Patent Application
20110044900
1. Field of the Invention
The present invention relates to the treatment of cancer, and in particular relates to a method for treating and/or diagnosing a tumor by gold particles coated with a polymer.
2. Description of the Related Art
Colloidal nanoparticles are utilized as active elements in biosensor, bio-imaging and tumor treatment biomedical applications.
The use of nanoparticles for cancer therapy as drug carriers or radiotherapy enhancers strictly depends on the selective accumulation of the nanoparticles in tumors. Accumulation of nanoparticles is the result of the enhanced permeation and retention (EPR) effect due to the vascular leakage and abnormal vessel architecture of cancerous areas. Thus, long-term retention of nanoparticles in the tumor is important, since the decreases the nanoparticles concentration in normal areas reduces the risk of their damage by cancer therapy.
When utilizing gold nanoparticles in cancer therapy, the gold nanoparticles quickly dissipate in cancerous areas, because of the phagocytosis of the macropharge or immune cells. Thus, required absolute concentrations are difficult to achieve by utilizing a simple tail vein injection. To increase the accumulation of the nanoparticles, a PEG modification is utilized. The surface modification of the PEG can increase accumulation time to several hours.
However, in previous studies, the PEGlyated gold nanoparticle is prepared by PEG-thiol and/or their derivatives to modify the surfaces of pre-synthesized citrated reduced gold nanoparticle. Thus, the conventional PEGlyated gold nanoparticles contain various reducing agents, surfactant, or other chemical compounds to hinder reduction of the gold nanoparticles. The reducing agents and surfactant however, may lead to the cytotoxicity of healthy tissues. For example, the chemical compounds may damage cell DNA or cause cancer. Further, the chemical compounds also may lead to environmental pollution.
To circumvent the previously mentioned problems, a novel particle and method for treating cancer is required.
The invention provides a method for treating and/or diagnosing a tumor, comprising administrating an effective amount of gold particles to a subject in need thereof, and observing the distribution of the gold particles in the subject, wherein the gold particles are coated with a polymer, and the gold particle has a size of about 6.1±1.9 nm.
A detailed description is given in the following embodiments with reference to the accompanying drawings.
The present invention can be more fully understood by reading the subsequent detailed description and examples with references made to the accompanying drawings, wherein:
a shows a TEM micrograph of the gold particles of the invention;
b shows the PEG-gold particles of the invention with a 6.1±1.9 nm in diameter and reasonable size distribution.
c is X-ray diffraction (XRD) measurements of the crystal nature of PEG-gold particles of the invention;
d is a fourier transform infrared (FTIR) spectrum of a PEG-gold particle of the invention;
a-2b show that large amounts of PEG-gold particles are internalized in the cytoplasm;
c is a graph plotting cellular uptake against particle concentration;
d shows that the particle of the invention is not toxic;
a-3e are graphs plotting X-ray dosage against cell colony number;
a-4c show the time-dependent distribution profiles of PEG-gold colloidal at different administrated doses;
a-6f shows a time sequence of microradiographs extracted from real-time video sequence taken during and after the injection of PEG-gold particles;
a-7f show TEM micrographs of various mice organs and tumors;
a-8f show microscopy images of tumor, spleen, liver and lung, kidney, and muscle after H-E staining, and
The following description is of the best-contemplated mode of carrying out the invention. This description is made for the purpose of illustrating the general principles of the invention and should not be taken in a limiting sense. The scope of the invention is best determined by reference to the appended claims.
The invention provides a gold particle. The gold particle comprises a polymer coating on a surface of the particle, wherein the polymer coating does not comprise thiol groups.
The surface of the gold particle of the invention is coated with a polymer. The polymer includes PEG, PEI, PVP, IPA, or a combination thereof. In one embodiment, the particle of the invention is a gold PEGylated particle. In another embodiment, the particle of the invention is a gold PVPylated particle. The size of the particle of the invention is about 6.1±1.9 nm, and the particles of the invention have superior dispersion, shape, and size.
Note that the particle of the invention is a thiol-free particle. The gold particles of the invention may be prepared by using a high energy and high flux radiation process. For example, a precursor solution containing PEG, PEI, PVP, or IPV is irradiated with an ionizing radiation beam with high energy and high flux to convert the precursor to the particle coated with PEG, PEI, PVP, or IPV. The concentration ratio of the PEG, PEI, PVP, or IPA to the precursor may be about 0.0001:0.12. The molecular weight of the PEG may be between 1000 and 250000. Since no reducing agent or stabilizer is required in the precursor solution, the particle colloidal is clean and non-toxic, and the thiol-free particle is more suitable for biomedical applications.
Further, the gold particle of the invention has superior stability and uniform size (less than 100 nm) so that the gold particle of the invention can be significantly aggregated in the cancerous cell or tumor by EPR (enhanced permeation and retention) effect.
The thiol-free particle is used to treat and/or diagnosis tumors. The invention further provides a method for treating and/or diagnosing a tumor. The method comprises: administrating an effective amount of the gold particles of the invention to a subject in need thereof, and irradiating the tumor with a radiation. The radiation is applied to provide cancer radiotherapy or a radiology diagnosis.
The term “tumor” refers to an abnormal benign or malignant mass of tissue that is not inflammatory and possesses no physiological function. Generally, the tumor occurs in the organ selected from the group consisting of breast, lung, brain, liver, skin, kidney, GI organ, prostate, bladder, gynecological organ and any other hollow organ. The tumor comprises breast cancer, a lung cancer, a brain cancer, a liver cancer, a skin cancer, a kidney cancer, a GI cancer (gastric, colon and rectal carcinoma), a prostate cancer, a bladder cancer, or a gynecologic cancer (cervical, ovarian, uterine, vaginal, and vulvar carcinoma).
The “subject” of the invention refers to human or non-human mammal, e.g. a dog, a cat, a mouse, a rat, a cow, a sheep, a pig, a goat, or a primate, and expressly includes laboratory mammals, livestock, and domestic mammals. In one embodiment, the mammal may be a human, in others, the mammal may be a rodent, such as a mouse or a rat. In another embodiment, the subject is an animal modeled for cancer. Alternatively, the subject is a cancer patient.
The invention provides a method for diagnosing a tumor. The method comprises administrating an effective amount of gold particles to a subject in need thereof, and observing the distribution of the gold particles in the subject.
The gold particle coated with polymer has high selective accumulation and long retention in cancerous regions. Thus, the gold particles of the invention can reach much higher concentration in cancerous area to improve cancer therapy. The concentration of the gold particles in the tumor is higher than a concentration of the gold particle in a healthy tissue, such as 5 times higher than that in the healthy tissue. The gold particles concentrated in tumor areas can enhance the cell killing effects of radiotherapy, and the gold particles are easier excreted from healthy tissues, so that secondary damage is limited. In one embodiment, the concentration of the gold particle in the tumor is 21.2 times higher than the concentration of the gold particle in the healthy tissue at 36 hours after 170 mg/kg of the particle is intravenously rejected to the subject. In another embodiment, the concentration of the gold particle in the tumor is 30 times higher than the concentration of the gold particle in the healthy tissue at 12 hours after 170 mg/kg of the gold particle is intravenously rejected to the subject.
Since the gold particles of the invention have high biocompatibility, large quantity, and size homogeneity, it has a high selective accumulation in cancer regions and long retention there and in blood by the EPR effect.
The term “radiotherapy” refers to any therapeutic application of ionic radiation. The radiation may be radioactive radiation including, X-ray, ion beams, Gamma ray, fast electrons, neutrons, protons, Pi-mesons, microwaves, IR, or UV radiation. Preferably, the radiation is used to treat cancer or malignant hematopoietic diseases.
Further, because the gold particle of the invention is significantly aggregated in the tumor region, it also can be used as contrast enhancers for radiology in the diagnostic phase and during the assessment of the effects of therapy.
The gold particle of the invention can be orally, intravenously, or topically administrated to the subject; preferably, intravenously injection.
PEGylated gold particles were synthesized from aqueous hydrogen tetrachloroaurate trihydrate (HAuCl4.3H2O, Aldrich) solutions by synchrotron X-ray irradiation. To achieve the best irradiation conditions, the pH value of the HAuCl4.3H2O solution was adjusted adding a NaOH solution. The synthesis of the gold particle was performed at the BL01A beam line of the NSRRC (National Synchrotron Radiation Research Center) storage rings for 5 minutes. The photon energy distribution was centered between 10 and 15 keV and the dose rate was 5.1±0.9 kGy/sec as determined by a Fricke dosimeter with an estimated G value of 13. To obtain well-dispersed PEGylated gold colloidal solutions, a mixed water solution of gold precursors (2 mM HAuCl4.3H2O, Aldrich, Mo., US) with appropriate NaOH (0.1 M, Showa Inc., Japan) and 3.3×10−5M polyethylene glycol (PEG) (MW 6000, Showa Inc., Japan) were placed into polypropylene conical tubes (15 ml, Falcon®, Becton Dickinson, N.J.) and transferred to the facility for X-ray irradiation.
a illustrates TEM micrographs of the gold particles prepared by Example 1. The inset high-resolution image in
Mice colorectal adenocarcinoma CT26 cells (CRL-2638, ATCC, Rockville, Md.) were cultured in RPMI-1640 (Gibco, Invitrogen Corp., Carlsbad, Calif.) medium containing 10% fetal bovine serum (FBS) at 37° C. in a humidified 5% CO2 incubator. The cells grew to 80% confluence and were detached by trypsin (0.5 g porcine trypsin and 0.2 g EDTA.4Na per liter of Hanks' Balanced Salt Solution) (Sigma, Saint Louis, Mo.). For the TEM sample preparation, 1×105 CT-26 cells were seeded on a 100 mm culture dish. After 24 hours, an appropriate volume of concentrated PEGylated gold particles was added to the culture media to achieve a final colloidal concentration of 500 μm. After co-incubation of 48 hours, the cells with gold particles were trypsinized, centrifuged, and washed with PBS/5% sucrose for at least three times to remove the remaining particles. Subsequently, the cells were fixed for 2 hours in 2.5% glutaraldehyde, and postfixed for 2 hours in 1% osmium tetroxide. Dehydration was achieved by a 25%, 50%, 75%, 95%, and 100% ethanol solution. The samples were then infiltrated and embedded in 100% resin. Ultrathin sections prepared by an ultramicrotome were placed on 200-mesh copper grids for TEM measurement. Cells grown on glass slides and fixed with 2% paraformaldehyde for 15 minutes were imaged by confocal microscopy (with an Olympus FV-1000 system), wherein the cell nuclei, stained with a fluorescent dye (Hoechst 33258), were clearly observed.
Referring to
For quantitative analysis of the cellular uptake of PEGylated gold particles, CT26 cells were seeded in 6-well microplates at a density of 2×104 cell/well. After 24 hours of cell attachment, the cells were treated with different concentrations of colloidal PEGylated gold, and a quantitative analysis of gold particles was performed by ICP assay. A colonogenic cell survival test was performed with a radio-oncology linear accelerator (Clinac IX, Varian Associates, Inc., PaloAlto, Calif.) operating at 6 MV and with a dose rate of 2.4 Gy/min. 150 CT-26 cells/well were seeded and grown in a 6-well culture dish for 24 hours. PEGylated gold particles in the colloid solution (500 μM) were then introduced and retained for 48 hours, followed by irradiation by a 2 Gy dose of X-rays. The irradiated cells were further incubated for 14 days. Finally the cells were stained by 0.4% crystal violet and colonies were counted.
c shows that after co-culture for 48 hours, the amount of cellular uptake is dependant on the concentration of the added gold, wherein the uptake was about 0.5×105 particles per cell at 500 μM and increased to more than 1.0×106 particles per cell at 3000 μM. Further, standard cell viability tests demonstrated that the particles were not toxic, as shown in
For RS 2000 biological irradiator and linear accelerator irradiation, 100 EMT-6 cells/well were seeded and grown in a 6-well culture. For the laboratory-based Cu Kα1 X-ray and monochromatic synchrotron X-ray irradiation, 100 EMT-6 cells/well and CT-26 cells/well were seeded and grown in a 24-well culture and in a 48-well culture. 24 hours after cell seeding, PEG-gold particles (400 or 500 μM) were introduced and kept for 48 hours before X-ray irradiation. After irradiation, the cells were further incubated for 14 days. Finally the cells were stained by 0.4% crystal violet and colonies were counted.
a is a graph plotting X-ray dosage against colony number (EMT-6 cell), wherein the full dots refer to control cells without PEG-gold particles, and the open circles refer to cells cultured in the presence of 400 μM of PEG-gold particles. Referring to
b-3c are graphs plotting X-ray dosage against colony number (EMT-6 cell), wherein X-ray includes Cu Kα1 X-ray (
d-3e are graphs plotting X-ray dosage against colony number (EMT-6 cell), wherein the concentration of the PEG-gold particle is 500 μm (
EMT-6 syngeneic mammary carcinoma cell lines were cultured under standard conditions. Male BALB/c mice (20-25 g, 6-8-week-old) were obtained from the National Laboratory Animal Center (Taiwan). The BALB/c ByJNarl tumor models were generated by inoculating 1×106 EMT-6 cells in 10 μl PBS into the thigh of mice. The mice were used for the study 1 week after inoculation, when the tumor had grown to 50-90 mm3 (estimated as half the product of the square of the smaller diameter multiplied by the larger diameter). All animal experiments were performed according to the guidelines approved by the Laboratory Animal Care and Use Committee of Academia Sinica (Taiwan). Three individual bio-distribution experiments were performed with different injected doses of PEG-gold: 170, 231, and 488 mg/kg. The tumor-bearing mice were sacrificed at a given time points at 5 min, 10 min, 30 min, 90 min, 4 hr, 12 hr, 24 hr, and 36 hr after the colloidal injection. After sacrifice, important organs or tissues (blood, lung, tumor, muscle, brain, heart, liver, spleen and kidney) were collected for gold analysis by ICP-OES (Inductive Coupled Plasma-Optical Emission Spectroscopy).
a shows the time-dependent distribution profiles of 6 nm PEG-gold colloidal at the largest administrated dose (488 mg/kg). At 5 min, there were only trace amounts of gold particles in either tumors or muscles. At 90 min, the gold concentration in all tumors monotonically was increased. On the contrary, gold particle amounts in muscles remain unchanged or decayed so that the tumor/muscle ratio showed a linearly increasing pattern reaching 6.4 at 90 min.
b shows the time-dependent distribution profiles of 6 nm PEG-gold colloidal at a middle administrated dose (231 mg/kg) for 30 minutes to 4 hours. Referring to
The pharmacokinetics of uptake of PEG-gold nanoparticles by a RES system was also affected by the injected dose. The blood half time clearance at three administrated doses were estimated as >1.5 hr, about 4 hr and >12 hr for 488 mg/kg, 231 mg/kg and 170 mg/kg, respectively.
The strongest contrast appeared 15 min after injection. The tumors became clearly visible with no image processing. However, compared to the 50 sec images of the tail region, the boundaries of the large vessels were less visible. This indicates that between 50 and 100 sec the gold accumulation in the large vessels was depleted whereas the accumulation in the tumor and in the nearby microvascularization increased. This indicates that the EPR effect for different organs has different and sometimes complex time evolutions, not revealed by mere visual inspection.
To reveal the PEGylated gold particle distribution, TEM samples were prepared. Firstly, after the scarification of the mice, the organs were immediately fixed with glutaraldyhyde at 4 C for 24 hrs. After replacing the glutaraldyhyde by 0.1 M PBS, the samples were further fixed and stained with 1% osmium tetraoxide in a buffer and dehydrated by a series of alcohol treatments, embedded in resin, and sliced to 90-100 nm in thicknesses using a Leica Ultracut R ultramicrotone. After being double stained with uranyl acetate and lead citrate, the specimens were observed by a Hitachi H-7500 TEM operating at 100 keV.
TEM micrographs of various mice organs and tumor are shown in
To examine the pathological characteristics of PEG-gold loaded organs/tissues, different organs—tumor, spleen, liver, lung, kidney and muscle—were immediately fixed in 10% formalin and dehydrated by a series of immersions in a 50%, 70%, 90% and 100% ethanol solution. They were then embedded in paraffin wax and sectioned to 2-5 μm slices with a Leica RM2235 microtome. After histological H-E staining, the slices were observed by a confocal laser scanning microscope (Leica TCS-ST, Germany).
Referring to
c shows the gold particle distribution within the network-like lobules of liver. The image indicates the formation of particle aggregates. The hypatocytes within the lobule captured the particle aggregates that accumulated within both the eosinophilic cytoplasm and the interface region.
Referring to
Referring to
Referring to
8 Balb/C mice (20 g) were injected subcutaneously in the thigh with 5×106 EMT-6 syngeneic mammary carcinoma cells performed on a RS 2000 x-ray Biological Irradiator (RadSource Tech. Inc., Boca Raton, Fla.) working at 160 kV and 25 mA with an average photon energy of about 73 KeV. The mean dose rate was 0.037 Gy/sec. After 1 week, 3 mg (0.2 cc Au, 25 mg/ml) of PEG-Au particles was introduced via tail vain injection. 12 hours after PEG-Au particles injection, a radiation dose of 10 Gy was applied for the tumor treatment. The tumor volume was t monitored every 3 days till to 3 weeks by the two perpendicular diameters with a vernier caliper. The tumor volume was calculated according to the below formula: The tumor volume=0.4(ab2). “a” is the length of the longer diameter and “b” is the length of shorter diameter.
The results clearly reveal the particle enhancement effect on the suppression of the tumor growth by x-ray irradiation as shown in
While the invention has been described by way of example and in terms of the preferred embodiments, it is to be understood that the invention is not limited to the disclosed embodiments. To the contrary, it is intended to cover various modifications and similar arrangements (as would be apparent to those skilled in the art). Therefore, the scope of the appended claims should be accorded the broadest interpretation so as to encompass all such modifications and similar arrangements.
