ANTHRACYCLINE ENCAPSULATED WITH A POLYSACCHARIDE FOR USE IN THE TREATMENT OF TUMOURS

TECHNICAL FIELD

The invention relates to a new form of a drug in the form of anthracycline encapsulated with a polysaccharide, selected from epirubicin, daunorubicin, doxorubicin, idarubicin, especially encapsulated with dextran, for use in the treatment of specific tumours. The new form of drug administration allows to increase the relative amount of chemotherapeutic agent administered, improve its targeting to the site of the desired effect while ensuring lower toxicity for the body, which makes it possible to increase the effectiveness of anti-tumour (anti-cancer) therapy carried out using an anthracycline encapsulated with a polysaccharide.

STATE OF THE ART

Anthracyclines belong to the group of anticancer antibiotics and are widely used as low-dose chemotherapeutic drugs for various tumours, in particular, leukaemia, metastatic breast cancer, ovarian cancer and colon and rectal cancer. Anthracyclines interfere with the functioning of essential cellular processes, including DNA reading and replication and cell protein synthesis. These drugs include doxorubicin, daunorubicin, idarubicin, epirubicin, dactinomycin and bleomycin. Anthracyclines have a very similar chemical structure. Anthracyclines are among the most active groups of chemotherapeutic drugs. They are highly effective against a spectrum of tumours, including both haematological malignancies and solid tumours (lymphoma, gastric cancer, non-small cell lung cancer, sarcoma, breast cancer). Among the many derivatives produced, several anthracyclines are currently used as drugs, including doxorubicin (DOX), daunorubicin (DAU), epirubicin (EPI) and idarubicin (IDA) [see literature, item 200].

Clinical use of anthracyclines is limited by the development of tumour cell resistance and toxicity to healthy tissues. Particularly severe side effects of anthracycline administration include nausea and vomiting, mucositis, stomatitis, hair loss, myelosuppression, which are for the most part reversible. Bone marrow suppression, although reversible, predisposes the patient to severe complications, such as infections during treatment. Administration of anthracyclines also causes irreversible side effects due to their high toxicity: soft tissue necrosis at the administration site in case of unintentional extravascular administration as well as high cardiotoxicity (in particular in the form of chronic congestive cardiomyopathy and heart failure). High cardiotoxicity poses a particularly high risk when administering anthracyclines in their current form, as free radicals produced by anthracyclines cause peroxidation of the sarcoplasmic reticulum of the heart, leading to the Ca²⁺-mediated necrosis of the myocardium. Said toxicity is selective for cardiac tissue because the catalase able to neutralise free radicals is not present in cardiac tissue [see literature, item 207].

To limit side effects, it was established that the maximum recommended cumulative doses of anthracyclines DAU and DOX should amount to 500 or 450 to 600 mg/m², respectively [see literature, item 201].

In various situations individual anthracyclines can be used interchangeably; however, as a rule [see literature, item 202]:

- doxorubicin (DOX) is used to treat breast tumours, breast cancer, paediatric solid tumours, Wilms tumour, sarcoma, soft tissue sarcoma, Ewing sarcoma, non-Hodgkin's lymphoma, aggressive lymphoma, lymphatic leukaemia, myeloblastic leukaemia, acute leukaemia, multiple myeloma, Hodgkin's disease, endometrial cancer, small cell lung cancer, gastric cancer, papillary and follicular thyroid cancer, bladder cancer, osteosarcoma, neuroblastoma,
- daunorubicin (DAU) is used to treat leukaemia, particularly acute lymphoblastic leukaemia and myeloid leukaemia,
- idarubicin (IDA) is used to treat leukaemia, especially acute myeloid leukaemia and acute lymphatic leukaemia and breast cancer;
- epirubicin (EPI) is used to treat breast cancer, lymphoma, including malignant lymphoma, non-Hodgkin's lymphoma, sarcoma, including soft tissues, ovarian cancer, leukaemia, small cell lung cancer, gastric tumour, bladder tumour.

Patent PL221351 discloses a method for obtaining nanoparticles from polysaccharides and their derivatives, which are carriers of active substances due to their specific partial oxidation to form aldehyde groups and the attachment of compounds containing an amine or other group with an R—NH2 binding reacting with aldehyde groups, wherein the active substance containing an amine, amide or hydrazide group may be a drug, for example, daunorubicin, doxorubicin. Accordingly, PL221351 discloses a method for producing anthracyclines encapsulated with a polysaccharide.

The first drug authorised for medical use (FDA 1995) based on nanoparticles was a combination of liposomes and doxorubicin. Since then, several combinations of nanoparticles with anthracycline drugs have been authorised for therapeutic use. However, all solutions are based on liposomes, and they only involve two drugs from this group: doxorubicin and daunorubicin [see literature, item 208].

The efficacy of anthracyclines in the treatment of tumours, especially doxorubicin, daunorubicin, idarubicin, epirubicin, is reduced due to the lack of targeted drug delivery to tissues with neoplastic lesions and low therapeutic index as well as relatively high toxicity.

SUMMARY OF THE INVENTION

The subject of this invention is to overcome the aforementioned state of the art drawbacks and to provide new forms of anthracycline drugs for the treatment of specific tumours in the form of doxorubicin, daunorubicin, epirubicin and idarubicin encapsulated with a polysaccharide, preferably dextran, which will ensure enhanced targeted delivery of the drug to tissues with neoplastic lesions, will have a higher therapeutic index compared to free forms of anthracyclines and are characterised by reduced toxicity.

Although various forms of drugs in the form of nanoparticles have been known, including anti-tumour drugs, no use is known of specific anthracyclines encapsulated with a specific polysaccharide for treating specific tumours, which, by using a new form of the drug have a reduced toxicity, so that they can be used in modified form, including higher doses, to consequently achieve a better therapeutic effect.

Surprisingly, it was found that anthracyclines encapsulated with a polysaccharide, more preferably with dextran, selected from doxorubicin, daunorubicin, epirubicin and idarubicin reduce the overall toxicity of the pharmaceutical and increase drug tolerance in the subject even without being targeted to the respective site by targeting particles.

The invention relates to an anthracycline encapsulated with a polysaccharide for use in tumour treatment, which anthracycline is selected from epirubicin, daunorubicin, doxorubicin, idarubicin, and the tumour is selected from pediatric solid tumours, Wilms tumour, sarcoma, soft tissue sarcoma, Ewing sarcoma, non-Hodgkin's lymphoma, leukaemia, acute leukaemia, lymphoblastic leukaemia, myeloblastic leukaemia, myeloid leukaemia, multiple myeloma, Hodgkin's disease, sarcomas, soft tissue sarcoma, breast tumour, breast cancer, lung tumours, lung cancer, small cell lung cancer, gastric tumour, gastric cancer, bladder cancer, papillary bladder cancer from transitional epithelium cells, thyroid cancer, thyroid cancer, papillary or follicular thyroid cancer, pancreatic tumour, cervical cancer, ovarian cancer, endometrial cancer, kidney cancer, osteosarcoma, neuroblastoma, colorectal cancer.

Preferably, in the anthracycline encapsulated with a polysaccharide for use in tumour treatment the polysaccharide is selected from dextran, starch and derivatives thereof, amylose and derivatives thereof, derivatives of cellulose, glycogen, hyaluronic acid, heparin, alginic acid, carrageenan, and more preferably, the polysaccharide is selected from dextran, cellulose and derivatives thereof, amylose, starch and heparin. Preferably in the use of the anthracycline encapsulated with a polysaccharide for use in tumour treatment, the tumour is selected from a breast tumour, breast cancer, cervical cancer, ovarian cancer, pancreatic cancer, kidney cancer, lung cancer, colorectal cancer.

Preferably in the use of the anthracycline encapsulated with a polysaccharide for use in tumour treatment, a particular anthracycline encapsulated with a particular polysaccharide is administered to the subject being treated at a dose higher than the maximum tolerated dose (MTD) established for the same anthracycline not encapsulated with a polysaccharide, and at a dose lower than the maximum tolerated dose established for a particular anthracycline encapsulated with the same polysaccharide, wherein the subject is preferably a mammal, and, more preferably, the subject is a human.

Preferably, the anthracycline encapsulated with a polysaccharide for use in tumour treatment is epirubicin, which is used to treat tumour selected from breast tumours, breast cancer, lymphomas including malignant lymphomas, non-Hodgkin's lymphoma, sarcomas including soft tissue sarcomas, ovarian cancer, cervical cancer, leukaemia, lung tumours, lung cancer, small cell lung cancer, gastric cancer, kidney cancer, bladder cancer, pancreatic cancer, colorectal cancer.

Preferably, the anthracycline encapsulated with a polysaccharide for use in tumour treatment is epirubicin encapsulated with dextran.

Preferably, the anthracycline encapsulated with a polysaccharide for use in tumour treatment, when it is epirubicin encapsulated with dextran, is for treating breast tumour, breast cancer, cervical cancer, ovarian cancer, pancreatic cancer, kidney cancer, lung cancer, colorectal cancer.

In an equally preferable embodiment, the anthracycline encapsulated with a polysaccharide for tumour treatment in the form of epirubicin encapsulated with dextran is intended for the treatment of ovarian cancer.

In a particularly preferred embodiment, the anthracycline encapsulated with a polysaccharide for tumour treatment in the form of epirubicin encapsulated with dextran is intended for the treatment of pancreatic cancer.

Preferably, the anthracycline encapsulated with a polysaccharide for use in tumour treatment is daunorubicin, which is used to tumour selected from leukaemia, especially acute lymphoblastic leukaemia and myeloid leukaemia, breast tumours, breast cancer, cervical cancer, ovarian cancer, pancreatic cancer, kidney cancer, lung cancer, colorectal cancer, and more preferably, daunorubicin is encapsulated with dextran.

Preferably, the anthracycline encapsulated with a polysaccharide for tumour treatment in the form of daunorubicin encapsulated with dextran is intended for the treatment of tumour selected from leukaemia, especially acute lymphoblastic leukaemia and myeloid leukaemia, ovarian cancer, breast tumours, breast cancer, cervical cancer.

Equally preferably, the anthracycline encapsulated with a polysaccharide for use in tumour treatment is doxorubicin encapsulated with a polysaccharide, which is used for the treatment of a tumour selected from paediatric solid tumours, Wilms tumour, sarcoma, soft tissue sarcoma, Ewing sarcoma, non-Hodgkin's lymphoma, aggressive lymphoma, lymphatic leukaemia, lymphoblastic leukaemia, myeloblastic leukaemia, acute leukaemia, multiple myeloma, Hodgkin's disease, breast tumours, breast cancer, endometrial cancer, lung tumours, small cell lung cancer, gastric cancer, thyroid cancer, papillary or follicular thyroid cancer, bladder cancer, osteosarcoma, neuroblastoma, cervical cancer, ovarian cancer, pancreatic cancer, kidney cancer, colorectal cancer, wherein preferably doxorubicin is encapsulated with dextran.

When the anthracycline encapsulated with a polysaccharide for use in tumour treatment is idarubicin, encapsulated with a polysaccharide, preferably it is used to treat tumour selected from leukaemia, especially acute myeloid leukaemia and acute lymphatic leukaemia, breast tumours, breast cancer, cervical cancer, ovarian cancer, pancreatic cancer, kidney cancer, lung cancer, colorectal cancer, wherein preferably idarubicin is encapsulated with dextran.

In a preferable embodiment, the anthracycline encapsulated with a polysaccharide for tumour treatment, anthracycline particles used for tumour treatment have an average size in the range of 10-500 nm, more preferably 50-200 nm, most preferably 70-160 nm (diameters in a hydrated state).

In said embodiment of the invention, anthracyclines encapsulated with a polysaccharide can be used for monotherapy, combined therapy, simultaneous or subsequent use in anti-tumour therapy. A known chemotherapeutic agent, e.g. cis-platinum or a radiotherapeutic agent may be an additional auxiliary component. Therapy of this kind reduces undesired side effects.

In general, anthracyclines encapsulated with a polysaccharide are intended for intravenous administration, although in specific embodiments, e.g. for the treatment of bladder cancer, they may be used as intravesical infusions.

Anthracyclines encapsulated with a polysaccharide in use for tumour treatment according to the invention in the form of finished injectable formulations comprise aqueous and non-aqueous isotonic sterile solutions, optionally containing antioxidants, buffers, isotonic additives and the like. A typical carrier is, e.g. injection water or saline solution.

In general, the formulation for final use containing anthracyclines encapsulated with a polysaccharide for use in tumour treatment according to the invention is obtained by diluting or mixing them with a carrier or diluent.

The dose of anthracyclines encapsulated with a polysaccharide for use in tumour treatment of the invention is determined taking into account the type of tumour, type of therapy, patient's age, patient's weight, approximate body surface of the patient, as well as other special circumstances such as liver parameters, kidneys, cardiac history etc. A person skilled in the art will be able to determine the right dose for a particular patient. However, the single dose administered should not exceed the maximum tolerated dose established for a specific anthracycline encapsulated in a specific polysaccharide.

The publications referred to in the description and the references therein are also included herein as a reference.

BRIEF DESCRIPTION OF THE FIGURES

To be better understood, the invention has been illustrated in embodiments and the accompanying figures, where.

FIG. 1 shows the distribution of diameters of the obtained nanoparticles with the drug (A) NPs_EPI, B) NPs-DAU. Diameter distribution obtained after repeated rehydration of nanoparticles in injection water after 3 h.

FIG. 2 is a comparison of cytotoxicity to selected tumour lines. Nanoparticles with encapsulated epirubicin on lines A) A2780, B) A549, C) ACHN, D) AU565, E) COLO205, F) OVCAR-3, G) PANC1, H) HeLa and I) MCF7. The designation Epi- refers to epirubicin administered alone, NPs_Epi is the administration of dextran-encapsulated epirubicin.

FIG. 3 is a comparison of cytotoxicity to selected tumour lines. Nanoparticles with encapsulated daunorubicin on lines A) A2780, B) MCF7 C) HeLa, D) OVCAR-3, E) AU565. The designation DAU- refers to daunorubicin administered alone, NPs_DAU is the administration of dextran-encapsulated daunorubicin.

FIG. 4 The graph shows changes in tumour size and body weight in mice during the anti-tumour efficacy determination of encapsulated epirubicin (NPs_Epi) in dextran nanoparticles, administered in two doses: ½ MTD (dose of 3.75 mg/kg bw) and ¾ MTD (22.5 mg/kg bw) compared to the control (receiving water for injections) and administration of non-encapsulated Epirubicin (dose of 15 mg/kg bw).

EMBODIMENTS OF THE INVENTION

The following examples are provided solely to illustrate the invention and for clarifying the individual aspects thereof, and not to limit it, and should not be considered to be equivalent to the total scope thereof, which is defined in the appended claims. In the examples below, unless otherwise indicated, standard materials and methods were employed as used in the art, or it was proceeded according to the manufacturer's recommendations for particular materials and methods.

EXAMPLES
Example 1

Production of Anthracyclines Encapsulated with a Polysaccharide

(a) Preparation of Dextran-Encapsulated Epirubicin (NPs_EPI)

Dextran-encapsulated epirubicin was prepared according to the preparation method of nanoparticles from polysaccharides as described in patent PL221251 (see in particular Examples 2 and 4) using dextran with a molecular weight of 70 kDa (oxidation degree 5-15%) and dodecylamine hydrochloride. The substitution degree of aldehyde groups produced in dextran by winding agent dodecylamine is 10-20%. The substitution degree of aldehyde groups produced in dextran by epirubicin is 4-10%. The other generated aldehyde groups were substituted with alanine. Nanoparticles were prepared with an average size-between 80 and 140 nm (FIG. 1 A) as measured in aqueous solutions using NanoSight LM 10 (405 nm laser). The determined epirubicin content in a dry matter of nanoparticles is 3.0-5%. The obtained nanoparticles were freeze-dried and stored in sealed containers at the temperature of 4° C. Before the tests, the nanoparticles were again rehydrated (suspended) for 3 h in injection water.

(b) Preparation of Dextran-Encapsulated Daunorubicin (NPs_DAU)

Dextran-encapsulated daunorubicin was prepared according to the preparation method of nanoparticles from polysaccharides as described in patent PL221251 (see in particular Examples 2 and 4) using Dextran with a molecular weight of 70 kDa (oxidation degree 5-15%) and dodecylamine hydrochloride. The substitution degree of aldehyde groups produced in dextran by winding agent dodecylamine is 10-20%. The substitution degree of aldehyde groups produced in dextran by daunorubicin is 4-10%. The other generated aldehyde groups were substituted with alanine. Nanoparticles were produced with an average size between 80 and 140 nm (FIG. 1B) as measured in aqueous solutions using NanoSight LM 10 (405 nm laser). The determined daunorubicin content in a dry matter of nanoparticles is 3.0-5%. The obtained nanoparticles were freeze-dried and stored in sealed containers at the temperature of 4° C. Before the tests, the nanoparticles were again rehydrated (suspended) for 3 h in injection water.

Dextran-encapsulated doxorubicin was prepared according to the preparation method of nanoparticles from polysaccharides as described in patent PL221251 (see in particular Examples 2 and 4) using Dextran with a molecular weight of 70 kDa (oxidation degree 5-15%) and dodecylamine hydrochloride. The substitution degree of aldehyde groups produced in dextran by winding agent dodecylamine is 10-20%. The substitution degree of aldehyde groups produced in dextran by doxorubicin is 4-10%. The other generated aldehyde groups were substituted with alanine. Nanoparticles of 80-150 nm were produced as measured in aqueous solutions using NanoSight LM 10 (405 nm laser). The determined doxorubicin content in a dry matter of nanoparticles is 3.0-5%. The obtained nanoparticles were freeze-dried and stored in sealed containers at the temperature of 4° C. Before the tests, the nanoparticles were again rehydrated (suspended) for 3 h in injection water.

(d) Preparation of Dextran-Encapsulated Idarubicin (NPs_IDA)

Dextran-encapsulated idarubicin was prepared according to the preparation method of nanoparticles from polysaccharides as described in patent PL221251 (see in particular Examples 2 and 4) using Dextran with a molecular weight of 70 kDa (oxidation degree 5-15%) and dodecylamine hydrochloride. The substitution degree of aldehyde groups produced in dextran by winding agent dodecylamine is 10-20%. The substitution degree of aldehyde groups produced in dextran by idarubicin is 4-10%. The other generated aldehyde groups were substituted with alanine. Nanoparticles were produced with an average size of 80-150 nm, as measured in aqueous solutions using NanoSight LM 10 (405 nm laser). The determined idarubicin content in a dry matter of nanoparticles is 3.0-5%. The obtained nanoparticles were freeze-dried and stored in sealed containers at the temperature of 4° C. Before the tests, the nanoparticles were again rehydrated (suspended) for 3 h in injection water.

A similar method was used to prepare nanoparticles encapsulated with another polysaccharide: cellulose, amylose, starch and heparin, encapsulating: epirubicin, daunorubicin, doxorubicin and idarubicin. A similar method was used to obtain nanoparticles from particular polysaccharides dextran and cellulose, amylose, starch, heparin, which contained no anthracyclines, and which served as controls in further studies.

Example 2

Determination of Cytotoxicity of Anthracyclines Encapsulated with a Polysaccharide on Cell Lines (Nanoparticles Combined with the Drug)

The subject of the study was to determine the cytotoxicity of a combination of anthracyclines encapsulated with a polysaccharide EPI, DAU, DOX, IDA on cell lines. Toxicity was assessed using a quantitative method based on the colourimetric technique (MTT) [see literature item 203]. In this test, amber dehydrogenase present in the cells converts the soluble tetrazolium salt (3-4,5-dimethylthiazol-2-yl)-2,5-diphenyltetrazolium bromide) into a reduced form. The reaction yields water-insoluble purple crystalline formazan. The number of crystals formed depends on the enzyme activity so that it is directly proportional to the number of viable cells in the sample. Spectrophotometric measurement requires the use of an organic solvent to dissolve the crystals obtained (isopropanol). The change in colour intensity is measured by spectrophotometry at 570 nm wavelength. The test was performed for a number of dilutions (9) of nanoparticle solutions containing the tested anthracycline. The baseline concentration of nanoparticles for MTT tests was 2.5 mg of nanoparticles/ml. The results were compared to cytotoxicity results obtained for pure drugs with equimolar drug concentration (equal to the concentration encapsulated in nanoparticles). The study was also performed for drug-free nanoparticles (the carrier itself was obtained similarly to the nanoparticles with the drug). Cells not exposed to toxic substances were used as a control for toxicity studies.

Study protocol [see literature items 204, 205].

After reaching 85-90% confluence, the cells were trypsinised using a 0.25% trypsin solution. The cells were then centrifuged (1200 rpm, 5 min.) and suspended in a culture medium suitable for a particular cell line. The medium did not contain phenolic red. The cells were plated at a concentration of 1000 cells/100 μl of medium per culture well (96-well plates). The prepared plates were incubated (37° C./5% CO₂/22 h to 26 h). Subsequently, the culture medium was replaced with a fresh one (100 μl) containing the appropriate concentration of the tested nanoparticles and set aside for 24 h (37° C./5% CO₂). After the lapse of the test time, the medium was removed and replaced with 50 μl of an MTT reagent solution at a concentration of 1 mg/ml. The plate was incubated for 2 hours (37° C./5% CO₂). Subsequently, the MTT solution was removed, and 100 μl of isopropanol was added. After shaking the plate on the shaker for 2 minutes, the results for 570 nm wavelength were read (reference value of 650 nm). The mean value of absorbance read OD570 of the cells not exposed to a toxic agent (control) should be above 0.7 [see literature item 206].

Data Analysis

A decrease in the number of viable cells causes a decrease in metabolic activity in the sample. This reduction directly correlates with the amount of blue and purple formazan formed, monitored basing on the optical density at 570 nm. The following equation (C.1) is used to calculate viability reduction compared to control:

$V_{iab %} = \frac{100 \times {OD}_{570 e}}{{OD}_{570 b}}$

where: • OD570e is the mean value of the measured absorbance of the test samples; • OD570b is the mean value of the measured absorbance of the control.

The results obtained were statistically analysed using the Dixon Q test.

TABLE 1

Tested cell lines:

Cell line

(derived from tumour -

tumour testing model)
Source
Medium used

MCF-7
ECACC
DMEM

breast/mammary gland

10% foetal bovine serum

1% Penicillin-Streptomycin

L-glutamine 2 mM

AU565
ATCC ®
RPMI-1640

breast/mammary gland

10% foetal bovine serum

1% Penicillin-Streptomycin

L-glutamine 2 mM

HeLa
ECACC
DMEM

uterine cervix

10% foetal bovine serum

1% Penicillin-Streptomycin

L-glutamine 2 mM

PANC-1
ECACC
DMEM

pancreas

10% foetal bovine serum

1% Penicillin-Streptomycin

L-glutamine 2 mM

OVCAR-3
ATCC ®
RPMI-1640

Ovary

20% foetal bovine serum

1% Penicillin-Streptomycin

L-glutamine 2 mM + insulin

ACHN
ECACC
DMEM

Kidneys

10% foetal bovine serum

1% Penicillin-Streptomycin

L-glutamine 2 mM

A2780
ECACC
RPMI-1640

Ovary

10% foetal bovine serum

1% Penicillin-Streptomycin

L-glutamine 2 mM

A549
ECACC
DMEM

Lung

10% foetal bovine serum

1% Penicillin-Streptomycin

L-glutamine 2 mM

COLO 205
ECACC
RPMI-1640

Large intestine/colon

10% foetal bovine serum

1% Penicillin-Streptomycin

L-glutamine 2 mM

The toxicity of the test nanoparticle formulation containing an anthracycline should be similar to that of a pure drug. There should be no toxicity of nanoparticles as such.

Toxicity Analysis of Polysaccharide Nanoparticles without Anthracycline

The obtained results confirmed the lack of toxicity of the carrier alone in the form of polysaccharide nanoparticles in the form of dextran nanoparticles for all cell lines tested. Similar results were obtained for the other polysaccharide carriers (carriers in the form of nanoparticles of cellulose, amylose, starch and heparin).

The highest concentration of nanoparticles (2.5 mg nanoparticles/ml) causes up to 20% decrease in toxicity (Table 1).

TABLE 1

Shows the result of the MTT cytotoxicity test on the HeLa cell line for the dextran carrier

NPs-carrier

Concentration of NPs [ng/ml]
1.00E+07
5.00E+06
2.50E+06
2.50E+05
2.50E+04
2.50E+03
2.50E+02
2.50E+01

Average cell viability [%]
75.437
82.389
87.647
91.003
107.418
104.579
106.158
104.212

SD [%]
0.978
0.223
0.104
1.969
2.929
1.196
3.251
3.658

where SD: standard deviation for n = 8

Toxicity Analysis of Polysaccharide Nanoparticles with Anthracycline

Studies conducted for anthracycline-containing nanoparticles (produced according to Example 1) mostly showed a toxicity profile similar to that of a pure drug (e.g. FIG. 2, toxicity graph of DAU nanoparticles for the MCF-7 cell line and EPI nanoparticles for the COLO 205 cell line). On the other hand, higher in vitro toxicity was observed for some cell lines despite the use of an equimolar drug concentration (e.g. FIG. 3 D (OVCAR3_NPs-DAU) toxicity graph for DAU-dextran nanoparticles on the OVCAR-3 cell line, FIG. 2A, B, C, F, G toxicity graphs for NPs_EPI). Such a result indicates that selected cell lines, and, consequently, the corresponding tumours, are more sensitive to drugs encapsulated in polysaccharide nanoparticles due to no defence mechanisms against drugs encapsulated in polysaccharide nanoparticles or increased uptake of such structures by cells. For the animal tests disclosed in the following examples, tumour lines were selected with a higher toxic response on given tumour line than the pure drug or which had at least the same response. Such a choice was dictated by the expected higher efficacy of the formulation against tumour or at least the same efficacy of the formulation in the form encapsulated with the polysaccharide. The obtained results are presented in the graphs in FIG. 2 and FIG. 3 and in Table 2 below.

TABLE 2

shows the results of MTT NPs_Epi and NPs_Dau cytotoxicity test versus Epi and

Dau for some tumour lines. Where: NPs_Epi/NPs_Dau: epirubicin/daunorubicin encapsulated

with dextran nanoparticles; Epi, Dau is epirubicin and daunorubicin administered as

a pure non-encapsulated drug, respectively; SD: is standard deviation expressed in

% for 8 test replicates for a specific drug concentration or NPs-drug concentration

A2780_Epi

Concentration of NPs [ng/ml]
5.00E+03
1.25E+04
2.50E+04
5.00E+04
1.2E+05

Average viability [%]
95.203
90.784
89.24
83.629
69.996

SD [%]
4.656
1.756
5.715
6.047
4.455

A2780_NPs_Epi

Concentration of NPs [ng/ml]
5.00E+03
1.25E+04
2.50E+04
5.00E+04
1.25E+05

Average viability [%]
87.857
85.783
87.666
88.661
71.576

SD [%]
2.64
2.35
2.76
3.189
3.084

A549_NPs_Epi

Concentration of NPs [ng/ml]
5.00E+03
1.25E+04
2.50E+04
5.00E+04
1.25E+05

Average viability [%]
103.66
96.938
96.926
93.941
82.055

SD [%]
6.278
6.107
5.521
4.269
5.202

A549_Epi

Concentration of NPs [ng/ml]
5.00E+03
1.25E+04
2.50E+04
5.00E+04
1.25E+05

Average viability [%]
103.44
95.631
88.608
74.693
83.913

SD [%]
3.412
2.589
6.123
10.105
4.674

ACHN_Epi

Concentration of NPs [ng/ml]
5.00E+03
1.25E+04
2.50E+04
5.00E+04
1.25E+05

Average viability [%]
81.178
65.301
63.713
59.828
63.237

SD [%]
7.627
3.938
3.629
3.093
3.669

ACHN_NPs_Epi

Concentration of NPs [ng/ml]
5000
12500
25000
50000
125000

Average viability [%]
89.542
73.785
69.871
66.614
62.764

SD [%]
5.396
5.251
5.281
2.844
6.691

AU565_Epi

Concentration of NPs [ng/ml]
5.00E+03
1.25E-04
2.50E+04
5.00E-04
1.25E+05

Average viability [%]
84.738
66.48
66.439
48.052
48.38

SD [%]
5.662
2.336
4.299
4.205
3.48

AU565_NPs_Epi

Concentration of NPs [ng/ml]
5.00E+03
1.25E+04
2.50E+04
5.00E+04
1.25E+05

Average viability [%]
89.859
78.632
73.084
64.315
52.404

SD [%]
4.847
5.117
3.234
3.906
3.999

Colo205_Epi

Concentration of NPs [ng/ml]
5.00E+03
1.25E+04
2.50E+04
5.00E+04
1.25E-05

Average viability [%]
83.936
63.431
66.212
61.427
55.748

SD [%]
2.771
5.072
3.61
6.188
3.73

Colo205_NPs_Epi

Concentration of NPs [ng/ml]
5.00E+03
1.25E+04
25000
5.00E+04
1.25E+05

Average viability [%]
111.719
102.72
87.182
62.646
66.796

SD [%]
10.617
3.581
7.267
3.398
6.308

HeLa_Epi

Concentration of NPs [ng/ml]
5.00E+03
1.25E+04
25000
5.00E+04
1.25E+05

Average viability [%]
100.18
98.38
72.85
17.04
12.73

SD [%]
9.75
10.77
3.11
2.13
1.42

HeLa_NPs_Epi

Concentration of NPs [ng/ml]
5.00E+03
1.25E+04
25000
5.00E+04
1.25E+05

Average viability [%]
105.72
105.61
97.67
42.81
21.77

SD [%]
3.72
1.66
5.31
2.03
1.23

MCF-7_Epi

Concentration of NPs [ng/ml]
5.00E+03
1.25E+04
25000
5.00E+04
1.25E+05

Average viability [%]
97.78
88.51
64.7
56.01
46.97

SD [%]
1.57
6.29
3.44
2.53
2.12

MCF-7_NPs_Epi

Concentration of NPs [ng/ml]
5.00E+03
1.25E+04
25000
5.00E+04
1.25E+05

Average viability [%]
101.89
91.3607
80.0486
55.3861
54.0362

SD [%]
6.48
8.73
7.26
5.16
5.53

OVCAR3_Epi

Concentration of NPs fng/mll
5.00E+03
1.25E+04
2.50E+04
5.00E+04
1.25E+05

Average viability [%]
104.596
102.184
99.208
92.151
91.668

SD [%]
11.436
8.525
9.347
8.336
7.569

OVCAR3_NPs_Epi

Concentration of NPs [ng/ml]
5.00E+03
1.25E+04
2.50E+04
5.00E+04
1.25E+05

Average viability [%]
104.928
103.836
104.979
100.735
87.78

SD [%]
5.028
7.684
5.685
3.37
4.896

PANC1_Epi

Concentration of NPs [ng/ml]
5.00E+03
1.25E+04
2.50E+04
5.00E+04
1.25E+05

Average viability [%]
97.954
94.813
99.155
89.898
82.872

SD [%]
8.867
8.039
9.519
10.598
7.933

PANC1_NPs_Epi

Concentration of NPs [ng/ml]
5.00E+03
1.25E+04
2.50E+04
5.00E+04
1.25E+05

Average viability [%]
95.844
93.654
97.858
94.913
86.271

SD [%]
3.811
5.859
7.306
3.017
4.051

A2780_Dau

Concentration of NPs [ng/ml]
5.00E+03
1.25E+04
2.50E+04
5.00E+04
1.25E+05

Average viability [%]
0.295
0.540
3.689
11.600
18.312

SD [%]
0.035
0.223
0.931
1.770
2.355

A2780_NPs_Dau

Concentration of NPs [ng/ml]
5.00E+03
1.25E+04
2.50E+04
5.00E+04
1.25E+05

Average viability [%]
1.514
0.574
1.150
14.843
22.915

SD [%]
0.937
0.087
0.346
1.073
4.256

AU565_Dau

Concentration of NPs [ng/ml]
5.00E+03
1.25E+04
2.50E+04
5.00E+04
1.25E+05

Average viability [%]
75.95658
58.57172
33.21763
28.25821
25.83484

SD [%]
2.539451
3.629251
2.721307
1.90153
2.585976

AU565_NPs_Dau

Concentration of NPs [ng/ml]
5.00E+03
1.25E+04
2.50E+04
5.00E+04
1.25E+05

Average viability [%]
71.95658
52.57172
32.21763
29.25821
30.83484

SD [%]
2.539451
3.629251
2.721307
1.90153
2.585976

HeLa_Dau

Concentration of NPs [ng/ml]
5.00E+03
1.25E+04
2.50E+04
5.00E+04
1.25E+05

Average viability [%]
2.054
2.851
2.108
4.138
7.890

SD [%]
0.592
1.899
1.524
0.857
2.888

HeLa_NPs_Dau

Concentration of NPs [ng/ml]
5.00E+03
1.25E+04
2.50E+04
5.00E+04
1.25E+05

Average viability [%]
3.324
3.726
4.734
6.759
5.897

SD [%]
1.583
2.104
2.407
0.827
1.122

MCF-7_Dau

Concentration of NPs [ng/ml]
5.00E+03
1.25E+04
2.50E+04
5.00E+04
1.25E+05

Average viability [%]
1.311
1.153
1.072
4.421
17.162

SD [%]
0.625
0.312
0.371
2.079
6.357

MCF-7_NPs_Dau

Concentration of NPs [ng/ml]
5.00E+03
1.25E+04
2.50E+04
5.00E+04
1.25E+05

Average viability [%]
1.585
2.972
1.132
11.281
19.679

SD [%]
0.266
1.500
0.224
3.806
3.086

OVCAR-3_Dau

Concentration of NPs [ng/ml]
5.00E+03
1.25E+04
2.50E+04
5.00E+04
1.25E+05

Average viability [%]
1.330
3.616
43.386
52.550
59.635

SD [%]
0.251
2.964
1.967
3.236
2.514

OVCAR-3_NPs_Dau

Concentration of NPs [ng/ml]
5.00E+03
1.25E+04
2.50E+04
5.00E+04
1.25E+05

Average viability [%]
3.400
2.580
31.840
50.660
50.740

SD [%]
1.245
0.723
2.189
2.464
2.535

Colo205_Dau

Concentration of NPs [ng/ml]
5.00E+03
1.25E+04
2.50E+04
5.00E+04
1.25E+05

Average viability [%]
30.89
34.20
19.17
4.46
3.75

SD [%]
3.63
1.77
1.43
2.96
1.88

Colo205_NPs_Dau

Concentration of NPs [ng/ml]
5.00E+03
1.25E+04
2.50E+04
5.00E+04
1.25E+05

Average viability [%]
85.11
58.04
38.61
26.77
30.98

SD [%]
4.61
4.39
1.73
1.32
2.10

PANC-1_Dau

Concentration of NPs [ng/ml]
5.00E+03
1.25E+04
2.50E+04
5.00E+04
1.25E+05

Average viability [%]
95.12
93.89
61.24
56.67
48.79

SD [%]
5.16
4.73
3.88
3.67
2.83

PANC-1_NPs_Dau

Concentration of NPs [ng/ml]
5.00E+03
1.25E+04
2.50E+04
5.00E+04
1.25E+05

Average viability [%]
94.94
90.75
70.25
59.95
51.99

SD [%]
6.91
1.78
4.67
4.79
3.07

ACHN_Dau

Concentration of NPs [ng/ml]
5.00E+03
1.25E+04
2.50E+04
5.00E+04
1.25E+05

Average viability [%]
62.65
43.86
1.60
2.88
2.75

SD [%]
12.06
6.85
0.45
2.02
1.81

ACHN_NPs_Dau

Concentration of NPs [ng/ml]
5.00E+03
1.25E+04
2.50E+04
5.00E+04
1.25E+05

Average viability [%]
66.26
71.36
65.71
74.82
75.62

SD [%]
10.10
7.85
6.07
7.31
8.19

A549_Dau

Concentration of NPs [ng/ml]
5.00E+03
1.25E+04
2.50E+04
5.00E+04
1.25E+05

Average viability [%]
65.72
57.00
55.31
50.80
49.55

SD [%]
8.49
8.01
4.37
2.30
1.16

A549_NPs_Dau

Concentration of NPs [ng/ml]
5.00E+03
1.25E+04
2.50E+04
5.00E+04
1.25E+05

Average viability [%]
80.73
74.25
59.67
60.67
56.27

SD [%]
0.71
1.22
2.84
2.09
1.72

A2780_Epi

Concentration of NPs [ng/ml]
2.50E+05
5.00E+05
1.25E+06
2.50E+06

Average viability [%]
58.252
41.752
14.869
3.102

SD [%]
8.266
6.192
2.8
0.434

A2780_NPs_Epi

Concentration of NPs [ng/ml]
2.50E+05
5.00E+05
1.25E+06
2.50E+06

Average viability [%]
56.884
16.563
1.432
1.38

SD [%]
2.744
2
0.615
0.511

A549_NPs_Epi

Concentration of NPs [ng/ml]
2.50E+05
5.00E+05
1.25E+06
2.50E+06

Average viability [%]
71.201
48.475
2.267
2.565

SD [%]
11.099
7.152
0.443
0.834

A549_Epi

Concentration of NPs [ng/ml]
2.50E+05
5.00E+05
1.25E+06
2.50E+06

Average viability [%]
75.153
62.796
29.508
23.423

SD [%]
10.91
12.273
7.877
5.337

ACHN_Epi

Concentration of NPs [ng/ml]
2.50E+05
5.00E+05
1.25E+06
2.50E+06

Average viability [%]
60.112
50.916
46.66
32.352

SD [%]
2.166
2.569
2.795
3.797

ACHN_NPs_Epi

Concentration of NPs [ng/ml]
250000
500000
1250000
2500000

Average viability [%]
62.586
46.799
2.038
1.872

SD [%]
3.261
2.731
0.98
0.398

AU565_Epi

Concentration of NPs [ng/ml]
2.50E+05
5.00E+05
1.25E+06
2.50E+06

Average viability [%]
29.222
11.723
1.912
1.822

SD [%]
2.693
0.87
0.347
0.517

AU565_NPs_Epi

Concentration of NPs [ng/ml]
2.50E+05
5.00E+05
1.25E+06
2.50E+06

Average viability f %]
44.84
28.783
1.501
1.484

SD [%]
5.056
4.97
0.864
0.734

Colo205_Epi

Concentration of NPs [ng/ml]
2.50E+05
5.00E+05
1.25E+06
2.50E+06

Average viability [%]
49.549
23.946
5.063
2.239

SD [%]
4.79
5.206
1.233
1.137

Colo205_NPs_Epi

Concentration of NPs [ng/ml]
2.50E+05
5.00E+05
1.25E+06
2.50E+06

Average viability ]%]
53.903
26.718
2.136
1.231

SD ]%]
6.918
3.188
1.817
0.31

HeLa_Epi

Concentration of NPs [ng/ml]
2.50E+05
5.00E+05
1.25E+06
2.50E+06

Average viability [%]
14.93
7.96
3.6
4.21

SD [%]
1.86
1.77
0.79
0.42

HeLa_NPs_Epi

Concentration of NPs [ng/ml]
2.50E+05
5.00E+05
1.25E+06
2.50E+06

Average viability [%]
12.78
1.64
2.4
1.84

SD [%]
0.41
0.75
1
0.33

MCF-7_Epi

Concentration of NPs [ng/ml]
2.50E+05
5.00E+05
1.25E+06
2.50E+06

Average viability [%]
41.35
31.11
5.9
1.68

SD [%]
2.37
4.22
0.59
0.45

MCF-7_NPs_Epi

Concentration of NPs [ng/ml]
2.50E+05
5.00E+05
1.25E+06
2.50E+06

Average viability [%]
47.8267
8.61231
1.13391
1.12041

SD [%]
7.29
1.54
0.15
0.31

OVCAR3_Epi

Concentration of NPs fng/mll
2.50E+05
5.00E+05
1.25E+06
2.50E+06

Average viability [%]
88.222
75.986
58.803
33.266

SD [%]
7.035
6.199
7.362
1.856

OVCAR3_NPs_Epi

Concentration of NPs [ng/ml]
2.50E+05
5.00E+05
1.25E+06
2.50E+06

Average viability [%]
76.81
51.264
8.307
1.575

SD [%]
3.517
3.897
4.354
0.428

PANC1_Epi

Concentration of NPs [ng/ml]
2.50E+05
5.00E+05
1.25E+06
2.50E+06

Average viability [%]
79.499
54.929
27.965
5.339

SD [%]
6.948
6.351
5.771
1.299

PANC1_NPs_Epi

Concentration of NPs [ng/ml]
2.50E+05
5.00E+05
1.25E+06
2.50E+06

Average viability [%]
81.874
45.271
1.909
1.777

SD [%]
3.87
3.47
0.555
0.284

A2780_Dau

Concentration of NPs [ng/ml]
2.50E+05
5.00E+05
1.25E+06
2.50E+06

Average viability [%]
35.542
60.621
60.422
54.259

SD [%]
5.641
4.390
8.988
4.656

A2780_NPs_Dau

Concentration of NPs [ng/ml]
2.50E+05
5.00E+05
1.25E+06
2.50E+06

Average viability [%]
28.381
42.996
40.073
43.611

SD [%]
6.746
8.623
14.150
12.369

AU565_Dau

Concentration of NPs [ng/ml]
2.50E+05
5.00E+05
1.25E+06
2.50E+06

Average viability [%]
12.13614
3.244951
1.544017
1.052948

SD [%]
0.876678
0.366567
0.521341
0.760732

AU565_NPs_Dau

Concentration of NPs [ng/ml]
2.50E+05
5.00E+05
1.25E+06
2.50E+06

Average viability [%]
11.13614
2.244951
1.344017
2.052948

SD [%]
0.876678
0.366567
0.521341
0.760732

HeLa_Dau

Concentration of NPs [ng/ml]
2.50E+05
5.00E+05
1.25E+06
2.50E+06

Average viability [%]
7.579
28.287
107.342
111.366

SD [%]
0.962
2.600
3.105
6.636

HeLa_NPs_Dau

Concentration of NPs [ng/ml]
2.50E+05
5.00E+05
1.25E+06
2.50E+06

Average viability [%]
13.776
34.299
83.013
98.005

SD [%]
2.282
4.639
9.485
2.638

MCF-7_Dau

Concentration of NPs [ng/ml]
2.50E+05
5.00E+05
1.25E+06
2.50E+06

Average viability [%]
23.086
25.325
40.867
69.450

SD [%]
6.812
5.820
4.646
3.975

MCF-7_NPs_Dau

Concentration of NPs [ng/ml]
2.50E+05
5.00E+05
1.25E+06
2.50E+06

Average viability [%]
20.980
20.504
29.155
61.507

SD [%]
3.062
3.368
4.225
8.928

OVCAR-3_Dau

Concentration of NPs [ng/ml]
2.50E+05
5.00E+05
1.25E+06
2.50E+06

Average viability [%]
71.147
120.518
94.253
99.822

SD [%]
5.825
8.619
8.962
7.221

OVCAR-3_NPs_Dau

Concentration of NPs [ng/ml]
2.50E+05
5.00E+05
1.25E+06
2.50E+06

Average viability [%]
60.560
83.543
82.286
75.566

SD [%]
2.852
6.593
12.896
7.598

Colo205_Dau

Concentration of NPs [ng/ml]
2.50E+05
5.00E+05
1.25E+06
2.50E+06

Average viability [%]
3.47
2.93
5.07
30.89

SD [%]
1.93
0.93
1.44
3.63

Colo205_NPs_Dau

Concentration of NPs [ng/ml]
2.50E+05
5.00E+05
1.25E+06
2.50E+06

Average viability [%]
19.95
3.06
2.82
85.11

SD [%]
2.48
0.26
0.28
4.61

PANC-1_Dau

Concentration of NPs [ng/ml]
2.50E+05
5.00E+05
1.25E+06
2.50E+06

Average viability [%]
33.21
0.54
1.02
95.12

SD [%]
3.51
0.09
0.48
5.16

PANC-1_NPs_Dau

Concentration of NPs [ng/ml]
2.50E+05
5.00E+05
1.25E+06
2.50E+06

Average viability [%]
54.42
23.38
2.76
94.94

SD [%]
3.38
3.77
0.94
6.91

ACHN_Dau

Concentration of NPs [ng/ml]
2.50E+05
5.00E+05
1.25E+06
2.50E+06

Average viability [%]
2.24
3.02
5.35
62.65

SD [%]
0.67
0.58
0.68
12.06

ACHN_NPs_Dau

Concentration of NPs [ng/ml]
2.50E+05
5.00E+05
1.25E+06
2.50E+06

Average viability [%]
22.85
1.12
1.23
66.26

SD [%]
5.58
0.28
0.11
10.10

A549_Dau

Concentration of NPs [ng/ml]
2.50E+05
5.00E+05
1.25E+06
2.50E+06

Average viability [%]
52.82
0.60
0.53
65.72

SD [%]
1.80
0.09
0.09
8.49

A549_NPs_Dau

Concentration of NPs [ng/ml]
2.50E+05
5.00E+05
1.25E+06
2.50E+06

Average viability [%]
54.55
14.77
1.34
80.73

SD [%]
4.09
2.22
0.98
0.71

Example 3

Determination of Anti-Tumour Efficacy of Anthracyclines Encapsulated with a Polysaccharide

A) Determination of a Maximum Tolerated Dose (MTD) for Dextran-Encapsulated Epirubicin (NPs-EPI)

The evaluation of acute toxicity of anthracycline encapsulated with a polysaccharide in the form of dextran-encapsulated epirubicin (NPs-EPI) as produced in Example 1 with MTD determination was performed using the acute oral toxicity—up-and-down procedure according to the OECD procedure no. 425 with a modification of the administration route of the test material.

Intravenous administration (i.v.; to the caudal vein) was dictated by how epirubicin in its currently used form, i.e. epirubicin hydrochloride (EPI), is administered to patents, and NPs-EPI will be administered if its anti-tumour efficacy is demonstrated.

The acute toxicity assessment method used is an alternative method recommended by the OECD (OECD procedure 425), which takes into account the aim to improve animal welfare and the 3Rs principle. (Replacement, Reduction, Refinement).

The higher-lower dose acute toxicity assessment procedure involves administering test material to an individual animal at a single dose lower than the expected median lethal dose (LD₅₀). Depending on the effect obtained following the administration of the first dose of the test or reference material, the next subject was administered a dose increased or reduced by a fixed coefficient. This procedure was continued sequentially until achieving a dose, the increase by which (by the established coefficient) caused death, and the decrease (by the established coefficient) resulted in the survival of the animal.

Following the determination of MTD for NPs-EPI (dextran-encapsulated epirubicin) in part A of the experiment, part B of the experiment was conducted to compare the acute toxicity and MTD of free EPI (in the form of epirubicin hydrochloride) at a dose equivalent to the dose of the drug contained in the combination thereof with NPs (EPI-NPs) at a dose constituting the MTD.

B) Comparative Assessment of Acute Toxicity and MTD of Free EPI at a Dose Equivalent to that of the Drug Contained in the Combination Thereof with NPs (NPs-EPI) at a Dose Constituting the MTD

Acute toxicity assessment of EPI at a dose equivalent to its content in the dose constituting the MTD of NPs-EPI (determined during the implementation of part A of the experiment) was carried out using the up-and-down method according to OECD procedure no. 425.

Dextran-encapsulated epirubicin (NPs-EPI) and epirubicin in free form, i.e. of epirubicin hydrochloride EPI were administered to mice once, to the caudal vein. Two hours before the administration of NPs-EPI and EPI, the animals were deprived of food. 30 minutes after the administration of NPs-EPI (test material) and EPI (reference material), the feed was again made available to the mice. The administration of another dose to the next animal took place after the result of the previous dose administration was obtained. The baseline dose of NPs-EPI contained the equivalent of 27.39 mg EP/kg bw (body weight) The EPI as reference material was administered at a dose of 30 and 31 mg/kg bw NPs-EPI and EPI were administered to mice in the form of aqueous solutions (water for injections) in volumes of no more than 0.18 cm³/mouse. The amount of the dose administered to the next animal depended on the result of administration of the previous dose. If the animal survived 48 hours after administration, the dose for the next animal was increased by a modified coefficient of more than 1 and less than 1.3 (coefficients 1.02; 1.05; 1.10 and 1.15 were used). If the animal died, the dose for the next subject was reduced by the same coefficient. The test material was administered until the dose was reached where 3 subsequent animals survived the administration of the highest dose. By OECD procedure no. 425, the recommended dose modification coefficient is 3.2, but due to the small difference between the minimum therapeutic dose and the MTD for the EPI, it was necessary to use a coefficient by which successive doses of the new formulation of said drug (NPs-EPI) were modified which was significantly less than 1.3 (not as provided for in the OECD 425). The method of individual coding animals was not known to persons who took care of the animals and performed the planned procedures being part of the study.

Accordingly, the maximum tolerated dose (MTD) for anthracycline NPs-EPI encapsulated with a polysaccharide for intravenous administration to mice was determined at 30 mg/kg bw (based on EPI) (90 mg/m²).

C) Determination of the Anti-Tumour Efficacy of Epirubicin Encapsulated in Dextran Nanoparticles in Ovarian Tumour

The subject of the study is to determine the anti-tumour efficacy and potential adverse effects of NPs-EP therapy versus the classical form of EPI in mice with implanted xenograft (ovarian tumour model). The study used epirubicin encapsulated in dextran nanoparticles (NPs-EPI) prepared according to Example 1. Epirubicin does not penetrate the blood-brain barrier, and it is eliminated in three stages. The biological half-life (t_1/2) is 15-45 h, approx. 40 h on average.

Obtaining a Tumour Study Model

To develop a tumour model, female mice from the CByJ.Cg-Foxn1<nu>/cmdb inbred strain were implanted OVCAR3 line ovarian tumour cells. Following anaesthesia, 5×10⁵ovarian tumour cells (OVCAR3 line cells) in the volume of 100 μl of PBS and Matrigel were subcutaneous (s.c.) injected into the right side of the female mice. During cell implantation, the animals did not experience any pain, as they were previously introduced into a state of mild inhalation narcosis using isoflurane.

After the tumour grew to the size of approx. 150 mm³, the mice were divided into 3 groups:

- K1/OVCAR3—control group A, which received water for injections;
- NPs/EPI/OVCAR3—the group which received epirubicin encapsulated with dextran nanoparticles (NPs-EPI) in the amount of 22.5 mg/kg bw (67.5 mg/m²)—test group B, and test group C which received NPs-EPI in the amount of 3.75 mg/kg bw (11.25 mg/m²);
- EPI/OVCAR3—reference group D, which received epirubicin in the standard form as epirubicin hydrochloride in the amount of 15 mg/kg bw (45 mg/m²).

All mice, except for the animals constituting the reference group, were treated with EPI encapsulated in dextran nanoparticles (NPs-EPI) or the standard form (EPI). During the treatment, the size of the tumours was measured, and the animals were closely observed. After the end of treatment, tumour measurements, haematological examinations, as well as macroscopic and histopathological examinations of internal organs and tumours were performed to allow the assessment of the efficacy and safety of using the NPs-EPI anti-tumour therapy in comparison to the standard form of the drug.

Procedures Performed on the K1/OVCAR3 Control Group (Administration of Water for Injection into the Caudal Vein)

Females with induced tumours, constituting the reference group (K1/OVCAR3), qualified for the anti-tumour efficacy assessment of NPs-EPI in a mouse model of ovarian tumour (OVCAR3 cell line), were administered water for injection every second day (10 administrations) into the caudal vein. Water for injection was administered (duration of single administration—30 seconds/mouse) at a volume of 0.18 cm³/mouse. During intravenous administration of water for injection, the animals did not experience any pain associated with the method of administration as the site of administration had previously been anaesthetised by spraying it with 10% lidocaine. The water for injection was administered 10 times. All mice in this group were sacrificed one day after the 10^thadministration of water for injection.

Procedure in the EP/OVCAR3 Test Group—Mouse Model of the Ovarian Tumour with Implanted OVCAR3 Line Cells

Female mice with induced tumours qualified for EPI/OVCAR3 anti-tumour efficacy assessment in a mouse model of ovarian tumour—the OVCAR3 cell line, EPI was administered into the caudal vein (application duration—30 seconds/mouse), once daily, every second day (2 administrations) at a dose equivalent to the drug content in a dose of 15 mg/kg bw EPI (½ MTD for epirubicin dextran nanoparticles) was administered to mice in the form of aqueous solutions in volumes of no more than 0.18 cm³/mouse. To administer the same dose of EPI to the animals, the animals were weighed before each administration, and the volume of the solutions administered was modified as a function of the change in body weight. During intravenous administration of EPI solutions, the animals did not experience any pain associated with the method of administration as the site of administration was anaesthetised by spraying it with 10% lidocaine.

Administration of NPs-EPI in the NPsEPI/OVCAR3 Test Group at Doses of 3.75 and 22.5 mg/kg bw in a Mouse Model of the Ovarian Tumour with Implanted OVCAR3 Line Cells

Female mice with induced tumours qualified for NPs-EPI anti-tumour efficacy assessment in the mouse model of ovarian tumour (OVCAR3 cell line) were administered NPs-EPI into the caudal vein once a day, every second day at doses of 3.75 mg/kg bw constituting ⅛, and 22.5 mg/kg bw constituting ¾ of the MTD for NPs-EPI administered to mice as aqueous solutions in volumes of no more than 0.18 cm³/mouse. To administer the same dose of NPs-EPI to the animals, the animals were weighed before each administration, and the volume of the solutions administered was modified as a function of the change in body weight. During intravenous administration of NPs-EPI solutions, the animals did not experience any pain associated with the method of administration as the site of administration had previously been anaesthetised by spraying it with 10% lidocaine.

The obtained results are presented in graphs in FIG. 4A and Band in the Tables 4-15 below.

TABLE 4

Body weight of the mice in the K1/OVCAR group during intravenous

administration of water for injection (detailed results).

Mouse
Body weight (g) before the subsequent administration/necropsy

Group
#
Before 1
Before 2
Before 3
Before 4
Before 5
Before 6

Injection
3
23.30
23.90
24.10
23.90
24.20
24.00

water
7
24.60
25.20
25.00
25.50
25.40
25.20

(group A)
14
23.00
23.60
23.50
23.50
23.30
23.00

28
21.40
21.90
22.20
22.20
21.90
21.60

30
24.20
25.10
25.60
25.40
25.20
25.40

33
23.50
23.50
23.30
23.60
23.70
23.30

Average ± SD
23.33 ± 1.12
23.87 ± 1.21
23.95 ± 1.23
24.02 ± 1.25
23.95 ± 1.30
23.75 ± 1.43

Body weight (g) before the subsequent administration/necropsy
Weight

Mouse

Before
gain

Group
#
Before 7
Before 8
Before 9
Before 10
necropsy
(g)

Injection
3
24.65
24.00
24.30
24.30
23.50
0.20

water
7
25.60
25.30
25.80
25.10
25.30
0.70

(group A)
14
23.75
23.10
23.75
23.50
23.40
0.40

28
22.15
21.50
22.10
22.00
21.50
0.10

30
25.40
25.60
25.85
25.70
26.00
1.80

33
23.80
23.30
24.10
24.40
23.80
0.30

Average ± SD
24.23 ± 1.28
23.80 ± 1.52
24.32 ± 1.40
24.17 ± 1.30
23.92 ± 1.58
0.58 ± 0.63

TABLE 5

Tumour size in mice in the K1/OVCAR group during intravenous administration of water for injection (detailed results)

Tumour volume (mm³) before subsequent administration/necropsy

Group
Mouse#
Before 1
Before 2
Before 3
Before 4
Before 5
Before 6
Before 7

Injection
3
165.14
174.13
165.01
166.79
153.79
145.27
137.96

water
7
201.10
224.27
295.36
239.06
255.51
263.93
301.04

(group A)
14
189.04
187.88
273.96
270.54
287.88
287.02
331.26

28
197.47
182.12
205.59
164.67
174.14
140.61
156.86

30
192.79
178.29
218.98
200.23
205.02
164.36
180.20

33
219.39
277.07
325.78
230.79
296.25
261.86
370.74

Average ± SD
194.16 ± 17.70
203.96 ± 40.11
247.45 ± 60.82
212.01 ± 42.27
228.77 ± 59.89
210.51 ± 67.26
246.34 ± 99.81

Volume of

Change in
the tumour

Tumour volume (mm³) before subsequent administration/necropsy
tumour
following

Before
volume
dissection

Group
Mouse#
Before 8
Before 9
Before 10
necropsy
(mm3)
(mm3)

Injection
3
131.00
172.48
175.32
136.32
−28.82
52.99

water
7
311.46
335.91
271.05
263.97
62.87
141.53

(group A)
14
322.54
415.94
331.26
356.99
167.95
174.53

28
154.08
149.65
147.70
126.88
−70.59
58.98

30
172.12
192.30
206.04
209.76
16.97
82.07

33
369.15
355.27
400.12
465.61
246.22
297.65

Average ± SD
243.39 ± 102.37
270.26 ± 112.20
255.25 ± 97.36
259.92 ± 132.09

134.63 ± 93.13

TABLE 6

Results of macroscopic observations during the necropsy

of the mice in the K1/OVCAR group, which was administered

water for injection (mouse no. 3)

External appearance

of the mouse
Skin thickness 0.30 mm

Organs
Macroscopic evaluation of internal organs

Liver
No visible changes

Left kidney
No visible changes

Right kidney
No visible changes

Adrenal glands
No visible changes

Spleen
No visible changes

Pancreas
No visible changes

Lung
No visible changes

Heart
No visible changes

Thymus
No visible changes

Intestines
Intestines filled with green food content, the

content prevents an accurate assessment of the

mucous membrane

Stomach
No visible changes

Reproductive organs
No visible changes

Bladder
No visible changes

Brain
No visible changes

Tumour
5.40 mm × 4.43 mm in size in the subcutaneous

tissue, immobile about the skin.

TABLE 7

Body weight of the mice from the NPsEPI/OVCAR3 group during intravenous

administration of NPs-EPI at a dose of 3.75 mg/kg bw (detailed results)

Weight (g)
Weight

Mouse
Before 1st
Before 2nd
Before 3rd
Before 4th
Before
loss

Group
#
administration
administration
administration
administration
necropsy
(g)

EP-NPs 3
17
23.00
22.80
22.50
20.50
19.00
4.00

3.75 mg/kg bw
18
23.50
22.60
22.20
20.10
18.40
5.10

(group C)
19
23.50
22.60
22.60
21.40
19.60
3.90

20
24.20
23.30
23.10
21.50
19.10
5.10

22
22.60
22.10
21.80
20.80
18.00
4.60

34
25.00
24.50
23.30
22.85
21.40
3.60

38
20.50
20.30
20.40
19.15
17.00
3.50

Average ± SD
23.19 ± 1.42
22.60 ± 1.27
22.27 ± 0.97
20.90 ± 1.18
18.93 ± 1.38
4.26 ± 0.68

TABLE 8

Tumour size in the mice from the NPsEPI/OVCAR3 group during intravenous

administration of NPs-EPI at a dose of 3.75 mg/kg bw (detailed results).

Tumour volume (mm3) before/after subsequent administration

Percentage
Volume of

Before
Before
Before
Before

Change in
change in
the tumour

1st
2nd
3rd
4th
One day
tumour
tumour
following

Mouse
adminis-
adminis-
adminis-
adminis-
after 4th
volume
volume
dissection

Group
#
tration
tration
tration
tration
administration
(mm3)
(%)
(mm³)

EP-NPs
17
138.40
110.88
107.01
100.32
93.86
−44.54
32.18
84.79

in dose
18
162.50
160.99
150.13
145.76
143.01
−19.49
11.99
101.79

3.75 mg/kg bw
19
177.77
172.05
161.94
153.15
150.83
−26.94
15.15
156.31

20
126.90
108.02
98.20
83.33
59.70
−67.20
52.95
71.65

22
154.70
150.93
144.87
140.82
129.58
−25.12
16.24
123.02

34
153.42
139.71
129.42
124.97
108.87
−44.55
29.04
95.78

38
128.72
150.08
140.72
122.30
109.35
−19.37
15.05
95.33

Average ± SD
148.92 ±
141.81 ±
133.18 ±
124.38 ±
113.60 ±
−25.54 ±
24.66
104.10 ±

18.59
24.28
23.20
25.24
1.20
13.31

27.87

TABLE 9

Results of macroscopic observations during necropsy

of the NPsEPI/OVCAR3 group that received NPs-EPI

at a dose of 3.75 mg/kg bw (mouse #17).

External appearance
Anal area dirty with faeces, mouse

of the mouse
is cachectic, skin 0.30 mm thick

Organs
Macroscopic evaluation of internal organs

Liver
No visible changes

Left kidney
No visible changes

Right kidney
No visible changes

Adrenal glands
No visible changes

Spleen
1.5 cm × 0.4 cm × 0.2 cm in size

(probably reduced)

Pancreas
No visible changes

Lung
No visible changes

Heart
No visible changes

Thymus
No visible changes

Intestines
Large intestine filled with liquid food content,

the content prevents an accurate assessment of

the mucous membrane

Stomach
No visible changes

Reproductive organs
No visible changes

Bladder
No visible changes

Brain
No visible changes

Tumour
7.58 mm × 4.73 mm in size in the subcutaneous

tissue, immobile about the skin.

TABLE 10

Body weight of the mice from the NPsEPI/OVCAR3 group during intravenous

administration of NPs-EPI at a dose of 22.50 mg/kg bw (detailed results).

Weight (g)

Two

Weight

Mouse
Before 1st
Before 2nd
Before 3rd
days after 3rd
Before
loss

Group
#
administration
administration
administration
administration
necropsy
(g)

EP-NPs
4
24.90
23.40
22.90
20.20
18.61***
6.29

in dose
10
24.50
23.10
21.40
19.40
17.50***
7.00

22.5 mg/kg bw
13
23.20
21.80
20.10
17.60
15.90***
7.30

(group B)
21
24.50
23.30
22.20
21.40
19.60
4.90

26
22.70
21.80
21.40
19.90
18.30***
4.40

35
22.90
22.10
21.00
19.40
18.30
4.60

37
23.80
23.60
21.50
18.80
17.30***
6.50

39
21.20
20.70
18.30
15.30
14.40***
6.80

Average ± SD
23.46 ± 1.22
22.48 ± 1.03
21.10 ± 1.40
19.00 ± 1.85
17.49 ± 1.65
5.97 ± 1.16

***weight of the mouse before the necropsy

TABLE 11

Tumour size in the mice from the NPsEPI/OVCAR3 group during intravenous

administration of NPs-EPI at a dose of 22.5 mg/kg bw (detailed results).

Tumour volume (mm3) before/after subsequent administration

Percentage
Volume of

Before
Before
Before
One day
Two day
Change in
change in
the tumour

1st
2nd
3rd
after 3rd
after 3rd
tumour
tumour
following

adminis-
adminis-
adminis-
adminis-
adminis-
volume
volume
dissection

Group
Mouse #
tration
tration
tration
tration
tration
(mm³)
(%)
(mm³)

Tumour volume
4
154.67
198.95
112.71
61.82
91.30
−63.37
40.97
44.72

(mm³) before/after
10
160.12
212.24
118.50
102.29
97.12
−63.00
39.35
30.80

subsequent
13
155.36
225.70
134.31
105.40
105.32
−50.04
32.21
83.40

21
179.56
196.14
145.54
117.83
97.49
−82.07
45.71
105.12

26
152.73
184.59
112.33
104.39
96.39
−56.34
36.89
49.30

35
149.88
174.37
82.74
85.67
73.26
−76.62
51.12
26.27

37
176.02
188.07
156.66
114.05
132.35
−43.67
24.81
59.37

39
173.46
225.17
133.92
154.87
145.93
−27.53
15.87
67.75

Average ± SD
162.73 ±
200.65 ±
124.59 ±
105.79 ±
104.90 ±
−56.94 ±
35.87
58.34 ±

11.75
18.87
23.08
26.66
23.33
20.65

26.62

TABLE 12

Results of macroscopic observations during necropsy of the mouse

no. 4 which received NPs-EPI at a dose of 22.5 mg/kg bw

External appearance
Anal area dirty with faeces, mouse

mice
is cachectic

Organs
Macroscopic evaluation of internal organs

Liver
On the surface of the liver, there are many

cream-colour changes, the size of a pinhead

Left kidney
No visible changes

Right kidney
No visible changes

Adrenal glands
No visible changes

Spleen
Dark cherry colour (slightly darker)

Pancreas
No-visible changes

Lung
No visible changes

Heart
No visible changes

Thymus
No visible changes

Intestines
The intestines are filled with cream-like

gastro intestinal contents,which content

prevented an accurate assessment of the

mucous membrane

Stomach
No visible changes

Reproductive organs
No visible changes

Bladder
No visible changes

Brain
No visible changes

Tumour
6.16 mm × 3.81 mm in size in the subcutaneous

tissue, immobile about the skin.

TABLE 13

Body weight of the mice from the EPI/OVCAR3 group during intravenous

administration of EPI at a dose of 15 mg/kg bw (detailed results).

Weight (g)

Before 1st
Before 2nd
Before
Weight loss

Group
Mouse #
administration
administration
necropsy
(g)

EP in a dose
5
23.80
23.65
20.55
3.25

of 15 mg/kg bw
15
25.90
22.45
22.30
3.60

(group D)
24
23.80
23.10
22.25
1.55

29
24.00
24.30
20.35
3.65

31
23.10
22.45
20.60
2.50

32
21.90
21.40
19.00
2.90

76
22.30***
—
—
—

82
21.80
21.25
18.40
3.40

Average ± SD
23.33 ± 1.36
22.66 + 1.12
20.49 ± 1.47
2.98 ± 0.75

***- the weight of the mouse before the necropsy

TABLE 14

Tumour size in the mice from the EPI/OVCAR3 group during intravenous administration of EPI at a dose of 15 mg/kg bw (detailed results).

Tumour volume (mm³)

Percentage

One
Two
Change in
change in
Volume of the

Mouse
Before 1st
Before 2nd
day after 2nd
days after 2nd
tumour
tumour
tumour following

Group
#
administration
administration
administration
administration
volume (mm³)
volume (%)
dissection (mm³)

EP-NPs
5
100.29
90.06
87.07
86.25
−14.04
−14.00
73.37

in dose
15
164.36
160.79
155.78
135.44
−28.92
−17.60
85.22

15 mg/kg bw
24
138.93
146.21
143.57
145.58
6.65
+4.79
98.45

(group D)
29
116.49
106.88
103.86
119.24
2.75
+2.36
67.46

31
121.68
123.19
120.51
103.15
−18.53
−15.23
58.06

32
100.05
114.78
110.86
105.54
5.49
+5.49
65.33

82
139.54
128.92
124.62
98.95
−40.59
−29.09
48.97

76^θ
107.13
—
—
—
—

47.01

Average ± SD
125.91 ± 23.33
124.40 ± 23.81
120.90 ± 23.38
113.45 ± 21.09

67.98 ± 17.57

* mouse died directly after EPI administration

TABLE 15

Results of macroscopic observations during necropsy

of a mouse from the EPI/OVCAR3 group which received

EPI at a dose of 15 mg/kg bw (mouse #5).

External appearance
Anal area dirty with faeces, mouse

of the mouse
is cachectic, skin 0.21 mm thick

Organs
Macroscopic evaluation of internal organs

Liver
Liver surface colour dark cherry to brown,

consistency softer than normal, blood vessels

highly filled with blood

Left kidney
Consistency softer than normal

Right kidney
Consistency softer than normal

Adrenal glands
No visible changes

Spleen
1.6 cm × 0.4 cm × 0.1 cm in size,

slightly smaller, dark brown in colour

Pancreas
No visible changes

Lung
No visible changes

Heart
No visible changes

Thymus
No visible changes

Intestines
Intestines filled with green food content, the

content prevents an accurate assessment of the

mucous membrane

Stomach
No visible changes

Reproductive organs
No visible changes

Bladder
No visible changes

Brain
No visible changes

Tumour
5.80 mm × 5.03 mm in size in the subcutaneous

tissue, immobile about the skin.

EPI administration to the mice from the EPI/OVCAR3 group resulted in the death of the mice a soon as on the 4th day after the first administration of the drug (after the second administration), one mouse died directly following the first administration of EPI, while the mice from the NPs/EPI/OVCAR3 group which received NPs-EPI in both concentrations survived to the end of the experiment.

Mice from the EPI/OVCAR3 group which received EPI exhibited severe inflammation and changes in the structure of the liver, as well as changes in the colour and structure of the spleen compared to the K1/OVCAR control group. Such changes were not observed in the NPsEPI/OVCAR3 group, which received NPs-EPI. Pure drug results in significant damage to local blood vessels, liver damage and the need to sacrifice the animals due to cachexia, which is not observed for epirubicin administered in the form encapsulated with a polysaccharide.

A significant decrease in the size of the induced ovarian tumour is observed in the mice from the NPsEPI/OVCAR3 group which received NPs-EPI in both concentrations (FIGS. 4 A and B) compared to the size of tumours in the control group, with an increased decrease in tumour size observed when administering a higher dose of NPs-EPI.

Surprisingly, it was found that the use of an anthracycline encapsulated with a polysaccharide instead of its non-encapsulated form, e.g. NPs-EPI instead of EPI, reduces the drug toxicity sufficiently (despite not being a form of drug with an attached target cell targeting factor) to allow for intravenous administration of a higher dose of the drug and achieving a faster reduction of tumour volume.

Example 4

Comparison of Anti-Tumour Efficacy, Safety, Side Effects of the Therapy Using Encapsulated Epirubicin NPs-EPI and EPI in Free Form in a Mouse Ovarian Tumour Model with Implanted OVCAR3 Line Cells

By Example 1, dextran nanoparticles NPs were prepared without epirubicin, nanoparticles with epirubicin encapsulated into dextran nanoparticles (NPs-EPI). The administration protocol was changed compared to Example 3 to administer the dose of EPI or NPs-EPI every 3 days in an amount based on epirubicin 10 mg/kg bw or administer NPs as a control. Following Example 3, mice were obtained constituting an ovarian tumour test model, which were divided into 3 groups.

L—control group injected with NPs;

J—the test group which received epirubicin encapsulated in dextran nanoparticles (NPs-EPI) in the amount of 10 mg/kg bw

K—the test group which received epirubicin in the form of epirubicin hydrochloride in the amount of 10 mg/kg bw

The results obtained in the form of the size of tumour changes in individual mice and the average tumour volume are presented in Tables 16 and 17 below.

TABLE 16

Changes in tumour volume after subsequent administrations of NPs-EPI, EPI and NPs to mice.

Volume of

the tumour
Percentage change in tumour volume (%)

Mouse
before 1st
Before 2nd
Before 3rd
Before 4th
Before 5th

Group
#
administration
administration
administration
administration
administration

NPs
132
112.33

↑ 4.44% ^E
↑ 18.20%
↑ 22.01%
↑ 26.25%

380 mg/kg bw
146
104.97
↑ 3.89%
↑ 3.44%
↑ 6.24%
↑ 9.40%

(group L)
147
100.36
↑ 30.70%
↑ 34.45%
↑ 35.12%
↑ 36.22%

153
105.89

↓ 1.51% ^E
↑ 65.82%
↑ 82.17%
↑ 102.04%

156
104.14
↓ 0.87%
↓ 1.83%
↓ 0.41%
↑ 2.44%

163
118.69
↑ 13.31%
↑ 24.80%
↑ 39.27%
↑ 59.73%

NPs-EPI
136
254.35
0.00%
↑ 7.38%
↑ 8.17%
—

10 mg/kg bw
140
187.30
↓ 2.22%
↓ 7.17%
— ^F
—

(group J)
143
176.60
↓ 1.50%
↓ 18.71%
↓ 17.15%
—

152
162.03
↑ 7.39%
↑ 16.56%
↑ 8.46%
—

157
163.08
↑ 3.93%
↓ 7.67%
↓ 3.94%
—

158
158.37
↓ 5.64%
↓ 12.64%
↓ 21.46%
↓ 29.75%

159
172.90
↓ 12.34%
↓ 13.02%
↓ 21.31%
↓ 41.97%

160
173.02
↓ 6.38%
↓ 18.84%
↓ 34.53%
—

164
179.25
↓ 22.52%
↓ 22.64%
↓ 26.20%
↓ 21.76%

NPs
131
134.37
↑ 0.26%
↓ 9.02%
—
—

10 mg/kg bw
142
157.38
↓ 14.33%
↓ 9.58%
—
—

(group K)
148
137.41
↑ 7.21%
↓ 28.86%
—
—

149
136.13
↓ 8.76%
↓ 20.03%
—
—

162
150.89
↑ 53.65%,
↑ 40.73%
—
—

165
145.19
↓ 17.56%
↓ 29.43%
—
—

Volume of

Percentage change in tumour volume (%)
the tumour

Mouse
Before 6th
Before 7th
Before
before the

Group
#
administration
administration
necropsy
necropsy (mm³)

NPs
132
↑ 27.99%
↑ 31.14%
↑ 115.96% ^G

242.59 ^G

380 mg/kg bw
146
↑ 11.14%
↑ 16.48%
↑ 73.44%
182.07

(group L)
147
↑ 21.82%
↑ 29.92%
↑ 50.35%
150.89

153
↑ 174.10%
↑ 336.91%
↑ 498.42%
633.67

156
↑ 2.86%
↑ 5.01%
↑ 56.78%
163.27

163
↑ 66.85%
↑ 72.42%
↑ 209.38%
367.20

NPs-EPI
136
—
—
↑ 5.33% ^H

267.91 ^H

10 mg/kg bw
140
—
—
↓ 11.71%
165.37

(group J)
143
—
—
↓ 5.83%
166.30

152
—
—
↓ 3.04%
157.11

157
—
—
↑ 19.18%
194.36

158
↓ 33.66%
↓ 27.12%
↓ 21.56%
124.23

159
↓ 42.37%
↓ 36.59%
↓ 33.65%
114.72

160
—
—
↓ 43.54%
97.69

164
—
—
↓ 30.80%
124.05

NPs
131
—
—
↓ 34.62% ^I
87.85 ^I

10 mg/kg bw
142
—
—
↓ 20.82%
124.62

(group K)
148
—
—
↓ 33.27%
91.69

149
—
—
↓ 24.10%
103.33

162
—
—
↑ 57.69%
237.94

165
—
—
↓ 30.24%
101.28

^Epercentage increase (↑) or decrease (↓) in tumour volume compared to the volume before the commencement of administration

^Fthe mouse was sacrificed earlier for humanitarian reasons

^Gfollowing 12 administrations in all animals in the group

^Hfollowing 3 to 7 administrations in all animals in the group

^Iafter 3 administrations in all animals in the group

TABLE 17

Comparison of changes in average tumour volume after subsequent

administrations of NPs-EPI, EPI and NPs to mice.

Average tumour volume (mm³)

Before 1^st
Before 2^nd
Before 3^rd
Before 4^th

Group
administration
administration
administration
administration

NPs
107.73 ± 6.63
116.59 ± 13.57
133.71 ± 26.78
141.02 ± 33.43

(group L)

↑ 8.22% ^J
↑ 24.12%
↑ 30.90%

NPs-EPI
180.77 ± 29.08
172.98 ± 33.61
166.42 ± 43.60
157.47 ± 51.33

10 mg/kg bw

↓ 4.31% ^J
↓ 7.94%
↓ 12.89%

(group J)

EPI
143.56 ± 9.22
148.77 ± 41.82
131.00 ± 42.96
— ^K

10 mg/kg bw

↑ 3.63%
↓ 8.75%

(group K)

Average tumour volume (mm³)

Before 5^th
Before 6^th
Before 7^th
Before

Group
administration
administration
administration
necropsy

NPs
150.60 ± 42.45
163.01 ± 70.31
196.10 ± 134.75
289.95 ± 186.21

(group L)
↑ 39.79%
↑ 51.31%
↑ 82.03%
↑ 169.15% ^G

NPs-EPI
117.28
102.35
112.53
156.86 ± 51.62

10 mg/kg bw
↓ 35.12%
↓ 43.38%
↓ 37.75%
↓ 13.23% ^H

(group J)

EPI
—
—
—
124.45 ± 57.05

10 mg/kg bw

↓ 13.31% ^I

(group K)

^Gfollowing 12 administrations in all animals in the group

^Hfollowing 3 to 7 administrations in all animals in the group

^Iafter 3 administrations in all animals in the group

^Jpercentage increase (↑) or decrease (↓) in average tumour volume compared in the group to the volume before the commencement of administration

^Kall mice from the group were sacrificed earlier for humanitarian reasons

The results presented indicate that epirubicin encapsulated in dextran nanoparticles (NPs-EPI) has greater anti-tumour efficacy and less pronounced adverse effects than EPI. The higher toxicity of EPI is also demonstrated by the fact that as soon as following 3 administrations of drug doses, body weight decreased by 22.55% on average, while during the entire NPs-EPI treatment (3-7 doses), the body weight of the animals decreased by an average of 11.37%.

Thus, administration of NPs-EPI improves and prolongs the total survival time.

The analysis of average change in tumour volume showed that in animals treated with NPs-EPI, the tumours decreased on average by 4.31% as soon as after the administration of the first dose, while in animals receiving EPI during the same period the tumour was observed to increase by 3.63% on average. During the administration of NPs-EPI, increased efficacy was observed over time, which may confirm the gradual release of the drug from dextran nanoparticles. Microscopic images of internal organs indicated lower toxicity of NPs-EPI at a dose of 10 mg/kg bw versus the equivalent dose of EPI (Table 18).

TABLE 18

Appearance

of the organ
NPs-EPI at a dose of 10 mg/kg bw
EPI at a dose of 10 mg/kg bw

Liver
Hyperaemia, features of
Hyperaemia, features of hepatocyte

hepatocyte feathery degeneration
feathery degeneration, focal necrosis

of hepatocytes

Reproductive
Moderate changes,
Severe lesions, endometrial hypertrophy,

organs
lymphocytes in the myometrium
cystic lesions, the growth of Leydig cells

within the ovary

Tumour
anaplastic lesions,
anaplastic lesions, moderate tumour necrosis

pronounced tumour necrosis

NPs-EPI administration observably resulted in increased survival of the mice, which allowed for the administration of the drug over a longer time, indicating that the encapsulation of EPI into polysaccharide nanoparticles improves the treatment efficacy with decreased toxicity.

The use of drugs from the group of anthracyclines, preferably epirubicin, daunorubicin, doxorubicin, idarubicin in the form of nanoparticles encapsulated with a polysaccharide, in particular, nanoparticles of epirubicin, daunorubicin, doxorubicin, idarubicin encapsulated with dextran reduces the toxicity of these compounds. The encapsulation of these anthracyclines with dextran allows for administering a higher intravenous dose of the drug, such as epirubicin, as demonstrated in tissue cultures of various tumours, the treatment of which uses these anthracyclines, as well as in a mouse model of ovarian tumour.

Due to similar curves of effect on tissue cultures of breast tumour, cervical cancer, ovarian cancer, pancreatic tumour, kidney tumour, lung tumour, colorectal tumour cancer lines obtained for epirubicin, daunorubicin, doxorubicin, idarubicin encapsulated both with dextran and other polysaccharides, which in the new form reduce toxicity of said drugs to the body (with the mechanism thereof not being clear, as these are particles without targeting particles attached), similar results of increased drug efficacy combined with reduced systemic toxicity with the possibility of administering a higher dose of the drug are obtained for epirubicin, daunorubicin, doxorubicin, idarubicin encapsulated with both dextran and other polysaccharides: cellulose and its derivatives, amylose, starch and heparin.

Surprisingly, it was found that the new form of anthracycline administration in the form of epirubicin, daunorubicin, doxorubicin, idarubicin encapsulated with a polysaccharide, particularly epirubicin encapsulated with dextran, allows for achieving a therapeutic effect while using lower doses of the drug, and it also allows for administering higher doses of the drug, longer therapy due to their reduced toxicity to the body, which provides improved efficacy of tumour treatment. Pure drug results in significant damage to local blood vessels, liver damage, as observed in an animal model, since in an exemplary EPI study it was necessary to sacrifice the animals due to cachexia much earlier than when administering NPs-EPI.

What is very promising is not only the unexpected achievement of the effect of reduced drug toxicity, but also the possibility of using encapsulated epirubicin, particularly encapsulated with dextran, to treat pancreatic tumour (observed significantly increased toxicity for PNAC1 cells—FIG. 3 G.), in which treatment, according to the art, this chemotherapeutic agent was completely ineffective despite the attempts made.

LITERATURE

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[205] http://www.thermofisher.com/pl/en/home/references/protocols/cell-culture/mtt-assay-protocol/vybrant-mtt-cell-proliferation-assay-kit.htm

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ANTHRACYCLINE ENCAPSULATED WITH A POLYSACCHARIDE FOR USE IN THE TREATMENT OF TUMOURS

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