to the DTX-PLA-TPGS and DocelTM. These results may be
6
explained by the influence of transferrin on the micelles surface which was included as TPGS-Tf.
7
The t50% in PBS (pH 7.4) for DocelTM, polymeric micelles of DTX-PLA-TPGS and
8
DTX-PLA-TPGS-Tf containing DTX were about 16, 44 and 58 h, respectively. The DocelTM did
9
not show sustain the drug release. There was a significant (P<0.05) decrease in the t50% of the
10
DTX-PLA-TPGS, and DTX-PLA-TPGS-Tf in comparison with the DocelTM. It may be because of
11
PLA-TPGS structure polymeric micelles, which have followed sustained drug release in PBS up to
12
72 h. Interestingly, the sustained drug release kinetics of DTX-PLA-TPGS-Tf was related to the
13
transferrin conjugate on the micelles [20].
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Figure 4 (approximate position)
3.6. Cytotoxicity of drug formulations
18
In-vitro cytotoxicity in the A549 human lung cancer cells was assessed after 24 h
19
incubation with the DTX formulated in the DTX-PLA-TPGS and DTX-PLA-TPGS-Tf at 37 0C in
20
comparison with that of DocelTM at the equivalent drug concentration. The results are presented in
21
Fig. 5. It is worthy to note that the DTX-PLA-TPGS achieved the higher cytotoxicity compared
22
with the case of DocelTM treatment. This could be due to the effect of enhanced cellular uptake and
23
sustained drug release manner of DTX from the PLA-TPGS polymeric micelles structure.
Singh et al: Revised submission to Int. Journal of Biological Macromolecules (26 Nov 2015) 17
Page 17 of 40
Interestingly, DTX-PLA-TPGS-Tf resulted in further raise in cytotoxicity for A549 cells
2
compared with the DTX-PLA-TPGS. It is straightforward to understand that the increase in drug
3
concentration from 0.025 µg/ml to 25 µg/ml resulted in targeted and higher cytotoxicity for
4
DTX-PLA-TPGS-Tf due to transferrin receptor mediated endocytosis mechanism (Fig.5 and
5
Fig.6). In order to demonstrate the advantages of the DTX loaded polymeric micelles, a
6
quantitative index of inhibitory concentration, IC50, which is the drug concentration required to
7
induce 50% death of the cells incubated in a designated period, was determined. For instance, after
8
24 h incubation, IC50 for each of the three types of DTX formulations, namely the
9
DTX-PLA-TPGS and DTX-PLA-TPGS-Tf vs DocelTM were determined from the cytotoxicity
10
data to be 5.12 ± 1.39, 0.63 ± 0.22 vs 45.98 ± 1.70 µg/mL, respectively observed for A549 cells
11
which imply that the drug formulated in the DTX-PLA-TPGS and DTX-PLA-TPGS-Tf could be
12
7.7 and 70.34 folds more efficient than DocelTM after 24 h treatment (Table 3), respectively. Also,
13
results indicate that in order to kill A549 cells, the DTX-PLA-TPGS and DTX-PLA-TPGS-Tf
14
require significantly (P<0.05) lower drug concentrations in comparison to DocelTM (Fig.5 and
15
Table 4). DTX-PLA-TPGS has enhanced cytotoxicity in A549 cells because of PLA-TPGS
16
amphiphilic structure polymeric micelles, which inhibited P-gp efflux mechanism and provide
17
higher
18
(DTX-PLA-TPGS-Tf) have further enhanced cytotoxicity in A549 cells can be possibly attributed
19
to transferrin receptor targeting effect on the A549 cells (Fig.6). These results suggest that
20
transferrin decoration could significantly increase the cellular uptake of the polymeric micelles
21
[42]. Most importantly, transferrin conjugation on the polymeric micelles (DTX-PLA-TPGS-Tf)
22
would imply high concentration of drug to lung cancer cells which may reduce the systemic side
23
effects as well as cost for clinical use. Fig. 6 shows the cellular uptake mechanism of DTX
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drug
concentration
into
cells
(Fig.6).
The
targeted
polymeric
micelles
Singh et al: Revised submission to Int. Journal of Biological Macromolecules (26 Nov 2015) 18
Page 18 of 40
formulations. The targeted and non-trageted polymeric micelles have followed transferrin receptor
2
targeted endocytosis and phogocytosis effects, respectively. Kim et al., have proved that
3
polymeric micelles did not produce any toxicity at the concentration 0.0001–1 µg/ml of
4
mPEG-PDLLA copolymer in both cell lines i.e., human breast cancer cell lines (MCF7) and
5
human ovarian cancer cell lines (OVCAR-3) [37]. Recent study, de Melo-Diogo et al., have
6
proved that the biocompatibility of PLA-TPGS copolymer on 549 cell line, suggested that the
7
PLA-TPGS will not produce cytotoxic effects on cells [17].
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Table 3 (approximate position)
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Figure 5 (approximate position)
10
Figure 6 (approximate position) 3.7. In-vivo safety using bronchoalveolar lavage (BAL) fluids of rats
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8
Lung toxicity of DTX has been reported by various researcher in both mouse and rat
13
models. Normal saline exposure did not show any changes of any biochemical parameters in BAL
14
fluid. The administration of DTX formulation into the animal models induced inflammations and
15
fibrosis. To prove the safety of the DTX for lung cancer therapy, lung toxicity parameters were
16
measured. The lung toxicity parameters were observed after 7, 15 and 30 days of i.v.
17
administrations of PLA-TPGS (placebo micelles), DTX-PLA-TPGS, DTX-PLA-TPGS-Tf and
18
DocelTM. The PLA-TPGS micelles, DTX-PLA-TPGS and DTX-PLA-TPGS-Tf did not induce
19
significant (P>0.05) lung toxicity in comparison to DocelTM treated group, as evidenced from the
20
different pulmonary toxicity marker levels such as ALP, LDH and total protein counts in BAL
21
fluid of rats [50, 51].
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After 7 days ALP, LHD and protein counts levels in BAL fluids were significantly
23
(P<0.05) increased in the animal group which received DocelTM in compared to the control group
Singh et al: Revised submission to Int. Journal of Biological Macromolecules (26 Nov 2015) 19
Page 19 of 40
(normal saline treated) of animals (Fig. 7). At 15 and 30 days of post exposure, similar trends were
2
found to DocelTM. In comparison to control group (saline treated), a non-significant (P>0.05)
3
differences were observed in the ALP (Fig.7A), LDH levels (Fig.7B) and total protein counts
4
(Fig.7C) after i.v. administration of DTX-PLA-TPGS and DTX-PLA-TPGS-Tf. The major
5
adverse effects of DTX are their capabilities of damage alveoli cells, tissue damage and induce the
6
pulmonary toxicity after the i.v. administrations. The pulmonary toxicity of DTX is mainly due to
7
the poor solubility in aqueous media and also higher risk to normal cells by the activation of ROS
8
generation in the lung cells (Fig.7).
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Figure 7 (approximate position)
12
4. Conclusions
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In this work, we developed transferrin conjugated PLA-TPGS micelles as effective and
14
safer platforms in DTX delivery for lung cancer therapy. Our research confirms that the solvent
15
displacement method as suitable for loading of DTX into polymeric micelles. The non-targeted
16
and targeted (transferrin conjugated) polymeric micelles showed drug encapsulation efficiency up
17
to 86%. The particle size analysis showed that the polymeric micelles are well structured in nano
18
size between 84.9 to 184.8 nm. In-vitro drug release profiles revealed a desired sustained drug
19
release manner of the polymeric micelles. The DTX-PLA-TPGS and DTX-PLA-TPGS-Tf
20
achieved up to 7.7 and 70.34 folds decrease in IC50 value compared with that of DocelTM after 24
21
h incubation with A549 human lung cancer cell lines. In comparison with the DocelTM, DTX
22
loaded PLA-TPGS micelles were showed significantly higher cytotoxicity, low toxic profiles and
23
thereby improved efficacy as well as safety for lung cancer therapy.
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Page 20 of 40
1 2
Acknowledgements Author Mr. Rahul Pratap Singh acknowledges the University Grants Commission (UGC),
4
New Delhi, India, for the award of Rajiv Gandhi National Fellowship (RGNF)
5
(RGNF-2012-13-SC-UTT-18279) to his doctoral research in the year of 2012-2013.
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Declaration of interest: The authors report no declaration of interest.
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(lactide)-vitamin E TPGS nanoparticles, Biomaterials 29 (2008) 2663-2672.
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Table Captions:
Table 1. Formulae of PLA-TPGS micelles.
Singh et al: Revised submission to Int. Journal of Biological Macromolecules (26 Nov 2015) 28
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Table 2. Particle size, polydispersity, zeta potential, encapsulation efficiency and drug loading of DTX loaded polymeric micelles.
d
M
an
us
cr
ip t
Table 3. IC50 values of DTX formulated as PLA-TPGS polymeric micelles or DocelTM for human lung cancer cells (n=4).
Ac ce pt e
1 2 3 4 5 6 7 8 9 10 11 12 13 14 15 16 17 18 19 20 21 22 23 24 25 26 27 28 29 30 31 32 33 34 35 36 37 38 39 40 41 42 43 44 45 46
Figure Captions: Fig.1. Schematic diagram for (A) synthesis of (i) PLA-TPGS copolymer (B) activation of (i) TPGS (TPGS-COOH) (ii) synthesis of TPGS-Tf (C) preparation of (i) DTX-PLA-TPGS: DTX loaded polymeric micelles and (ii DTX-PLA-TPGS-Tf: DTX loaded transferrin conjugated polymeric micelles. Singh et al: Revised submission to Int. Journal of Biological Macromolecules (26 Nov 2015) 29
Page 29 of 40
Fig.2. (A) FTIR spectra of L-LA, TPGS and PLA-TPGS copolymer (B) TPGS-COOH (carboxylated TPGS) and TPGS-Tf (transferrin conjugated TPGS).
cr
ip t
Fig.3. (A) Particle size and (B) polydispersity index of placebo polymeric micelles (PLA-TPGS), DTX-PLA-TPGS: DTX loaded polymeric micelles and DTX-PLA-TPGS-Tf: DTX loaded transferrin conjugated polymeric micelles and (C) particle size distribution of DTX-PLA-TPGS: DTX loaded polymeric micelles and (D), drug encapsulation efficiency of DTX-PLA-TPGS: DTX loaded polymeric micelles and DTX-PLA-TPGS-Tf: DTX loaded transferrin conjugated polymeric micelles.
us
Fig.4. In-vitro drug release from DTX loaded preparations in PBS (pH 7.4). Bar represent ± S.D (n=3). DocelTM: commercial DTX preparation (control), DTX-PLA-TPGS: DTX loaded polymeric micelles and DTX-PLA-TPGS-Tf: DTX loaded transferrin conjugated polymeric micelles.
M
an
Fig.5. Cytotoxicity and antiproliferative profile of DTX formulated as polymeric micelles or DocelTM for human lung cancer cells (n=4). DocelTM (DTX injection), DTX-PLA-TPGS (DTX loaded polymeric micelles) and DTX-PLA-TPGS-Tf (DTX loaded transferrin conjugated polymeric micelles).
d
Fig.6. The proposed mechanisms: passive diffusion, transferrin receptor mediated endocytosis and phagocytosis of various formulations. (A) Passive diffusion of DocelTM (marketed preparation) with p-gp efflux (B) transferrin receptor mediated endocytosis for DTX-PLA-TPGS polymeric micelles, involves the formation of vesicles transferrin receptor regions of the plasma membrane. The transferrin in the cytosol are then recycled back to the plasma membrane followed by movement of ingested materials from early endosome to the late endosome, finally fusing lysosome to form the lysosome-endosome hybrid and (C) phagocytosis occurs in phagosomes for DTX-PLA-TPGS (released DTX was involved in interaction with microtubule).
Ac ce pt e
1 2 3 4 5 6 7 8 9 10 11 12 13 14 15 16 17 18 19 20 21 22 23 24 25 26 27 28 29 30 31 32 33 34 35 36 37 38 39 40 41 42 43
Fig.7. In-vivo safety study of DTX loaded TPGS polymeric micelles; (A) Alkaline phosphatase activity (KA Units); (B) LDH activity (U/L) and (C) Total protein counts (g/dl) in BAL fluid of rats. Control; Saline treatment; DocelTM: DTX injection, PLA-TPGS: Placebo polymeric micelles, DTX-PLA-TPGS: DTX loaded polymeric micelles and DTX-PLA-TPGS-Tf: DTX loaded transferrin conjugated polymeric micelles.
Table 1 Formulae of PLA-TPGS micelles. S. No. 1 2 3
Batch PLA-TPGS (Placebo) DTX-PLA-TPGS DTX-PLA-TPGS-Tf
DTX (mg) 3 3
PLA-TPGS (mg) 25 25 25
TPGS-Tf (mg) 10
Singh et al: Revised submission to Int. Journal of Biological Macromolecules (26 Nov 2015) 30
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1 PLA-TPGS: Placebo polymeric micelles
3
DTX-PLA-TPGS: DTX loaded polymeric micelles
4
DTX-PLA-TPGS-Tf: DTX loaded transferrin conjugated polymeric micelles
cr us an M d Ac ce pt e
5 6 7 8 9 10 11 12 13 14 15 16 17 18 19 20 21 22 23 24 25 26 27 28 29 30 31 32 33 34 35 36 37 38 39 40
ip t
2
Table 2 Particle size, polydispersity, zeta potential, encapsulation efficiency and drug loading of DTX loaded polymeric micelles. Batches
Particle size (nm)
Polydispersity (mean ± S.Da)
Zeta potential
Encapsulation efficiency
Drug loading
Singh et al: Revised submission to Int. Journal of Biological Macromolecules (26 Nov 2015) 31
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(mean ± S.Da) PLA-TPGS DTX-PLA-TPGS DTX-PLA-TPGS-Tf
84.09 ± 7.3 135.3 ± 6.54 184.8 ± 9.22
0.45 ± 0.04 0.40 ± 0.05 0.43 ± 0.04
(mV) (mean ± S.Da) - 12.1 ± 1.8 - 8. 64 ± 0.6 2.88 ± 0.4
71.14 ± 6.7 86.63 ± 4.2
(µg/mg) (mean ± SDa,*) 37.23 ± 3.2 39.69 ± 2.4
ip t
1
(%) (mean ± S.Da,b)
a
n=3
3
b
Drug encapsulation efficiency (%) = (amount of DTX encapsulated in the micelles/ amount of
cr
2
DTX added during micelles fabrication) x 100
us
4
* Drug loading = (weight of DTX (µg) per one mg of the drug-loaded micelles)
6
S.D: Standard deviation
7
PLA-TPGS: Placebo polymeric micelles
8
DTX-PLA-TPGS: DTX loaded polymeric micelles
9
DTX-PLA-TPGS-Tf: DTX loaded transferrin conjugated polymeric micelles
M
d Ac ce pt e
10 11 12 13 14 15 16 17 18 19 20 21 22 23 24 25 26 27 28
an
5
Table 3 IC50 values of DTX formulated as PLA-TPGS polymeric micelles or DocelTM for human lung cancer cells (n=4). Formulation TM
Docel
IC50 in µg/ml on human lung cancer cells (A549) 45.98 ± 1.70
Singh et al: Revised submission to Int. Journal of Biological Macromolecules (26 Nov 2015) 32
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5.12 ± 1.39* 0.63 ± 0.22*,a
DTX-PLA-TPGS DTX-PLA-TPGS-Tf 2
a
n=4
3
*
represents significant differences (p< 0.05) from the DocelTM
4
a
represents significant differences (p< 0.05) from the DTX-PLA-TPGS
5
ip t
1
DocelTM: (DTX injection)
7
DTX-PLA-TPGS: DTX loaded polymeric micelles
8
DTX-PLA-TPGS-Tf: DTX loaded transferrin conjugated polymeric micelles
us an
9 10 11 12 13 14
M
15
Ac ce pt e
d
16 17 18 19 20 21 22 23 24 25 26 27 28 29 30 31
A
Sn(Oct)2
(i)
+ L-LA
32 33
cr
6
TPGS
120 0C / 4 h, under N2 atmosphere
PLA-TPGS
Singh et al: Revised submission to Int. Journal of Biological Macromolecules (26 Nov 2015) 33
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Succinic Anhydride
- COOH
Transferrin - NH2
(ii)
- COOH
NHS/EDC
TPGS-Tf
(i)
+
Docetaxel
+
Ac ce pt e
(ii)
PLA-TPGS
TPGS-Tf
Non-targeted micelles
d
M
PLA-TPGS
an
C
us
TPGS-COOH
1 2
3 4 5 6 7 8 9 10 11
TPGS-COOH
ip t
DMAP / 100 0C
TPGS
cr
B
(i)
Docetaxel
Targeted micelles
Fig.1. Schematic diagram for (A) synthesis of (i) PLA-TPGS copolymer (B) activation of (i) TPGS (TPGS-COOH) (ii) synthesis of TPGS-Tf (C) preparation of (i) DTX-PLA-TPGS: DTX loaded polymeric micelles and (ii) DTX-PLA-TPGS-Tf: DTX loaded transferrin conjugated polymeric micelles.
Singh et al: Revised submission to Int. Journal of Biological Macromolecules (26 Nov 2015) 34
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A
110
TPGS-COOH TPGS-Tf
L -L A T PG S PL A -T P G S
110
90
90
80 70 60 50 40 30
80 70 60 50 40
20 10
30
0 500
100 0
1500
2000
25 00
300 0
3500
4 000
450 0
0
500
1000
1500
2500
3000
3500
4000
4500
Wavenumber (cm-1)
us
W a ven um ber (cm -1 )
d
M
an
Fig.2. (A) FTIR spectra of L-LA, TPGS and PLA-TPGS copolymer (B) TPGS-COOH (carboxylated TPGS) and TPGS-Tf (transferrin conjugated TPGS).
Ac ce pt e
1 2 3 4 5 6 7 8 9 10 11 12 13 14 15 16 17 18 19 20
2000
cr
0
ip t
Transmittance (%)
T ran sm ittan ce (% )
B
100
100
Singh et al: Revised submission to Int. Journal of Biological Macromolecules (26 Nov 2015) 35
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250
0.6
A
150
PLA-TPGS DTX-PLA-TPGS
100
DTX-PLA-TPGS-Tf
Polydispersity index
200
50
0.4 PLA-TPGS
0.3
DTX-PLA-TPGS DTX-PLA-TPGS-Tf
0.2 0.1
0
0 PLA-TPGS
DTX-PLA-TPGS
DTX-PLA-TPGS-Tf
PLA-TPGS
Formulation code
DTX-PLA-TPGS
DTX-PLA-TPGS-Tf
Formulation code
C D
100
cr
80 70 60 50 40 30 20 10
an
0
us
Drug encapsulation efficiency (%)
90
DTX-PLA-TPGS DTX-PLA-TPGS-Tf
DTX-PLA-TPGS-Tf
Formulation code
M
DTX-PLA-TPGS
d
Fig.3. (A) Particle size and (B) polydispersity index of placebo polymeric micelles (PLA-TPGS), DTX-PLA-TPGS: DTX loaded polymeric micelles and DTX-PLA-TPGS-Tf: DTX loaded transferrin conjugated polymeric micelles and (C) particle size distribution of DTX-PLA-TPGS: DTX loaded polymeric micelles and (D), drug encapsulation efficiency of DTX-PLA-TPGS: DTX loaded polymeric micelles and DTX-PLA-TPGS-Tf: DTX loaded transferrin conjugated polymeric micelles.
Ac ce pt e
1 2 3 4 5 6 7 8 9 10 11 12 13
ip t
Particle size (nm)
B
0.5
Singh et al: Revised submission to Int. Journal of Biological Macromolecules (26 Nov 2015) 36
Page 36 of 40
120
ip t
80 DocelTM
60
DTX-PLA-TPGS
DTX-PLA-TPGS-Tf
cr
40
20
0 20
30
40 50 Time (h)
60
70
80
d
M
Fig.4. In-vitro drug release from DTX loaded preparations in PBS (pH 7.4). Bar represent ± S.D (n=3). DocelTM: commercial DTX preparation (control), DTX-PLA-TPGS: DTX loaded polymeric micelles and DTX-PLA-TPGS-Tf: DTX loaded transferrin conjugated polymeric micelles.
Ac ce pt e
1 2 3 4 5 6 7 8 9 10 11 12
10
an
0
us
Drug released (%)
100
Singh et al: Revised submission to Int. Journal of Biological Macromolecules (26 Nov 2015) 37
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100 90
DocelTM DTX-PLA-TPGS DTX-PLA-TPGS-Tf
70
ip t
60 50 40 30
cr
Cell viability (%)
80
20
0 0.025
0.25
2.5
us
10 25
d
M
Fig.5. Cytotoxicity and antiproliferative profile of DTX formulated as polymeric micelles or DocelTM for human lung cancer cells (n=4). DocelTM (DTX injection), DTX-PLA-TPGS (DTX loaded polymeric micelles) and DTX-PLA-TPGS-Tf (DTX loaded transferrin conjugated polymeric micelles).
Ac ce pt e
1 2 3 4 5 6 7 8 9 10 11 12 13 14 15 16 17 18 19 20 21 22 23 24 25 26 27 28 29
an
Concentration of DTX in PLA-TPGS micelles (µg/ml)
Singh et al: Revised submission to Int. Journal of Biological Macromolecules (26 Nov 2015) 38
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A
B
Transferrin
Passive diffusion DocelTM
Transferrin receptor mediated endocytosis DTX-PLA-TPGS-Tf Transferrin receptor
C Phagocytosis DTX-PLA-TPGS
cr
Phagosome
P-gp excretion without inhibition Early endosome
us
Late endosome
ip t
Receptor recycling
Free TPGS
an
Inhibit P-gp
d
Fig.6. The proposed mechanisms: passive diffusion, transferrin receptor mediated endocytosis and phagocytosis of various formulations. (A) Passive diffusion of DocelTM (marketed preparation) with p-gp efflux (B) transferrin receptor mediated endocytosis for DTX-PLA-TPGS polymeric micelles, involves the formation of vesicles transferrin receptor regions of the plasma membrane. The transferrin in the cytosol are then recycled back to the plasma membrane followed by movement of ingested materials from early endosome to the late endosome, finally fusing lysosome to form the lysosome-endosome hybrid and (C) phagocytosis occurs in phagosomes for DTX-PLA-TPGS (released DTX was involved in interaction with microtubule).
Ac ce pt e
1 2 3 4 5 6 7 8 9 10 11 12 13 14 15
M
Stabilized microtubule
Singh et al: Revised submission to Int. Journal of Biological Macromolecules (26 Nov 2015) 39
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Contol
A
DocelTM
16 )s it n U14 A K ( yt 12 i ivt c 10 A se ta a 8 h p s o h 6 P e in l 4 a lk A 2
PLA-TPGS DTX-PLA-TPGS
ip t
DTX-PLA-TPGS-Tf
0 15 days
B
C
Contol DocelTM
700
12
DTX-PLA-TPGS
600
DTX-PLA-TPGS-Tf
l) /d 8 g( ts n u o C 6 n eit or lP 4 ta o T
500 400 300 200
DocelTM PLA-TPGS DTX-PLA-TPGS
2
100 0 15 days
30 days
M
0
7 days
7 days
15 days
30 days
d
Fig.7. In-vivo safety study of DTX loaded polymeric micelles; (A) Alkaline phosphatase activity (KA Units); (B) LDH activity (U/L) and (C) Total protein counts (g/dl) in BAL fluid of rats. Control; Saline treatment; DocelTM: DTX injection, PLA-TPGS: Placebo polymeric micelles, DTX-PLA-TPGS: DTX loaded polymeric micelles and DTX-PLA-TPGS-Tf: DTX loaded transferrin conjugated polymeric micelles.
Ac ce pt e
1 2 3 4 5 6 7 8 9 10
10
us
PLA-TPGS
Contol
an
) /L U ( yt i ivt c A sea n e g or d y h e D et tac a L
30 days
cr
7 days
Singh et al: Revised submission to Int. Journal of Biological Macromolecules (26 Nov 2015) 40
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S0141-8130(15)30177-X http://dx.doi.org/doi:10.1016/j.ijbiomac.2015.11.081 BIOMAC 5586
To appear in:
International Journal of Biological Macromolecules
Received date: Revised date: Accepted date:
17-10-2015 26-11-2015 27-11-2015
Please cite this article as: R.P. Singh, G. Sharma, P. Agrawal, B.L. Pandey, B. Koch, M.S. Muthu, Transferrin receptor targeted PLA-TPGS micellesimproved efficacy and safety in docetaxel delivery, International Journal of Biological Macromolecules (2015), http://dx.doi.org/10.1016/j.ijbiomac.2015.11.081 This is a PDF file of an unedited manuscript that has been accepted for publication. As a service to our customers we are providing this early version of the manuscript. The manuscript will undergo copyediting, typesetting, and review of the resulting proof before it is published in its final form. Please note that during the production process errors may be discovered which could affect the content, and all legal disclaimers that apply to the journal pertain.
1
Transferrin receptor targeted PLA-TPGS micelles
2
improved efficacy and safety in docetaxel delivery
3
Rahul Pratap Singha, Gunjan Sharmac,
5
Sonalia, Poornima Agrawala, Bajarangprasad L. Pandeya,
6
Biplob Kochc, Madaswamy S. Muthua, b*
cr
a
us
Department of Pharmacology, Institute of Medical Sciences, Banaras Hindu University, Varanasi 221005, U.P., India
b
an
Department of Pharmaceutics, Indian Institute of Technology, Banaras Hindu University, Varanasi – 221005, India
c
d
M
Department of Zoology, Faculty of Science, Banaras Hindu University, Varanasi 221005, U.P., India
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_______________________________________ *
Corresponding author: Department of Pharmacology, Institute of Medical Sciences, Banaras Hindu University, Varanasi – 221005, India Tel.: +91 9235195928; Fax: +91 542 2367568; E-mail: [email protected] (Madaswamy S. Muthu).
Singh et al: Revised submission to Int. Journal of Biological Macromolecules (26 Nov 2015) 1
Page 1 of 40
ABSTRACT
2
The aim of this work was to develop targeted polymeric micelles of poly-lactic acid-D-
3
α-tocopheryl polyethylene glycol 1000 succinate (PLA-TPGS), which are assembled along with
4
D-alpha-tocopheryl polyethylene glycol 1000 succinate-transferrin conjugate (TPGS-Tf), and
5
loaded docetaxel (DTX) as a model drug for enhanced treatment of lung cancer in comparison to
6
non-targeted and DTX injection (DocelTM). A549 human lung cancer cells were employed as an
7
in-vitro model to access cytotoxicity study of the DTX loaded polymeric micelles. The safety of
8
DTX formulations were studied by the measurement of alkaline phosphatase (ALP), lactate
9
dehydrogenase (LDH) and total protein levels in bronchoalveolar lavage (BAL) fluid of rats after
10
the treatments. The IC50 values demonstrated that the non-targeted and transferrin receptor
11
targeted polymeric micelles could be 7 and 70 folds more effective than DocelTM after 24 h
12
treatment with the A549 cells. Results suggested that transferrin receptor targeted polymeric
13
micelles have showed better efficacy and safety than the non-targeted polymeric micelles and
14
DocelTM.
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Key words: Cytotoxicity, Lung cancer, Nanomedicine, Nanotechnology, Polymeric micelles,
17
Safety, Transferrin conjugation
18 19 20 21 22 23 24 25
1. Introduction Lung cancer is one of the top most deaths causing disease in the world in both sexes (men Singh et al: Revised submission to Int. Journal of Biological Macromolecules (26 Nov 2015) 2
Page 2 of 40
and women). Based on lethality, the lung cancer is further categorized in two major classes
2
including small cell lung cancer (13%) or non-small cell lung cancer (83%) for the purposes of
3
treatment. The 1 and 5 year relative survival rates for lung cancer are 44% and 17%, respectively.
4
The lung cancer treatment includes surgery, radiation therapy, chemotherapy, and/or targeted
5
therapies. The lung cancer patients are usually treated by chemotherapy and targeted drugs [1].
6
Presently, various receptor targeted drug delivery systems have showed the possibilities to provide
7
effective treatments to cancer cells which may minimize the adverse effects of drugs to the healthy
8
cells [2].
us
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1
The nanomedicine is the application of nanotechnology to medicine, which is highly
10
capable to develop nanoparticles drug delivery system [3]. These nano drug deliveries are enable
11
to target cancer cells in highly effective manner by enhanced permeability and retention (EPR)
12
effects, which is an important feature to make cancer targeting drug delivery system [4-10]. The
13
several
14
(D,L-lactide-co-glycolide) (PLGA) nanoparticles, carbon nanotubes and polymeric micelles
15
[11-22]. Among these, polymeric micelles are drug delivery systems, which are widely applied in
16
the lipophilic or poorly soluble drugs [17,23-25].
M
an
9
systems
have
been
d
delivery
developed
such
as
liposomes,
poly
Ac ce pt e
drug
17
The polymeric micelles are formed through the multimolecular assembly of block
18
copolymers as novel core-shell typed nano carriers for drug targeting [26,27]. The polymeric
19
micelles outer corona made up by using the hydrophilic polymer segments, which act as a
20
stabilizing interface between the hydrophobic drug and the external medium and maintains the
21
aqueous solubility of polymeric micelles [28-30].
22
Polymeric micelles are emerging polymeric nano carriers, which act as a highly integrated
23
nanoplatform for cancer targeting (passive as well as active targeting), drug delivery and tumor
Singh et al: Revised submission to Int. Journal of Biological Macromolecules (26 Nov 2015) 3
Page 3 of 40
imaging applications [31-33]. It have several extraordinary properties including biocompatibility,
2
high stability in both in-vitro and in-vivo, and also have capacity to effectively solubilize a variety
3
of poorly soluble drugs, changing the release profile of the incorporated pharmaceutical agents,
4
and the ability to accumulate in the target zone based on the EPR effects [34-35]. These polymeric
5
micelles can be used as targeted drug delivery systems in lung cancer treatment [17, 36]. Also, it
6
can be conjugated with different biomolecules including targeting ligand, antibody,
7
P-glycoprotein (P-gp) inhibitor and diagnostic agents, which are highly beneficial to multiple drug
8
resistance (MDR) types of lung cancer treatment [37-39]. Also, polymeric micelles are highly
9
effective to increase EPR effect in cancer treatment. The polymeric micelles are frequently using
10
in the several cancer treatment including glioma, renal, stomach, lung, and pancreatic cancer at
11
phase I and phase II clinical trials. [28, 40, 41].
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Poly-lactic acid (PLA) is a biodegradable and biocompatible polymer, which is widely
13
using in the biomedical for making safe and biodegradable nano carriers for cancer treatment. The
14
United States Food and Drug Administration (US FDA) has approved their uses in drug delivery
15
systems. The monomer of PLA i.e., L-lactic acid (L-LA), which can be efficiently produced by
16
fermentation from renewable resources such as starchy materials and sugars. The PLA degrades to
17
its monomer, L-LA, which is a normal metabolite of the human [13]. D-α-tocopheryl polyethylene
18
glycol 1000 succinate (TPGS) mostly studied in liposomes and polymeric nanoparticles which
19
enhanced cellular uptake, cytotoxicity and showed prolonged circulation time [14,15]. TPGS is
20
simply known as vitamin E, which is provides better permeation effects of hydrophilic and
21
hydrophobic drug molecules. It is FDA approved water-soluble derivative of natural Vitamin E
22
(PEGylated vitamin E). TPGS is a derivative of the natural vitamin E (alpha-tocopherol) and
23
polyethylene glycol 1000. It is also non-ionic and highly hydrophilic, is used as solubilizer,
Ac ce pt e
d
12
Singh et al: Revised submission to Int. Journal of Biological Macromolecules (26 Nov 2015) 4
Page 4 of 40
absorption enhancer and a vehicle for various formulations [13,15,22]. PLA-TPGS is a block
2
copolymer of L-LA and TPGS. The PLA-TPGS block-copolymer was prepared by using ring
3
opening polymerization method. It has been used in the fabrication of nano drug delivery systems
4
because of its safety, stealth effect, targeting feasibility, multifunctional capability,
5
biocompatibility, size tunability and ease of preparation of nanoparticles. In recent study, de
6
Melo-Diogo et al., has prepared a highly effective drug delivery of triple multiple drugs
7
(crizotinib–palbociclib–sildenafil) loaded PLA-TPGS micelles and improved lung cancer
8
treatment
9
(Crizotinib–Palbociclib) loaded micelles treatment [17]. The polymeric micelles of PLA-TPGS
10
can be prepared at the critical micelles concentration (CMC) of 0.016 mg/mL [17]. Further,
11
targeting can be achieved via the EPR into the areas with the compromised vasculature and by
12
attaching specific targeting ligand molecules to the micelle surface [13, 42-44].
A549
cells
in
comparison
to
single
(Crizotinib)
and
dual
drug
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In this study, docetaxel (DTX) was used as anticancer model drug for the lung cancer
14
treatment. DTX (N-debenzoyl-N-tertbutoxycarbonyl-10-deacetyl-paclitaxel) is a semisynthetic
15
derivative of the taxoid family of antineoplastic agents. It is an analog of paclitaxel, which is
16
extracted from the needles of the European yew tree (Taxus baccata L). DTX has been found to be
17
more effective than paclitaxel against breast, ovarian, lung, brain and neck cancers [15, 16]. To
18
overcome the poor solubility of DTX and to reduce the systemic toxicity, conventional and various
19
novel formulations have been developed [20, 22, 45]. However, there is a problem that needs to be
20
solved to meet the requirements for its clinical use i.e., targeted delivery of DTX to cancer cells.
Ac ce pt e
d
13
21
Transferrin receptor is a cell membrane-associated glycoprotein on the surface of the cells. It
22
plays an important role in iron homeostasis and the regulation of cell growth in cells. The
23
transferrin receptor expression on cancer cells can be up to 100-fold higher than the average
Singh et al: Revised submission to Int. Journal of Biological Macromolecules (26 Nov 2015) 5
Page 5 of 40
expression in normal cells owing to their rapid proliferation rate and iron demand, thereby
2
transferrin has been explored as a targeting ligand for nanocarriers to deliver therapeutic and
3
diagnostic agent into cancer cells [46,47]. This approach shows the advantage of continuous
4
recycling of the transferrin receptor from the surface to the endosomal compartment to make it
5
efficient route for the internalization of nanoplatforms [20]. In one study, it was reported that
6
among the primary lung cancer cases, 19% of adenocarcinomas showed positive results for
7
transferrin receptor overexpression which showed the possibility of transferrin receptor targeted
8
delivery of micelles for lung cancer therapy [48].
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1
In this study, PLA-TPGS (block copolymer of L-LA and TPGS) was used to make polymeric
10
micelles. DTX was loaded into polymeric micelles by using solvent displacement method.
11
Transferrin was conjugated to activated TPGS-COOH, which serve as targeting agent to transport
12
DTX into the human lung cancer cells (A549). The targeting effects of transferrin conjugated
13
polymeric micelles (targeted) were compared closely with non-targeted polymeric micelles and
14
clinical DocelTM (DTX injection). In-vitro cytotoxicity of A549 cells was assessed and the IC50
15
value at 24 h was assessed to evaluate the therapeutic effect of the DTX loaded PLA-TPGS
16
polymeric micelles with or without targeting function. Further, PLA-TPGS micelles were tested
17
in-vivo on rats model for safety applications i.e., alkaline phosphatase (ALP), lactate
18
dehydrogenase (LDH), and total protein levels in bronchoalveolar lavage (BAL) fluid of lung
19
tissue after intravenous (i.v.) administrations.
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2. Materials and methods
22
2.1. Materials
23
Docetaxel (DTX) of purity 99.56% was obtained from Neon Laboratories Ltd, Mumbai, India
Singh et al: Revised submission to Int. Journal of Biological Macromolecules (26 Nov 2015) 6
Page 6 of 40
as gift sample. D-alpha-tocopheryl polyethylene glycol 1000 succinate (TPGS) was obtained from
2
Antares Health Products., St. Charles, U.S.A. as gift sample. Dialysis membrane (Spectra/Por7®)
3
of 1 KDa molecular weight cut off was purchased from Spectrum Laboratories Inc., Rancho
4
Dominguez, CA, U.S.A. Clinical formulation DocelTM was purchased from RPG Life Sciences
5
Limited, Mumbai, India. L-Lactide (L-LA) monomer (3,6-Dimethyl-1,4-dioxane-2,5-dione),
6
stannous octoate (Sn(Oct)2), transferrin (Molecular weight of 80 kDa), ethanol and phosphate
7
buffer saline (PBS) were purchased from Sigma–Aldrich, St. Louis, MO, USA. Anhydrous
8
toluene, dichloromethane and methanol were purchased from Loba Chemie Pvt. Ltd, New Delhi,
9
India. Human lung cancer cell lines (A549) were provided by National Centre for Cell Science,
10
Pune, India. Dulbecco's Modified Eagle’s Medium (DMEM), fetal bovine serum (FBS),
11
streptomycin, penicillin, L-glutamine and trypsin-EDTA were purchased from Genetix Biotech
12
Asia Pvt. Ltd., Mumbai, India. T-25 culture flask and 96-well culture plates purchased from
13
Tarsons
14
5-diphenyltetrazoliumbromide (MTT) were purchased from Himedia Laboratories, Mumbai,
15
India. All other chemicals were of analytical grade.
16
2.2. Methods
17
2.2.1. Synthesis of PLA-TPGS copolymer
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Ltd.,
Kolkata,
d
Pvt.
India.
3-(4,
5-dimethylthiazolyl-2-yl)-2,
Ac ce pt e
Products
18
The PLA-TPGS copolymer was synthesized by ring opening polymerization (ROP) of
19
L-LA with TPGS in the presence of stannous octoate [Sn(Oct)2] as catalyst. Briefly, L-LA and
20
TPGS (1:1 ratio) were added to a round bottom flask (RBF). The system was purged with nitrogen
21
and anhydrous toluene (25 mL per gram of L-LA) was added. Subsequently Sn(Oct)2 (0.5% w/v)
22
was added and the ROP reaction was carried out at 120 0C for 4 h, under nitrogen (N2) atmosphere.
23
At the end of polymerization, the toluene was evaporated by using rotary evaporator (Buchi R-210
Singh et al: Revised submission to Int. Journal of Biological Macromolecules (26 Nov 2015) 7
Page 7 of 40
Advanced, Switzerland) at 37 0C and the resulting product was dissolved in dichloromethane
2
(DCM) and precipitated in cold methanol. The recovered precipitate was dialyzed for 2 days
3
against acetone and 3 days against distilled water. Finally, the diblock copolymer was lyophilized
4
and a white powder was obtained [11,17,41,47,49]. The schematic diagram of PLA-TPGS
5
copolymer synthesis resents in Fig. 1A.
6
2.2.2. Synthesis of TPGS-COOH (activation of TPGS) and its conjugate
cr
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For the synthesis of TPGS and transferrin conjugate, TPGS was first activated (i.e.,
8
TPGS-COOH) by succinic anhydride through ring-opening reaction in the presence of DMAP
9
[20]. In brief, TPGS (0.77 g, 0.5 mM), succinic anhydride (0.10 g, 1 mM) and DMAP (0.12 g, 1
10
mM) were mixed and heated at 100 0C under nitrogen atmosphere for 24 h. The mixture was
11
cooled to room temperature, dissolved in 5 ml of cold dichloromethane, filtered to remove
12
excessive succinic anhydride and then precipitated in 100 ml of diethyl ether at -10 0C overnight.
13
The white TPGS-COOH precipitate was filtered and dried in vacuum [19,20,22]. The schematic
14
diagram of synthesis of TPGS-COOH (activation of TPGS) resents in Fig. 1B (i).
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Further, TPGS-COOH carboxyl group was conjugated to the transferrin by carbodiimide
16
chemistry with the help of EDC and NHS in phosphate buffer saline (pH 5.5) [20]. In brief, for
17
conjugation of transferrin to TPGS-COOH, 1-ethyl-3-(3- dimethylaminopropyl) carbodiimide
18
(EDC) and N-hydroxysuccinimide (NHS) (both are catalyst) were added into TPGS-COOH with a
19
molar ratio of 1:5 (TPGS-COOH : EDC or NHS) in phosphate buffer saline (pH 5.5). In brief,
20
TPGS-COOH (200 mg), EDC (96 mg) and NHS (74 mg) were mixed in 2 ml of phosphate buffer
21
saline (pH 5.5) at 25 0C for 5 h, stored in a refrigerator at 4 0C over 24 h, mixed with 1 ml of 0.2 %
22
(w/v) transferrin and stirred at 4 0C over 8 h. The resulted product was then dialyzed using a
23
dialyzing membrane (MWCO: 12 kDa) against phosphate buffer saline (pH 5.5) for 48 h in order
Singh et al: Revised submission to Int. Journal of Biological Macromolecules (26 Nov 2015) 8
Page 8 of 40
to remove excess TPGS-COOH, NHS and EDC. The dialyzed product (i.e., TPGS-Tf) was freeze
2
dried and used for micelle formation [20,22]. The schematic diagram of synthesis of TPGS-Tf
3
resents in Fig. 1B (ii).
4
2.2.3. Preparation of PLA-TPGS polymeric micelles using solvent displacement (SD) method
ip t
1
Briefly, for DTX loaded polymeric micelles formulation, 3 mg DTX and 25 mg
6
PLA-TPGS copolymer were dissolved in 5 ml of DCM/methanol (1:1 v/v). After that, the solvent
7
was evaporated by using rotary evaporator (Buchi R-210 Advanced, Switzerland) at 37 0C and
8
then film was hydrated with 10 ml of 1mM phosphate buffer saline (PBS), pH 7.4. After that the
9
mixture was incubated in an orbital water bath shaker at 37 0C for 48 h. The excess
10
non-incorporated DTX was separated by filtration (using a 0.22-µm filter) before characterization.
11
The targeted polymeric micelles were prepared with the addition of 10 mg of TPGS-Tf at 4 0C to
12
obtain higher drug encapsulation, drug controlled release and drug targeting effects on cancer cell
13
lines (Table 1). For the preparation of placebo polymeric micelles, the formulation process used
14
was the same as previously described but without the inclusion of DTX [16,17]. The schematic
15
diagram of preparation of non-targeted and targeted polymeric micelles resents in Fig. 1C (i) and
16
(ii), respectively.
17
2.2.4. Fourier transform infrared (FTIR) spectroscopy
Ac ce pt e
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18
The FTIR spectroscopy for L-LA, TPGS, PLA-TPGS copolymer, TPGS-COOH and
19
TPGS-Tf were performed using compressed KBr pellet method in Perkin Elmer FTIR
20
spectrophotometer (Perkin Elmer Spectrum Two, Waltham, Massachusetts, U.S.A). The scanning
21
range was 400-4000 cm-1.
22
2.2.5. Particle size, polydispersity and zeta potential of polymeric micelles
23
Size, polydispersity and zeta potential of the PLA-TPGS (placebo micelles),
Singh et al: Revised submission to Int. Journal of Biological Macromolecules (26 Nov 2015) 9
Page 9 of 40
1
DTX-PLA-TPGS (non-targeted micelles) and DTX-PLA-TPGS-Tf (targeted micelles) were
2
measured by PCS using a Zetasizer ver. 7.03, Malvern instruments Ltd, Malvern, UK [16].
3
2.2.6. Determination of encapsulation efficiency and drug loading of polymeric micelles The DTX encapsulation efficiency of non-targeted and targeted polymeric micelles were
5
determined by UV spectrophotometer (Shimadzu 1800, Tokyo, Japan). Briefly, 2 ml aliquots of
6
polymeric micelles were evaporated to dryness by rotary evaporator under reduced pressure at 35
7
0
8
h at 37 0C to fully leach out the DTX. Then, the solution was centrifuged at 10,000 rpm for 10 min
9
at 4 0C, and the supernatant was collected. The supernatant (500 µl) was further diluted to 2 ml of
10
methanol. Then light absorption was measured at 229 nm using spectrophotometer. The drug
11
encapsulation efficiency was defined as the ratio between the amount of DTX encapsulated in the
12
polymeric micelles and that added in the polymeric micelles preparation process. The drug loading
13
was calculated as the weight of drug (µg) per one mg of the drug-loaded polymeric micelles
14
[20,22]. All samples were done in triplicate.
15
2.2.7. In-vitro drug release studies
cr
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Ac ce pt e
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C. The residue was dissolved in 20 ml of methanol. Then it was gently shaken on a shaker for 24
16
The release patterns of DTX from DTX-PLA-TPGS and DTX-PLA-TPGS-Tf were studied
17
by using dialysis bag diffusion technique [15,22]. The formulation of a volume equivalent to 300
18
µg of DTX were placed in the dialysis bag (cellulose membrane, molecular weight cut off 1 kDa),
19
hermetically sealed and immersed into 100 ml of PBS (pH 7.4). The entire system as kept at 37 ±
20
0.5 0C with continuous shaking at 100 rpm/min. Then, 5 ml samples were withdrawn from the
21
receptor compartment at predetermined time intervals and replaced by fresh medium. The samples
22
were filtered through 0.45 mm syringe filter before analysis. The DTX content in the samples was
23
determined by using UV spectrophotometer (Shimadzu 1800, Tokyo, Japan). Then drug release
Singh et al: Revised submission to Int. Journal of Biological Macromolecules (26 Nov 2015) 10
Page 10 of 40
1
profiles were calculated [20, 50].
2
2.2.8. Cell culture A549 human lung cancer cell lines were grown in DMEM supplemented with 10% FBS,
4
100 units/mL penicillin and 100 µg/mL streptomycin solutions. The cell lines were grown at 37 °C
5
in the presence of 5% CO2.
6
2.2.9. Cytotoxicity of PLA-TPGS polymeric micelles
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The cytotoxicity of DTX formulations i.e., DTX-PLA-TPGS, DTX-PLA-TPGS-Tf and
8
DocelTM (DTX injection) were performed on A549 human lung cancer cell lines by standard MTT
9
assay. A549 cell lines were seeded into 96 well culture plates (Tarsons Products Pvt. Ltd.) at the
10
density of 1×104 viable cells/well with DMEM and incubated at least overnight to allow cell
11
attachment. The spent medium was discarded and the cells were incubated with both
12
DTX-PLA-TPGS and DTX-PLA-TPGS-Tf, and their cytotoxicity was assessed in comparison
13
with DocelTM at 0.025, 0.25, 2.5 and 25 µg/ml equivalent drug concentrations for 24 h. After 24 h,
14
medium was removed and 100 µL medium and 10 µL of 5 mg/mL MTT in PBS, pH 7.4 was added
15
to each well of the plate. The plates were further incubated for 2 h at 37 0C in the incubator. Then
16
the medium and MTT were removed and 100 µL of DMSO was added to dissolve the MTT
17
formazan crystals. The absorbance of samples was measured at 570 nm by microplate reader [23].
18
Cytotoxicity was calculated as the percentage of treated cells relative to untreated cells at 570 nm.
19
The percent of the cell viability was calculated using the equation:
21
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Cell viability (%) = Absorbance of treated cells/Absorbance of control cells) X 100 2.2.10. In-vivo safety using bronchoalveolar lavage (BAL) fluids of rats
22
The animal caring, handling, husbandry and the protocols were approved by the Institute of
23
Medical Sciences (IMS), Banaras Hindu University (BHU), Varanasi, India. Both sexes (male and
Singh et al: Revised submission to Int. Journal of Biological Macromolecules (26 Nov 2015) 11
Page 11 of 40
female) rats of 150-200 gm (or 4–5 weeks old) were supplied by the Central Animal House of
2
IMS, BHU and maintained at animal room of the Department of Pharmacology of IMS, BHU,
3
Varanasi, India. The animals were acclimatized at a temperature of 25 ± 2 0C and a relative
4
humidity of 50–60% under natural light/dark conditions and given aseptic full-price nutritional
5
pellet feed and sterile water available ad libitum for 4–5 days before experiments. The study
6
protocol was follow guideline of Committee for the Purpose of Control and Supervision on
7
Experiments on Animals (CPCSEA; Guidelines for Laboratory Animal Facility) Registration No.
8
Dean/2015/CAEC/1262 of Banaras Hindu University, Varanasi (U.P.), India.
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The animals were randomly divided into 5 (4 treatment groups + 1 control group) groups
10
with approximately 4 rats per group (n=4). One week after the initiation of acclimatization, all rats
11
(except control animal) were treated with plain PLA-TPGS (placebo micelles), DTX-PLA-TPGS
12
(5 mg/kg of DTX), DTX-PLA-TPGS-Tf (5 mg/kg of DTX) and DocelTM (5 mg/kg of DTX) and
13
one control group was treated with normal saline (0.9% NaCl) solution via the i.v. route. Drinking
14
water was available ad libitum. During the treatment, the health conditions of rats were monitored
15
every day. At the indicated time of interval 7, 15 and 30 days of polymeric micelles and DocelTM
16
formulation administrations. The rats were sacrificed with an intraperitoneal (i.p.) injection of
17
urethane (1.5 g/kg rats). The thorax was opened and the lung perfused with normal saline solution
18
(26.5 ml/kg rats). Further trachea was then cannulated and BAL fluid was performed by injecting
19
approximately 4 mL of normal saline solution and thorough rinsing of the lung. The BAL fluid
20
was recovered and centrifuged at 400×g at 4 0C for 10 min and then stored at -20 0C until analysis
21
[50]. All biochemical assays were performed on BAL fluids such as estimation of ALP (Span
22
Diagnostics Ltd., Surat, India), LDH and total protein count (Crest Biosystems, Goa, India) by
23
using respective diagnostic kits according to the manufacturer’s instructions. ALP activity is a
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Singh et al: Revised submission to Int. Journal of Biological Macromolecules (26 Nov 2015) 12
Page 12 of 40
measure of type II alveolar epithelial cell secretory activity, and increased ALP activity in BAL
2
fluids is considered to be an indicator of type II cell toxicity. LDH is a cytoplasmic enzyme and is
3
used as an indicator of cell injury. Increases in BAL fluid protein concentrations generally were
4
consistent with enhanced permeability of vascular proteins into alveolar regions [51, 52].
5
2.2.11. Statistical analysis
ip t
1
Results are given as mean ± standard deviation (S.D). Mean values of particle size,
7
encapsulation efficiency, in-vitro and in-vivo data were compared using the Student’s t-test.
8
Differences are considered significant at a level of P<0.05.
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3. Results and discussions
11
3.1. Preparation of different block-copolymer, TPGS-Tf and polymeric micelles
M
10
Fig. 1A shows the schematic production of PLA-TPGS block-copolymer, that was
13
prepared by using ring opening polymerization method in presence of stannous octoate (Sn(oct)2)
14
as catalyst in the reaction under nitrogen gas environment at 120 0C for 4 h [17,48]. In the
15
polymerization reaction hydroxyl terminus (-OH) of TPGS was used as initiator. Further, this
16
amphiphilic copolymer of PLA-TPGS was used to prepared polymeric micelles. Fig. 1B (i) shows
17
the activation TPGS in to TPGS-COOH in the presence of succinic anhydride and DMAP at 100
18
0
19
attached to the activated TPGS (TPGS-COOH) by carbodiimide chemistry with the help of EDC
20
and NHS in phosphate buffer saline (pH 5.5) [20]. Fig. 1C (i and ii) clearly shows the preparation
21
DTX loaded polymeric micelles. The DTX was loaded using solvent displacement (SD) method.
Ac ce pt e
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C under nitrogen atmosphere for 24 h [22]. Fig. 1B (ii) shows that transferrin was covalently
22 23
Table 1 (approximate position)
Singh et al: Revised submission to Int. Journal of Biological Macromolecules (26 Nov 2015) 13
Page 13 of 40
1
Fig. 1 (approximate position)
2 3
3.2. Characterization of L-LA, TPGS, PLA-TPGS, TPGS-COOH and TPGS-Tf by FTIR Fig.2A shows the FTIR spectra of L-LA, TPGS and PLA-TPGS, which is clearly revealed
5
the successful polymerization of L-LA and TPGS in to PLA-TPGS block-copolymer. In the
6
spectra, the C-H stretching is clearly appearing, which is due to methyl group vibrations from
7
L-LA (2925.55 cm-1), TPGS (2870.67 cm-1) and PLA-TPGS (2926.62 cm-1). The carbonyl
8
vibration peak was also present in all the spectra. The carbonyl band shift from TPGS to the
9
synthesized diblock-copolymer (PLA-TPGS) was also visible (TPGS: 1737.75 cm-1; PLA-TPGS:
10
1755.73 cm-1; L-LA: 1766.55 cm-1). Another important peak for -C-C- stretching is aromatic ring
11
was appeared in both TPGS and PLA-TPGS copolymer peak at 1465.06 and 1455.21 cm-1,
12
respectively. The peak at 1382.4 cm-1for -CH2 group of PEG chain was observed in PLA-TPGS
13
copolymer. In TPGS and PLA-TPGS FTIR spectra, the C-O stretch band is also present at peak
14
951.46 and 1252.4 cm-1, respectively. Finally at peak 3425.51 cm-1 band is assigned to the terminal
15
hydroxyl group of the PLA chain.
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16
Fig.2B shows FTIR spectra of TPGS-COOH and TPGS-Tf. In FTIR spectra of
17
TPGS-COOH, the –C=O stretching was clearly appeared peaks at 1736.47 cm-1, which is clearly
18
indicating a successful synthesis of TPGS-COOH. In transferrin conjugated TPGS, the linkage
19
between -COOH group of TPGS and -NH2 group of transferrin was confirmed by the amide
20
(-CO-NH-) stretching peak at 1634.02 cm-1. In both TPGS and TPGS-COOH, the absorption
21
bands at 3450.04 and 3452.3 cm-1 were due to the terminal hydroxyl group.
22 23
Figure 2 (approximate position)
Singh et al: Revised submission to Int. Journal of Biological Macromolecules (26 Nov 2015) 14
Page 14 of 40
1 2
3.3. Particle size, polydispersity and zeta potential of polymeric micelles The mean particle size and polydispersity of PLA-TPGS (placebo micelles),
4
DTX-PLA-TPGS and DTX-PLA-TPGS-Tf were listed in Table 2. PCS measurements were
5
undertaken in multimodal analysis to get a true reflection of particle size distribution. The particle
6
size distribution curves for all the samples were unimodal. The mean sizes of PLA-TPGS,
7
DTX-PLA-TPGS, and DTX-PLA-TPGS-Tf were 84.09 ± 7.3, 135 ± 6.5 and 184 ± 9.92 nm,
8
respectively (Fig.3A to C). The PLA-TPGS polymeric micelles were observed in very small size,
9
which are suitable for therapeutic application in cancer treatment [14,16]. The particle size results
10
indicate that incorporation of DTX and targeting ligand (transferrin) conjugation on the surface of
11
targeted polymeric micelles (DTX-PLA-TPGS-Tf) leads to significant (P < 0.05) increase in the
12
size in comparison to DTX-PLA-TPGS and PLA-TPGS. The size of non-targeted and targeted
13
polymeric micelles were bigger that the placebo polymeric micelles. This results may be due the
14
packaged micelles contained the more hydrophobic drugs in their cores, thus increasing the
15
diameter of the micelles in aggregation. It was reported that polymeric micelles size typically in
16
the range of ˂200 nm are suitable for drug delivery in cancer therapy. The polydispersity of all the
17
batches of polymeric micelles showed quite narrow size distribution, which is nearer to 0.5
18
(Fig.3B). The zeta potential of all the polymeric micelles were found to be negatively charged
19
except for the transferrin conjugated polymeric micelles (Table 2). The negative zeta potential of
20
plain was found to be higher than that of DTX loaded polymeric micelles owing to the better
21
packing of -OH on the surface of polymeric micelles. Also the raise in positive charge on the
22
transferrin conjugated polymeric micelles was due to the presence of amino ends on the surface
23
[20].
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Singh et al: Revised submission to Int. Journal of Biological Macromolecules (26 Nov 2015) 15
Page 15 of 40
1
3.4. Determination of encapsulation efficiency and drug loading of polymeric micelles Drug encapsulation efficiency was calculated as the percentage ratio between amount of
3
drug loaded in polymeric micelles and amount of the drug added during fabrication of polymeric
4
micelles [28,41,45]. Fig.3D shows the drug encapsulation efficiency of the DTX-PLA-TPGS and
5
DTX-PLA-TPGS-Tf were 71.14 ± 6.7 and 86.63 ± 4.2%, respectively (Table 2). The targeted
6
polymeric micelles (DTX-PLA-TPGS-Tf) showed significant increase (P<0.05) in the drug
7
encapsulation in comparison to non-targeted polymeric micelles (DTX-PLA-TPGS). This may be
8
because of the influence of TPGS-Tf conjugate to surface of polymeric micelles that leads to
9
enhance drug encapsulation efficiency. Drug loading is defined as the weight of drug (µg) per mg
10
of the drug loaded polymeric micelles. The drug loading of the non-targeted polymeric micelles
11
(DTX-PLA-TPGS) was 37.23±3.2 µg/mg. The drug loading of the targeted (DTX-PLA-TPGS-Tf)
12
polymeric micelles was 39.69 ± 2.4 µg/mg (Table 2). As mentioned earlier, addition of TPGS-Tf
13
into the micelle formation might lead to slight increase (P < 0.05) in drug loading and drug
14
encapsulation efficiency for DTX-PLA-TPGS-Tf comparison to DTX-PLA-TPGS.
16 17 18 19
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Table 2 (approximate position)
Figure 3 (approximate position)
3.5. In-vitro drug release studies
20
Fig. 4 shows the accumulated percentage release of DTX from polymeric micelles and
21
DocelTM in the medium of PBS (pH 7.4) under sink condition. The DTX-PLA-TPGS and
22
DTX-PLA-TPGS-Tf showed a sustained release for 72 h without any burst release in comparison
23
to DocelTM. After 72 h of dialysis in PBS (pH 7.4), the percentage of DTX released from the
Singh et al: Revised submission to Int. Journal of Biological Macromolecules (26 Nov 2015) 16
Page 16 of 40
preparations were 90.35, 66.72 and 58.23% for the DocelTM, DTX-PLA-TPGS, and
2
DTX-PLA-TPGS-Tf, respectively. The DTX-PLA-TPGS showed sustained drug release effects
3
due to a strong interaction between the DTX and polymeric micelles in comparison to DocelTM.
4
There was a significant (P<0.05) decrease in the in vitro drug release from the
5
DTX-PLA-TPGS-Tf comparison to the DTX-PLA-TPGS and DocelTM. These results may be
6
explained by the influence of transferrin on the micelles surface which was included as TPGS-Tf.
7
The t50% in PBS (pH 7.4) for DocelTM, polymeric micelles of DTX-PLA-TPGS and
8
DTX-PLA-TPGS-Tf containing DTX were about 16, 44 and 58 h, respectively. The DocelTM did
9
not show sustain the drug release. There was a significant (P<0.05) decrease in the t50% of the
10
DTX-PLA-TPGS, and DTX-PLA-TPGS-Tf in comparison with the DocelTM. It may be because of
11
PLA-TPGS structure polymeric micelles, which have followed sustained drug release in PBS up to
12
72 h. Interestingly, the sustained drug release kinetics of DTX-PLA-TPGS-Tf was related to the
13
transferrin conjugate on the micelles [20].
15 16 17
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Figure 4 (approximate position)
3.6. Cytotoxicity of drug formulations
18
In-vitro cytotoxicity in the A549 human lung cancer cells was assessed after 24 h
19
incubation with the DTX formulated in the DTX-PLA-TPGS and DTX-PLA-TPGS-Tf at 37 0C in
20
comparison with that of DocelTM at the equivalent drug concentration. The results are presented in
21
Fig. 5. It is worthy to note that the DTX-PLA-TPGS achieved the higher cytotoxicity compared
22
with the case of DocelTM treatment. This could be due to the effect of enhanced cellular uptake and
23
sustained drug release manner of DTX from the PLA-TPGS polymeric micelles structure.
Singh et al: Revised submission to Int. Journal of Biological Macromolecules (26 Nov 2015) 17
Page 17 of 40
Interestingly, DTX-PLA-TPGS-Tf resulted in further raise in cytotoxicity for A549 cells
2
compared with the DTX-PLA-TPGS. It is straightforward to understand that the increase in drug
3
concentration from 0.025 µg/ml to 25 µg/ml resulted in targeted and higher cytotoxicity for
4
DTX-PLA-TPGS-Tf due to transferrin receptor mediated endocytosis mechanism (Fig.5 and
5
Fig.6). In order to demonstrate the advantages of the DTX loaded polymeric micelles, a
6
quantitative index of inhibitory concentration, IC50, which is the drug concentration required to
7
induce 50% death of the cells incubated in a designated period, was determined. For instance, after
8
24 h incubation, IC50 for each of the three types of DTX formulations, namely the
9
DTX-PLA-TPGS and DTX-PLA-TPGS-Tf vs DocelTM were determined from the cytotoxicity
10
data to be 5.12 ± 1.39, 0.63 ± 0.22 vs 45.98 ± 1.70 µg/mL, respectively observed for A549 cells
11
which imply that the drug formulated in the DTX-PLA-TPGS and DTX-PLA-TPGS-Tf could be
12
7.7 and 70.34 folds more efficient than DocelTM after 24 h treatment (Table 3), respectively. Also,
13
results indicate that in order to kill A549 cells, the DTX-PLA-TPGS and DTX-PLA-TPGS-Tf
14
require significantly (P<0.05) lower drug concentrations in comparison to DocelTM (Fig.5 and
15
Table 4). DTX-PLA-TPGS has enhanced cytotoxicity in A549 cells because of PLA-TPGS
16
amphiphilic structure polymeric micelles, which inhibited P-gp efflux mechanism and provide
17
higher
18
(DTX-PLA-TPGS-Tf) have further enhanced cytotoxicity in A549 cells can be possibly attributed
19
to transferrin receptor targeting effect on the A549 cells (Fig.6). These results suggest that
20
transferrin decoration could significantly increase the cellular uptake of the polymeric micelles
21
[42]. Most importantly, transferrin conjugation on the polymeric micelles (DTX-PLA-TPGS-Tf)
22
would imply high concentration of drug to lung cancer cells which may reduce the systemic side
23
effects as well as cost for clinical use. Fig. 6 shows the cellular uptake mechanism of DTX
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drug
concentration
into
cells
(Fig.6).
The
targeted
polymeric
micelles
Singh et al: Revised submission to Int. Journal of Biological Macromolecules (26 Nov 2015) 18
Page 18 of 40
formulations. The targeted and non-trageted polymeric micelles have followed transferrin receptor
2
targeted endocytosis and phogocytosis effects, respectively. Kim et al., have proved that
3
polymeric micelles did not produce any toxicity at the concentration 0.0001–1 µg/ml of
4
mPEG-PDLLA copolymer in both cell lines i.e., human breast cancer cell lines (MCF7) and
5
human ovarian cancer cell lines (OVCAR-3) [37]. Recent study, de Melo-Diogo et al., have
6
proved that the biocompatibility of PLA-TPGS copolymer on 549 cell line, suggested that the
7
PLA-TPGS will not produce cytotoxic effects on cells [17].
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Table 3 (approximate position)
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Figure 5 (approximate position)
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Figure 6 (approximate position) 3.7. In-vivo safety using bronchoalveolar lavage (BAL) fluids of rats
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Lung toxicity of DTX has been reported by various researcher in both mouse and rat
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models. Normal saline exposure did not show any changes of any biochemical parameters in BAL
14
fluid. The administration of DTX formulation into the animal models induced inflammations and
15
fibrosis. To prove the safety of the DTX for lung cancer therapy, lung toxicity parameters were
16
measured. The lung toxicity parameters were observed after 7, 15 and 30 days of i.v.
17
administrations of PLA-TPGS (placebo micelles), DTX-PLA-TPGS, DTX-PLA-TPGS-Tf and
18
DocelTM. The PLA-TPGS micelles, DTX-PLA-TPGS and DTX-PLA-TPGS-Tf did not induce
19
significant (P>0.05) lung toxicity in comparison to DocelTM treated group, as evidenced from the
20
different pulmonary toxicity marker levels such as ALP, LDH and total protein counts in BAL
21
fluid of rats [50, 51].
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After 7 days ALP, LHD and protein counts levels in BAL fluids were significantly
23
(P<0.05) increased in the animal group which received DocelTM in compared to the control group
Singh et al: Revised submission to Int. Journal of Biological Macromolecules (26 Nov 2015) 19
Page 19 of 40
(normal saline treated) of animals (Fig. 7). At 15 and 30 days of post exposure, similar trends were
2
found to DocelTM. In comparison to control group (saline treated), a non-significant (P>0.05)
3
differences were observed in the ALP (Fig.7A), LDH levels (Fig.7B) and total protein counts
4
(Fig.7C) after i.v. administration of DTX-PLA-TPGS and DTX-PLA-TPGS-Tf. The major
5
adverse effects of DTX are their capabilities of damage alveoli cells, tissue damage and induce the
6
pulmonary toxicity after the i.v. administrations. The pulmonary toxicity of DTX is mainly due to
7
the poor solubility in aqueous media and also higher risk to normal cells by the activation of ROS
8
generation in the lung cells (Fig.7).
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Figure 7 (approximate position)
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4. Conclusions
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In this work, we developed transferrin conjugated PLA-TPGS micelles as effective and
14
safer platforms in DTX delivery for lung cancer therapy. Our research confirms that the solvent
15
displacement method as suitable for loading of DTX into polymeric micelles. The non-targeted
16
and targeted (transferrin conjugated) polymeric micelles showed drug encapsulation efficiency up
17
to 86%. The particle size analysis showed that the polymeric micelles are well structured in nano
18
size between 84.9 to 184.8 nm. In-vitro drug release profiles revealed a desired sustained drug
19
release manner of the polymeric micelles. The DTX-PLA-TPGS and DTX-PLA-TPGS-Tf
20
achieved up to 7.7 and 70.34 folds decrease in IC50 value compared with that of DocelTM after 24
21
h incubation with A549 human lung cancer cell lines. In comparison with the DocelTM, DTX
22
loaded PLA-TPGS micelles were showed significantly higher cytotoxicity, low toxic profiles and
23
thereby improved efficacy as well as safety for lung cancer therapy.
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1 2
Acknowledgements Author Mr. Rahul Pratap Singh acknowledges the University Grants Commission (UGC),
4
New Delhi, India, for the award of Rajiv Gandhi National Fellowship (RGNF)
5
(RGNF-2012-13-SC-UTT-18279) to his doctoral research in the year of 2012-2013.
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Declaration of interest: The authors report no declaration of interest.
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Table Captions:
Table 1. Formulae of PLA-TPGS micelles.
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Table 2. Particle size, polydispersity, zeta potential, encapsulation efficiency and drug loading of DTX loaded polymeric micelles.
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Table 3. IC50 values of DTX formulated as PLA-TPGS polymeric micelles or DocelTM for human lung cancer cells (n=4).
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Figure Captions: Fig.1. Schematic diagram for (A) synthesis of (i) PLA-TPGS copolymer (B) activation of (i) TPGS (TPGS-COOH) (ii) synthesis of TPGS-Tf (C) preparation of (i) DTX-PLA-TPGS: DTX loaded polymeric micelles and (ii DTX-PLA-TPGS-Tf: DTX loaded transferrin conjugated polymeric micelles. Singh et al: Revised submission to Int. Journal of Biological Macromolecules (26 Nov 2015) 29
Page 29 of 40
Fig.2. (A) FTIR spectra of L-LA, TPGS and PLA-TPGS copolymer (B) TPGS-COOH (carboxylated TPGS) and TPGS-Tf (transferrin conjugated TPGS).
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Fig.3. (A) Particle size and (B) polydispersity index of placebo polymeric micelles (PLA-TPGS), DTX-PLA-TPGS: DTX loaded polymeric micelles and DTX-PLA-TPGS-Tf: DTX loaded transferrin conjugated polymeric micelles and (C) particle size distribution of DTX-PLA-TPGS: DTX loaded polymeric micelles and (D), drug encapsulation efficiency of DTX-PLA-TPGS: DTX loaded polymeric micelles and DTX-PLA-TPGS-Tf: DTX loaded transferrin conjugated polymeric micelles.
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Fig.4. In-vitro drug release from DTX loaded preparations in PBS (pH 7.4). Bar represent ± S.D (n=3). DocelTM: commercial DTX preparation (control), DTX-PLA-TPGS: DTX loaded polymeric micelles and DTX-PLA-TPGS-Tf: DTX loaded transferrin conjugated polymeric micelles.
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Fig.5. Cytotoxicity and antiproliferative profile of DTX formulated as polymeric micelles or DocelTM for human lung cancer cells (n=4). DocelTM (DTX injection), DTX-PLA-TPGS (DTX loaded polymeric micelles) and DTX-PLA-TPGS-Tf (DTX loaded transferrin conjugated polymeric micelles).
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Fig.6. The proposed mechanisms: passive diffusion, transferrin receptor mediated endocytosis and phagocytosis of various formulations. (A) Passive diffusion of DocelTM (marketed preparation) with p-gp efflux (B) transferrin receptor mediated endocytosis for DTX-PLA-TPGS polymeric micelles, involves the formation of vesicles transferrin receptor regions of the plasma membrane. The transferrin in the cytosol are then recycled back to the plasma membrane followed by movement of ingested materials from early endosome to the late endosome, finally fusing lysosome to form the lysosome-endosome hybrid and (C) phagocytosis occurs in phagosomes for DTX-PLA-TPGS (released DTX was involved in interaction with microtubule).
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Fig.7. In-vivo safety study of DTX loaded TPGS polymeric micelles; (A) Alkaline phosphatase activity (KA Units); (B) LDH activity (U/L) and (C) Total protein counts (g/dl) in BAL fluid of rats. Control; Saline treatment; DocelTM: DTX injection, PLA-TPGS: Placebo polymeric micelles, DTX-PLA-TPGS: DTX loaded polymeric micelles and DTX-PLA-TPGS-Tf: DTX loaded transferrin conjugated polymeric micelles.
Table 1 Formulae of PLA-TPGS micelles. S. No. 1 2 3
Batch PLA-TPGS (Placebo) DTX-PLA-TPGS DTX-PLA-TPGS-Tf
DTX (mg) 3 3
PLA-TPGS (mg) 25 25 25
TPGS-Tf (mg) 10
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1 PLA-TPGS: Placebo polymeric micelles
3
DTX-PLA-TPGS: DTX loaded polymeric micelles
4
DTX-PLA-TPGS-Tf: DTX loaded transferrin conjugated polymeric micelles
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Table 2 Particle size, polydispersity, zeta potential, encapsulation efficiency and drug loading of DTX loaded polymeric micelles. Batches
Particle size (nm)
Polydispersity (mean ± S.Da)
Zeta potential
Encapsulation efficiency
Drug loading
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(mean ± S.Da) PLA-TPGS DTX-PLA-TPGS DTX-PLA-TPGS-Tf
84.09 ± 7.3 135.3 ± 6.54 184.8 ± 9.22
0.45 ± 0.04 0.40 ± 0.05 0.43 ± 0.04
(mV) (mean ± S.Da) - 12.1 ± 1.8 - 8. 64 ± 0.6 2.88 ± 0.4
71.14 ± 6.7 86.63 ± 4.2
(µg/mg) (mean ± SDa,*) 37.23 ± 3.2 39.69 ± 2.4
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(%) (mean ± S.Da,b)
a
n=3
3
b
Drug encapsulation efficiency (%) = (amount of DTX encapsulated in the micelles/ amount of
cr
2
DTX added during micelles fabrication) x 100
us
4
* Drug loading = (weight of DTX (µg) per one mg of the drug-loaded micelles)
6
S.D: Standard deviation
7
PLA-TPGS: Placebo polymeric micelles
8
DTX-PLA-TPGS: DTX loaded polymeric micelles
9
DTX-PLA-TPGS-Tf: DTX loaded transferrin conjugated polymeric micelles
M
d Ac ce pt e
10 11 12 13 14 15 16 17 18 19 20 21 22 23 24 25 26 27 28
an
5
Table 3 IC50 values of DTX formulated as PLA-TPGS polymeric micelles or DocelTM for human lung cancer cells (n=4). Formulation TM
Docel
IC50 in µg/ml on human lung cancer cells (A549) 45.98 ± 1.70
Singh et al: Revised submission to Int. Journal of Biological Macromolecules (26 Nov 2015) 32
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5.12 ± 1.39* 0.63 ± 0.22*,a
DTX-PLA-TPGS DTX-PLA-TPGS-Tf 2
a
n=4
3
*
represents significant differences (p< 0.05) from the DocelTM
4
a
represents significant differences (p< 0.05) from the DTX-PLA-TPGS
5
ip t
1
DocelTM: (DTX injection)
7
DTX-PLA-TPGS: DTX loaded polymeric micelles
8
DTX-PLA-TPGS-Tf: DTX loaded transferrin conjugated polymeric micelles
us an
9 10 11 12 13 14
M
15
Ac ce pt e
d
16 17 18 19 20 21 22 23 24 25 26 27 28 29 30 31
A
Sn(Oct)2
(i)
+ L-LA
32 33
cr
6
TPGS
120 0C / 4 h, under N2 atmosphere
PLA-TPGS
Singh et al: Revised submission to Int. Journal of Biological Macromolecules (26 Nov 2015) 33
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Succinic Anhydride
- COOH
Transferrin - NH2
(ii)
- COOH
NHS/EDC
TPGS-Tf
(i)
+
Docetaxel
+
Ac ce pt e
(ii)
PLA-TPGS
TPGS-Tf
Non-targeted micelles
d
M
PLA-TPGS
an
C
us
TPGS-COOH
1 2
3 4 5 6 7 8 9 10 11
TPGS-COOH
ip t
DMAP / 100 0C
TPGS
cr
B
(i)
Docetaxel
Targeted micelles
Fig.1. Schematic diagram for (A) synthesis of (i) PLA-TPGS copolymer (B) activation of (i) TPGS (TPGS-COOH) (ii) synthesis of TPGS-Tf (C) preparation of (i) DTX-PLA-TPGS: DTX loaded polymeric micelles and (ii) DTX-PLA-TPGS-Tf: DTX loaded transferrin conjugated polymeric micelles.
Singh et al: Revised submission to Int. Journal of Biological Macromolecules (26 Nov 2015) 34
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A
110
TPGS-COOH TPGS-Tf
L -L A T PG S PL A -T P G S
110
90
90
80 70 60 50 40 30
80 70 60 50 40
20 10
30
0 500
100 0
1500
2000
25 00
300 0
3500
4 000
450 0
0
500
1000
1500
2500
3000
3500
4000
4500
Wavenumber (cm-1)
us
W a ven um ber (cm -1 )
d
M
an
Fig.2. (A) FTIR spectra of L-LA, TPGS and PLA-TPGS copolymer (B) TPGS-COOH (carboxylated TPGS) and TPGS-Tf (transferrin conjugated TPGS).
Ac ce pt e
1 2 3 4 5 6 7 8 9 10 11 12 13 14 15 16 17 18 19 20
2000
cr
0
ip t
Transmittance (%)
T ran sm ittan ce (% )
B
100
100
Singh et al: Revised submission to Int. Journal of Biological Macromolecules (26 Nov 2015) 35
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250
0.6
A
150
PLA-TPGS DTX-PLA-TPGS
100
DTX-PLA-TPGS-Tf
Polydispersity index
200
50
0.4 PLA-TPGS
0.3
DTX-PLA-TPGS DTX-PLA-TPGS-Tf
0.2 0.1
0
0 PLA-TPGS
DTX-PLA-TPGS
DTX-PLA-TPGS-Tf
PLA-TPGS
Formulation code
DTX-PLA-TPGS
DTX-PLA-TPGS-Tf
Formulation code
C D
100
cr
80 70 60 50 40 30 20 10
an
0
us
Drug encapsulation efficiency (%)
90
DTX-PLA-TPGS DTX-PLA-TPGS-Tf
DTX-PLA-TPGS-Tf
Formulation code
M
DTX-PLA-TPGS
d
Fig.3. (A) Particle size and (B) polydispersity index of placebo polymeric micelles (PLA-TPGS), DTX-PLA-TPGS: DTX loaded polymeric micelles and DTX-PLA-TPGS-Tf: DTX loaded transferrin conjugated polymeric micelles and (C) particle size distribution of DTX-PLA-TPGS: DTX loaded polymeric micelles and (D), drug encapsulation efficiency of DTX-PLA-TPGS: DTX loaded polymeric micelles and DTX-PLA-TPGS-Tf: DTX loaded transferrin conjugated polymeric micelles.
Ac ce pt e
1 2 3 4 5 6 7 8 9 10 11 12 13
ip t
Particle size (nm)
B
0.5
Singh et al: Revised submission to Int. Journal of Biological Macromolecules (26 Nov 2015) 36
Page 36 of 40
120
ip t
80 DocelTM
60
DTX-PLA-TPGS
DTX-PLA-TPGS-Tf
cr
40
20
0 20
30
40 50 Time (h)
60
70
80
d
M
Fig.4. In-vitro drug release from DTX loaded preparations in PBS (pH 7.4). Bar represent ± S.D (n=3). DocelTM: commercial DTX preparation (control), DTX-PLA-TPGS: DTX loaded polymeric micelles and DTX-PLA-TPGS-Tf: DTX loaded transferrin conjugated polymeric micelles.
Ac ce pt e
1 2 3 4 5 6 7 8 9 10 11 12
10
an
0
us
Drug released (%)
100
Singh et al: Revised submission to Int. Journal of Biological Macromolecules (26 Nov 2015) 37
Page 37 of 40
100 90
DocelTM DTX-PLA-TPGS DTX-PLA-TPGS-Tf
70
ip t
60 50 40 30
cr
Cell viability (%)
80
20
0 0.025
0.25
2.5
us
10 25
d
M
Fig.5. Cytotoxicity and antiproliferative profile of DTX formulated as polymeric micelles or DocelTM for human lung cancer cells (n=4). DocelTM (DTX injection), DTX-PLA-TPGS (DTX loaded polymeric micelles) and DTX-PLA-TPGS-Tf (DTX loaded transferrin conjugated polymeric micelles).
Ac ce pt e
1 2 3 4 5 6 7 8 9 10 11 12 13 14 15 16 17 18 19 20 21 22 23 24 25 26 27 28 29
an
Concentration of DTX in PLA-TPGS micelles (µg/ml)
Singh et al: Revised submission to Int. Journal of Biological Macromolecules (26 Nov 2015) 38
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A
B
Transferrin
Passive diffusion DocelTM
Transferrin receptor mediated endocytosis DTX-PLA-TPGS-Tf Transferrin receptor
C Phagocytosis DTX-PLA-TPGS
cr
Phagosome
P-gp excretion without inhibition Early endosome
us
Late endosome
ip t
Receptor recycling
Free TPGS
an
Inhibit P-gp
d
Fig.6. The proposed mechanisms: passive diffusion, transferrin receptor mediated endocytosis and phagocytosis of various formulations. (A) Passive diffusion of DocelTM (marketed preparation) with p-gp efflux (B) transferrin receptor mediated endocytosis for DTX-PLA-TPGS polymeric micelles, involves the formation of vesicles transferrin receptor regions of the plasma membrane. The transferrin in the cytosol are then recycled back to the plasma membrane followed by movement of ingested materials from early endosome to the late endosome, finally fusing lysosome to form the lysosome-endosome hybrid and (C) phagocytosis occurs in phagosomes for DTX-PLA-TPGS (released DTX was involved in interaction with microtubule).
Ac ce pt e
1 2 3 4 5 6 7 8 9 10 11 12 13 14 15
M
Stabilized microtubule
Singh et al: Revised submission to Int. Journal of Biological Macromolecules (26 Nov 2015) 39
Page 39 of 40
Contol
A
DocelTM
16 )s it n U14 A K ( yt 12 i ivt c 10 A se ta a 8 h p s o h 6 P e in l 4 a lk A 2
PLA-TPGS DTX-PLA-TPGS
ip t
DTX-PLA-TPGS-Tf
0 15 days
B
C
Contol DocelTM
700
12
DTX-PLA-TPGS
600
DTX-PLA-TPGS-Tf
l) /d 8 g( ts n u o C 6 n eit or lP 4 ta o T
500 400 300 200
DocelTM PLA-TPGS DTX-PLA-TPGS
2
100 0 15 days
30 days
M
0
7 days
7 days
15 days
30 days
d
Fig.7. In-vivo safety study of DTX loaded polymeric micelles; (A) Alkaline phosphatase activity (KA Units); (B) LDH activity (U/L) and (C) Total protein counts (g/dl) in BAL fluid of rats. Control; Saline treatment; DocelTM: DTX injection, PLA-TPGS: Placebo polymeric micelles, DTX-PLA-TPGS: DTX loaded polymeric micelles and DTX-PLA-TPGS-Tf: DTX loaded transferrin conjugated polymeric micelles.
Ac ce pt e
1 2 3 4 5 6 7 8 9 10
10
us
PLA-TPGS
Contol
an
) /L U ( yt i ivt c A sea n e g or d y h e D et tac a L
30 days
cr
7 days
Singh et al: Revised submission to Int. Journal of Biological Macromolecules (26 Nov 2015) 40
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