ES2367190B1 - MULTIFUNCTIONAL Nanostructures AS MRI-SPECT BIMODAL DIAGNOSIS AGENTS. - Google Patents

Abstract

Multifunctional nanostructures as MRI-SPECT bimodal diagnostic agents. # Multifunctional nanostructures consisting of superparamagnetic magnetoferritin, which can also comprise chains of a biocompatible polymer covalently bonded to its surface. The invention also relates to a method for obtaining said nanostructures, as well as their use as a medicament and more preferably for the diagnosis of cancer or as a contrast agent.

Description

Multifunctional nanostructures as bimodal diagnostic agents MRI-SPECT.

The present invention refers to a multifunctional nanostructure, specifically a superparamagnetic magnetoferritin, in addition to its application as a contrast agent in MRI or SPECT. Therefore, the invention could be framed within the field of biomedicine.

State of the art

The integration of Nanotechnology into Biotechnology has made a new discipline flourish: Nanomedicine. In this field, metal nanoparticles are designed and prepared to obtain bio-images through the simultaneous use of several techniques, effective distribution of drugs or techniques of promising therapies such as hyperthermia caused locally by magnetic nanoparticles. It is an area of tremendous potential subject to the development of new nanostructures for its advancement.

Magnetic nanoparticles have attracted attention primarily because of their potential use as contrast agents in Magnetic Resonance Imaging (MRI). This technique is based on the magnetic resonance of the protons of body tissues (water, membranes, lipids, proteins, etc.) and is currently the most powerful method of diagnosis.

The contrast in MRI can be improved with paramagnetic substances. The ability of a compound to increase the relaxation rate of proton spins of surrounding water molecules is called relaxation and is defined as R1∼1 / T1 or R2∼1 / T2. Superparamagnetic nanoparticles are candidates to act as contrast agents in MRI. Like paramagnetic substances, they lose their magnetization when the external magnetic field is removed, but unlike them, their magnetization is significantly higher. Therefore, the relaxation they produce is much higher than those of the classic paramagnetic complexes of Gd (III). The effect of superparamagnetic nanoparticles can be described based on the heterogeneity of the intense magnetic field that affects the surrounding protons, inducing a lag of the magnetic moment and resulting in a shortening of the relaxation time T2. Thus, superparamagnetic nanoparticles are good candidates for the development of new and elegant contrast agents, allowing early detection of severe pathologies and great social impact.

One approach within Nanomedicine is the use of nanoparticles that can simultaneously combine different bioimaging techniques. Each bioimaging modality has its own merits but also certain disadvantages and therefore multimodal imaging methods have a greater capacity to obtain a comprehensive and more detailed image.

MRI, probably the most powerful imaging technique today, has a high spatial resolution but nevertheless does not have great sensitivity (10-5 M, with current technology) and requires accumulating significant concentrations of the contrast agent, which increases the toxicity risk However, OI has an extraordinary sensitivity (10-12 M) but on the contrary it presents problems of spatial resolution and low tissue penetration. In short, the challenge is to combine the strengths of each imaging technique into a single contrast agent, which allows parallel images to be obtained using several techniques. Although there are still no multimodal contrast agents for routine clinical use, a good number of them have been published, especially MRI-OI bimodal.

A key point for the in vivo biomedical application of metal nanoparticles is that they cannot be toxic and must remain in the bloodstream long enough to reach a biological target. The immune system through the opsonin, macrophage and antibody components (MPS, mononuclear phagocytic system) recognizes and removes particles from the bloodstream, with their simultaneous concentration in organs with high phagocytic activity (mainly the liver). Therefore, a sensible strategy is the use of nanoparticles that are able to evade the attack by the MPS and are not phagocytosed by macrophages, consequently increasing the half-life in plasma and allowing to reach a specific organ or tissue.

An ideal bimodal agent for clinical application should have a high and specific accumulation in the appropriate cells, which would result in the possibility of diagnosing an even treatable disease more and more early, in addition to having enough half-life in plasma sufficiently high and be able to reach a specific biological target. In this sense, the use of metal nanoparticles against classical metal compounds (salts or coordination compounds) has the advantage of being able to more easily accumulate a greater amount of active metal material in a given tissue. This means that the use of the drug is optimized in a definitive manner and that the necessary metal dose can be reduced, with the consequent decrease in the risk of toxicity.

Numerous physical and chemical methods have been used to prepare magnetic nanoparticles. Since the magnetic properties are very dependent on size, it is crucial that the method to be developed allows the obtaining of nanoparticles with uniform sizes. A possible route to obtain metallic nanoparticles without aggregation and with controlled size is the use of a pre-organized molecular platform, with a cavity that can act as a nanoreactor for chemical and spatial control in the formation of nanoparticles. A typical example of this type of molecules is the ferritin protein. Apoferritin consists of a spherical protein formed by 24 subunits surrounding an aqueous cavity with a diameter of approximately 8 nm.

The organization of multisubunities to form apoferritin generates the presence of channels. Eight hydrophilic channels of approximately 4 ˚

A allows the entry of metal ions and sufficiently small molecules into the cavity of the protein. This has allowed the introduction of magnetite into the apoferritin producing magnetoferritin, which has been used as a single-mode diagnostic method (MRI) (Journal of Magnetic Resonance Imaging. 4 (3): 497-505, 1994 May-Jun. ).

On the other hand, the use of 99mTcO4 - for diagnosis by SPECT scintigraphy (Single Photon Emission Computer Tomography) is widely used in Nuclear Medicine. The 99mTcO4 - has a short half-life (6 h) and emits gamma radiation of 141 keV. These values reduce its toxicity and make it an ideal radionuclide for contrast agent using SPECT. In fact, in the market there are a good number of drugs of this radionuclide (Ceretec®, Tc-MAG®, Cardiolite®, etc.), most of which are in the form of a complex of Tc of different oxidation states and which are obtained in situ by reaction with different ligands (Chem. Rev. 1999, 99, 2205; Chem. Rev. 1999, 99, 2235). The majority of Tc compounds are coordination compounds or salts, with some known trade names: cardiolite ® (for heart), Tc-MAG ® (for kidney), etc. US 20090035201 describes an example of a 99mTcO4 −-Fe2O3 complex, but does not address the issue of the inclusion of such complexes in the magnetoferritin cavity, and even less the use of the final product as a bimodal contrast agent.

Detailed description of the invention

In view of the state of the art, an objective of the present invention is to provide a bimodal contracting agent, MRI-SPECT, based on a superparamagnetic magnetoferritin, characterized in that the magnetite core occludes 99mTc, from now on magnetoferritin of the invention.

The superparamagnetic nanoparticle of the invention, that is, the superparamagnetic magnetoferritin, is constituted by a magnetite nanoparticle encapsulated in the ferritin that has properties to behave as a contrast agent in MRI.

The magnetoferritin of the invention is biocompatible and has a biodistribution in different organs, significantly improving the properties of other contrast agents such as magnetite alone. This can be used as a bimodal contrast agent in MRI (i), and SPECT-scintigraphy (iv) and shows half-life in blood, especially when biocompatible polymer chains such as polyethylene glycol (PEG) have been introduced, sufficiently long to distribute by the circulatory system without being phagocytosed in a time less than 3 h.

Other advantages of the magnetoferritin of the present invention is that the preparation of these 99mTcO4 nanoparticles - is carried out at room temperature at an optimal time for injection into the body. In addition it does not require reduction of Tc (VII) and its incorporation into the nanoparticle is practically total, which allows an optimal accumulation of the radionuclide. The fact that the pertecnectate is occluded in the Fe ore network makes it possible to control the amount of 99mTcO4 - per particle and therefore, drugs of different doses of radionuclide can be prepared, depending on the needs.

The preferred Tc species for inclusion in the magnetoferritin of the invention is 99mTcO4 -. The concentration of 99mTc can be adjusted according to need, for example diagnosis or therapy but preferably is between 10−9-10-5 M.

The present inventors have managed to obtain magnetite particles of high Fe content in the ferritin cavity. The Fe content can be modulated up to 3800 Fe atoms per unit of ferritin. Preferably, the amount of Fe from 3000 to 3800 Fe atoms per unit of ferritin is modulated, which makes it possible to improve its properties as a contrast agent in MRI.

During the preparation of the magnetite nanoparticle (i), the Tc is occluded within the magnetite, which is an advantage over the coordination complexes of Tc since the concentration of Tc per particle is much higher (up to 20 times higher ) and allows to accumulate a higher density of Tc atoms. This greater accumulation results in an increase in gamma radiation and a higher resolution. Also, the accumulation optimizes the concentration of the radiolabel, which allows the use of lower doses.

According to a preferred embodiment of the present invention the superparamagnetic magnetoferritin has chains of a biocompatible polymer covalently bonded to the surface of the magnetoferritin. The presence of this polymer improves the properties of the magnetoferritin of the invention to be used as a contrast agent since it increases its overall stability, obtaining adequate average life times in the blood for use. The preferred biocompatible polymer is polyethylene glycol (PEG), among other reasons for its industrial availability, its ease of incorporation into the surface of the magnetoferritin and its high biocompatibility. The process of covalently bonding the PEG polymer to other molecules, usually drugs or therapeutic proteins, is known as PEGylation (Kohler, N .; Fryxell, GE; Zhang, MJ Am. Chem. Soc. 2004, 126, 7206. Paul, KG ; Frigo, TB;

Groman, J. Y .; Groman, E. V. Bioconjugate Chem. 2004, 15, 394.). In our case, PEG is covalently linked to magnetoferritin. This process can be carried out easily, by incubating a derivative of the reactive PEG with the nanoparticles. The covalent union of PEG masks them of the immune system, increases hydrodynamic size (size in solution) which increases the half-life in blood and reduces their elimination by the immune system. This process also increases the water solubility of said nanoparticles and generally gives it additional stability. The number of PEG molecules that bind to the surface of the superparamagnetic nanoparticle can also be controlled. PEG derivatives of the succinimidyl ester type allow the formation of an amide type covalent bond by reaction with the amino groups on the outer surface of the superparamagnetic nanoparticles. In summary, to achieve the union of the PEG chains and the magnetoferritin, the PEG must be derivatized with functional groups capable of binding on their own or with the aid of a reagent to the surface of the magnetoferritin. The PEG is preferably linked by amide bonds, therefore the preferred PEG derivatives, as discussed above, contain the succinimidyl ester functional group, which allows direct functionalization of the magnetoferritin, since this activated ester group It reacts with the amino groups surrounding the nanoparticles, forming the covalent bond type amide. One of the preferred PEGs is PEG1163 MeO-PEG-COO-Su α-Methoxy-ω-carboxylic acid succinimidyl ester poly (ethylene glycol) PEG-WM 2,000 Dalton. PEGs functionalized as succinimidyl ester are commercial and their covalent coupling to the superparamagnetic particle can be carried out after the introduction of 99mTc.

The number of PEG chains introduced can be controlled depending on the stoichiometry and PEG used. For example, when activated ester derivatives are used, given the high reactivity of said esters and the amines of the superparamagnetic nanoparticle, the reaction is complete, such that the number of PEG covalently linked to the surface of the nanoparticle coincides with the number of molecules of the PEG derivative / nanoparticles that is used in the reaction. In addition, the number of chains introduced was checked through the use of an electrophoretic pattern, analyzing the different magnetoferritins derivatized with PEG and seeing their correspondence with a stepped and gradual increase in molecular weight and therefore a greater retention. The PEG can be mono-or bifunctionalized with activated esters and PEG with different density and crystallinity can be attached. The magnetoferritin stability of the invention is enhanced by the introduction of the biopolymer, and especially when this is PEG, but this greater increase in stability is not proportional to the number of chains introduced. Therefore, although between 1 and 72 chains can be introduced, free amino groups can be left if subsequent derivations are desired or simply to reduce manufacturing costs. Preferably, between 3 and 10 PEG chains are incorporated per magnetoferritin and more preferably between 4 and 6.

Here are some of the PEG derivatives useful for the present invention:

i) MeO-PEG-COOH: PEG1156 MeO-PEG (11) -COOH α-Methoxy-ω-propanoic acid unde (ethylene glycol) PEG-WM 588.7 g / mol, PEG1161 MeO-PEG-COOH α-Methoxy-ω -carboxylic acid poly (ethylene glycol) PEG-WM 750 D, PEG1158 MeO-PEG-COOH α-Methoxy-ω -carboxylic acid poly (ethylene glycol) PEG-WM 2,000 D, PEG1160 MeO-PEG-COOH α-Methoxy-ω- Poly (ethylene glycol) carboxylic acid PEG-WM 5,000 D, PEG1157 MeO-PEG-COOH α-Methoxy-ω-carboxylic acid poly (ethylene glycol) PEG-WM 10,000 D, PEG1159 MeO-PEG-COOH α-Methoxy-ω-carboxylic acid poly (ethylene glycol) PEG-WM 20,000 D, PEG1166 MeO-PEG-COO-Su α-Methoxy-ω-carboxylic acid succinimidyl ester poly (ethylene glycol) PEG-WM 750 D, PEG1163 MeO-PEG-COO-Su α-Methoxy- ω-carboxylic acid succinimidyl ester poly (ethylene glycol) PEG-WM 2,000 D, PEG1165 MeO-PEG-COO-Su α-Methoxy-ω-carboxylic acid succinimidyl ester poly (ethylene glycol) PEG-WM 5,000 D, PEG1162 MeO-PEG-COO -Your α-Methoxy-ω-carboxylic acid succinimidyl ester poly (ethylene glycol) PEG-WM 10,000 D, PEG1164 MeO-PEG-COO-Su α-Methoxy-ω-carboxylic acid succinimidyl ester poly (ethylene glycol) PEG-WM 20,000 D,

ii) HOOC-PEG-COOH: PEG1091 HOOC-PEG (12) -COOH α, ω-Bis (propionic acid) duodeca (ethylene glycol) PEG-WM 2,000 690.8 g / mol, PEG1083 HOOC-PEG-COOH α, ω-Bis-carboxy poly (ethylene glycol) PEG-WM 2,000 D, 4 PEG1085 HOOC-PEG-COOH α, ω-Bis-carboxy poly (ethylene glycol) PEG-WM 3,000 DPEG1086 HOOC-PEG-COOH α, ω-Bis -carboxy poly (ethylene glycol) PEG-WM 6,000 D, PEG1082 HOOC-PEG-COOH α, ω-Bis-carboxy poly (ethylene glycol) PEG-WM 10,000 D PEG1084 HOOC-PEG-COOH α, ω-Bis-carboxy poly (ethylene glycol) PEG-WM 20,000 D,

iii) NHS-PEG-NHS: PEG1184 Su-OOC-PEG-COO-Su α, ω-Di-succinimidyl ester poly (ethylene glycol) PEG-WM 2,000 D, PEG1186 Su-OOC-PEG-COO-Su α, ω -Di-succinimidyl poly (ethylene glycol) ester PEG-WM 3,000 D, PEG1187 Su-OOC-PEG-COO-Su α, ω-Di-succinimidyl poly (ethylene glycol) ester PEG-WM 6,000 D, PEG1183 Su-OOC- PEGCOO-Su α, ω-Di-succinimidyl ester poly (ethylene glycol) PEG-WM 10,000 D, PEG1185 Su-OOC-PEG-COO-Su α, ω-Disuccinimidyl ester poly (ethylene glycol) PEG-WM 20,000 D,

iv) H2N-PEG-COOH: PEG1096 H2N-PEG-COOH * HCl α-Amino-ω-carboxy poly (ethylene glycol) PEG-WM 3,000 D hydrochloride, PEG1097 H2N-PEG-COOH * HCl α-Amino-ω-carboxy poly (ethylene glycol) PEG-WM hydrochloride 5,000 Dalton PEG1095 H2N-PEG-COOH * HCl α-Amino-ω-carboxy poly (ethylene glycol) PEG-WM 10,000 Dalton hydrochloride.

PEG1163 MeO-PEG-COO-Su α-Methoxy-ω-carboxylic acid succinimidyl ester poly (ethylene glycol) PEG-WM 2,000 Dalton was preferably chosen. The PEG derivative containing the succinimidyl ester functional group allows direct functionalization of the magnetoferritins since this activated ester group reacts with the amino groups surrounding the nanoparticles, forming an amide-type covalent bond.

Experimental data have shown that after 3 h of injection, the particles accumulate significantly in the lung. On the other hand, since controlling the amount of Tc / particle (in a range 0-20, with 100% practically incorporating Tc) allows the optimum range of Tc concentrations to be reached in excess (10-9 M ) and that of MRI (of the order of 10-5 M).

Another aspect is to provide a method for the synthesis of magnetoferritins of the present invention. Although the introduction of magnetite can be done through the process described by Douglas (Masaki Uchida, Masahiro Terashima, Charles H. Cunningham, Yoriyasu Suzuki, Deborah A. Willits, Ann F. Willis, Philip C. Yang, Philip S. Tsao, Michael V. McConnell, Mark J. Young and Trevor Douglas, Magnetic Resonance in Medicine 60: 10731081 (2008)), the present inventors have developed a variation, which provide some advantages. The method of the invention comprises at least the steps of:

a) preparing an apoferritin solution, preferably of a concentration between 0.1 and 100 mg / ml, and more preferably between 5 and 20 mg / ml,

b) Prepare a solution comprising Fe (II) and Fe (III) in stoichiometry of approximately 1: 2, that is, between 1: 1.8 to 1.8: 1

c) prepare a solution of pertecnectate (99mTc)

d) intercalatedly add the solution prepared in step (b) and the solution prepared in step (c) over that prepared in step (a).

f) Preferably, the superparamagnetic magnetoferritin doped with 99mTc is isolated.

The initial stoichiometry of Fe (II) and Fe (III) is decisive for the proper preparation of magnetoferritin and hence its magnetic properties. Unlike the method reported by Douglas et al., Where all the initial Fe is in its oxidation state Fe (II) and it has been proven that with a rigorous control of the extent of oxidation, in our method, the stoichiometric balance of Departure confers optimal conditions and does not require exhaustive control of the air inlet in the system.

The iron (II) and (III) salts useful for the preparation of magnetoferritin are known to those skilled in the art. In a preferred embodiment step (b) is prepared by mixing a solution comprising iron (II) sulfate ammonia hexahydrate with another comprising Fe (NO3) 3 in HCl.

The inclusion of 99mTcO4 - is carried out by small additions of 99mTcO4 - at the same time as the magnetite network is made. The resulting solution can be dialyzed into dialysis bags with adequate pore size and separate particles from all remaining material. In the solution that does not contain the particles, the concentration of Tc can be measured and in this way the percentage of incorporated Tc is known. In some cases, the behavior of MoO42- has been studied, because it has a chemistry very similar to 99mTcO4 - but it is not radioactive. It has been observed that for small Mo contents (0-20 Mo / magnetoferritin atoms), the incorporation is practically 100%.

In order to carry out a more detailed characterization that allows to know the distribution of Tc in the superparamagnetic nanoparticle, a study was carried out by means of Transmission Electron Microscopy of similar samples in which instead of using the radio-marker pertecnectate, other anions of the type molybdate, vanadate, arsenate and phosphate. The chemistry of these anions is similar to that of pertecnectate, especially if there are no changes in the oxidation state of the metal.

The study of Transmission Electron Microscopy is especially useful in the case of nanoparticles doped with vanadate; This technique provides us with information about the nanoparticle size distribution as well as the chemical composition and spatial distribution of oxidation states in individual nanoparticles. Dark-field images at a high angle are sensitive to the atomic number of the material, that is, those areas where the heaviest elements are present will be shown in the image as points of greater intensity. In our case study, the nanoparticles, containing elements of high atomic number, will appear in the image with high contrast, being displayed directly and individually. Under these conditions of image registration, direct measurements of the size of the nanoparticles present in the sample can be made, from which a particle size distribution can be established. Additionally, the spatial distribution can be determined, with sub-nanometric resolution, of the chemical elements present in the individual particles, using the electron energy loss technique (EELS). This technique allows us to directly study the electronic transitions that occur in the atom when it is subjected to a beam of high-energy electrons, 200 kV. In particular, this technique measures the energy that the incident electron loses when it interacts with an atom. For example in the case of Vanadium atoms, the L2.3 transitions are directly studied where the 2p electrons of the atom are transferred to unoccupied states above the Fermi level. The energy required for this transition is a characteristic value for each atom and is equal to the energy lost by the incident electron. Thus, by measuring the energy loss of the incident electrons one can identify the different elements present in the nanoparticles, (V 513eV, O 532eV, Fe 708eV). Additionally, the fine structure of the EELS spectrum of transition metals is characterized by the presence of two intense peaks (white lines) whose intensity and position in energy varies depending on the oxidation state of the material (Leapman et al Phys. Rev. Lett. 45, 397 (1980), Turquat et al. International Journal of Inorganic Materials 3 (2001) 1025-1032). The detailed study of the fine structure of the absorption peak reflects information on the electronic state of the material, being able to study the possible variations in the oxidation state of iron or vanadium through the nanoparticles.

The study of the chemical composition and oxidation states in individual nanoparticles was carried out by combining the properties of the dark field images at high angle with the electron energy loss spectroscopy, using the acquisition method known as spectrum- image (Tence, M. Quartuccio and C. Colliex, Ultramicroscopy 58 (1995) 42, Maigne et al Journal of Electron Microscopy 58 (3): 99-109 (2009)). This mode consists of simultaneously acquiring the dark-field signal at a high angle and the EELS spectra while the probe sweeps a predetermined area, image (1D) or line spectrum. In particular, using an acquisition time of 2 seconds, an EELS spectrum was acquired, with dispersion energy of 0.5 eV, every 0.6 nm along a 36.7 nm line that passes through the nanoparticles. The analysis of each of the acquired spectra (quantification and study of the oxidation state) along the nanoparticle gives us the composition and oxidation state of the metal characterized to the sub-nanometer scale.

Preferably in the method in the solution of step (a) it is buffered with AMPSO at a pH between pH 7.5 and 9.5, preferably between 8.0 and 9.0.

In a particular embodiment, the chains of the biocompatible polymer, preferably PEG, are reacted with the magnetoferritin after the inclusion of the magnetite / Tc.

Another aspect relates to a pharmaceutical composition comprising the magnetoferritins of the present invention and at least one pharmaceutically acceptable excipient, as well as the use of said pharmaceutical composition for the preparation of a medicament.

The magnetoferritin of the present invention as well as the pharmaceutical composition that includes them are useful for the preparation of a medicament for the diagnosis of different diseases, according to the use of molecules that confidently specify it for a tissue or organ in question, but especially cancer , including cervical, head and neck, renal and ureter, colon, rectum and anus, endometrial, esophagus, stomach, liver, larynx, ovarian, pancreas, skin, prostate, lung, brain, testis, leukemia, melanoma, and lymphoma.

In addition to detecting diseases, both the magnetoferritin of the present invention and the pharmaceutical composition comprising them as contrast agents in general and as a contrast agent in MRI or scintigraphy in particular are also useful.

Throughout the description and the claims the word "comprises" and its variants are not intended to exclude other technical characteristics, additives, components or steps. For those skilled in the art, other objects, advantages and features of the invention will be derived partly from the description and partly from the practice of the invention. The following examples are provided by way of illustration, and are not intended to be limiting of the present invention.

Examples

Synthesis of magnetoferritin-99mTc

Solution 1. A 10 ml solution of apoferritin (Sigma-Aldrich Ref. A341-1G, lot. 048K7004) with a concentration of 10 mg / ml in AMPSO buffer pH 8.6 (Sigma A6659) is prepared. The solution is degassed with a strong stream of argon and under stirring for 10 min.

Solution 2. Two solutions are prepared: 5 ml of Mohr Salt (Iron (II) ammonium sulfate hexahydrate, Aldrich Chem. 20, 350-5) 0.05 M in 0.01M H5mldeFe (NO3) 3 0.1 M HCl in 0.01 M HCl, they are mixed and degassed with a strong stream of argon and under stirring for 10 min.

Solution 3. A solution of 0.1 M NaOH is degassed with a strong stream of argon and under stirring for 10 min.

Solution 4. A solution of a particulate (99mTc) obtained from a commercial kit is degassed with a strong argon current and under stirring for 2 min.

Suspension 5. Slow addition of solution 2 is carried out on solution 1. Additions of 0.25 ml are carried out every 2 min until 1 ml is completed. Before the addition of solution 2, 56 µl of the 99mTc solution (solution 4) is added.

Solution 6. Suspension 5 is slowly added 1 ml of a 0.1 M sodium citrate solution to remove all metal compounds that have not been encapsulated in apoferritin. The resulting solution is chromatographed (10 min) in size exclusion column (Sephadex G-25, lot. 360710, GE Healthcare, PD10 Desalting Columns, 17-0851-01), obtaining the final solution 6 containing mangnetite doped with 99mTc encapsulated in the apoferritin cavity.

Addition of Tc radioisotope to maqnetoferritin

Solution 4. A 99Mo / 99mTc generator with 12 GBq of calibrated activity is used. The elution performed is analyzed in terms of 99mTc activity. Once the specific ratio mCi / μg of 99mTc is known, it is possible to control the amount of Tc used and therefore its radiochemical activity.

Suspension 5. Slow addition of solution 2 is carried out on solution 1. Additions of 0.25 ml are carried out every 2 min until 1 ml is completed. Before the addition of solution 2, 0.5 ml of the 99mTc solution (solution 4) is added.

To carry out the quality control, we use Whatman 3 MM paper strips 10 cm long and 0.5 cm wide, in which we deposit an aliquot (150 μl) of the labeled radiopharmaceutical, and for its development we introduce them in chromatographic tanks with acetone up to about 0.5 mm from the base. When the chromatography has developed we measure it on the Raytest Minigit Chromatograph Radio. In the origin of the chromatographic strip the colloids will remain (Rf = 0), in this case the magnetoferritin doped with Tc, and in the front the free pertechnetate (Rf = 1)

PEG coupling

The polyethylene glycol derivative MeO-PEG-NHS α-Methoxy-ω-carboxylic acid succinimidyl ester poly (ethylene glycol) (PEG-MW 2,000 Dalton) / MW 2,000 g / mol) was purchased from Iris Biotech GmbH (PEG1164, lot. 125447) .

Solution 7. 1000 moles of PEG (0.0058 g in 0.5 ml of double distilled water) were added to solution 8 and left 30 min under gentle stirring and at room temperature. Chromatograph (10 min) on a size exclusion column (Sephadex G-25, lot. 360710, GE Healthcare, PD-10 Desalting Columns, 17-0851-01) until obtaining a pure solution of magnetite nanoparticles doped with 99mTc , covalently coupled with a PEG biopolymer.

Claims (18)

1. A superparamagnetic magnetoferritin, characterized in that the magnetite core occludes 99mTc.

2.

The superparamagnetic magnetoferritin according to the preceding claim, characterized in that the Tc species is 99mTcO4 -.

3.

The superparamagnetic magnetoferritin according to any of the preceding claims, characterized in that the concentration of the 99mTc species is between 10−9-10-5 M.

Four.

The superparamagnetic magnetoferritin according to any of the preceding claims, characterized in that it has chains of a biocompatible polymer covalently bonded to the surface of the magnetoferritin.

5.

The superparamagnetic magnetoferritin according to the preceding claim, characterized in that the biocompatible polymer is polyethylene glycol.

6.

The superparamagnetic magnetoferritin according to the preceding claim, characterized in that the polyethylene glycol is PEG1163 MeO-PEG-COO-Su α-Methoxy-ω-carboxylic acid succinimidyl ester poly (ethylene glycol) PEG-WM 2,000 Dalton.

7.

The superparamagnetic magnetoferritin according to any of the two preceding claims, characterized in that the PEG is linked by covalent bonds of the amide type.

8.

The superparamagnetic magnetoferritin according to any of the three preceding claims, characterized in that it has between 3 and 10 PEG chains covalently bonded to the surface of the magnetoferritin.

9.

A method for the synthesis of any of the superparamagnetic magnetoferritins as defined in the preceding claims comprising: a) preparing an apoferritin solution, preferably of a concentration between 0.1 and 100 mg / mL, and more preferably between 5 and 20 mg / mL, b) Prepare a solution comprising Fe (II) and Fe (III) in stoichiometry of approximately 1: 2. c) prepare a solution of pentactate (99mTc) d) intercalate the solution prepared in step (b) and the solution prepared in step (c)

about the one prepared in step (a). f) Isolate the superparamagnetic magnetoferritin doped with 99mTc.

10.

The method according to the preceding claim wherein the solution of step (b) is prepared by mixing a solution comprising iron (II) sulfate ammonia hexahydrate with another comprising Fe (NO3) 3 in HCl.

eleven.

The method according to any of the two preceding claims, wherein the solution of step (a) is buffered with AMPSO at a pH between pH 7.5 and 9.5, preferably between 8.0 and 9.0.

12.

The method according to any of the three preceding claims for the synthesis of any of the superparamagnetic magnetoferritins as defined in claims 5 to 8, comprising reacting the superparamagnetic magnetoferritins with the biocompatible polymer.

13.

A pharmaceutical composition comprising the superparamagnetic magnetoferritin as in any of claims 1-8 and at least one pharmaceutically acceptable excipient.

14. Use of the pharmaceutical composition according to the preceding claim for the preparation of a medicament.

fifteen.

The use of the composition according to the preceding claim for the preparation of a medicament for the diagnosis of cancer.

16.

The superparamagnetic magnetoferritin according to any one of claims 1 to 8 the pharmaceutical composition according to claim 13 for the preparation of a medicament for use as a contrast agent.

17.

The superparamagnetic magnetoferritin according to any one of claims 1 to 8 or the pharmaceutical composition according to claim 13 for the preparation of a medicament for use as a contrast agent in MRI or SPECT.

SPANISH OFFICE OF THE PATENTS AND BRAND Application no .: 200930845 SPAIN Date of submission of the application: 14.10.2009 Priority Date: REPORT ON THE STATE OF THE TECHNIQUE RELEVANT DOCUMENTS

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 Documents cited  Claims Affected

A A A A A A  US 20070258888 A1 (FELDMANN et al.) 08.11.2007, paragraphs [0007], [0009], [0012], [0019], [0022], [0035]. WO 2008115854 A2 (GOVERNMENT OF THE UNITED STATES OF AMERICA, UNIVERSITY OF OXFORD) 25.09.2008, paragraphs [0004], [0005], [0016], [0020], [0028], [0045], [0046]. US 5491219 A (MANN) 13.02.1996, columns 1.2. P.E. DICKSON et al. "Properties of magnetoferritin: a novel biomagnetic nanoparticle" NANOSTRUCTURED MATERIALS, vol. 9, 1997, pages 595-598. DOMINIC P.E. DICKSON "Nanostructured magnetism in living systems" JOURNAL OF MAGNETISM AND MAGNETIC MATERIALS, vol. 203, 1999, pages 46-49. Page 46, section 2 and page 48, section 3. MASAKI UCHIDA et al. "A human ferritin iron oxide nano-composite magnetic resonance contrast agent" MAGNETIC RESONANCE IN MEDICINE, vol. 60, 2008, pages 1073-1081. Summary and page 1080, conclusion section.  1-17 1-17 1-17 1-17 1-17 1-17

  Category of the documents cited X: of particular relevance Y: of particular relevance combined with other / s of the same category A: reflects the state of the art O: refers to unwritten disclosure P: published between the priority date and the date of priority submission of the application E: previous document, but published after the date of submission of the application

  This report has been produced � for all claims � for claims no:

Date of realization of the report 07.10.2011  Examiner S. González Peñalba  Page 1/4

REPORT OF THE STATE OF THE TECHNIQUE Application number: 200930845 CLASSIFICATION OBJECT OF THE APPLICATION  A61K49 / 14 (2006.01) A61K51 / 08 (2006.01) C07K14 / 435 (2006.01) A61B5 / 055 (2006.01) Minimum documentation sought (classification system followed by classification symbols) C07K, A61B Electronic databases consulted during the search (name of the database and, if possible, search terms used) INVENTIONS, EPODOC State of the Art Report Page 2/4  WRITTEN OPINION Application number: 200930845 Date of Completion of Written Opinion: 07.10.2011 Statement

Novelty (Art. 6.1 LP 11/1986)

Claims Claims 1-17 IF NOT

Inventive activity (Art. 8.1 LP11 / 1986)

Claims Claims 1-17 IF NOT

The application is considered to comply with the industrial application requirement. This requirement was evaluated during the formal and technical examination phase of the application (Article 31.2 Law 11/1986).  Basis of Opinion.- This opinion has been made on the basis of the patent application as published. State of the Art Report Page 3/4  WRITTEN OPINION Application number: 200930845 1. Documents considered.- The documents belonging to the state of the art taken into consideration for the realization of this opinion are listed below.

Document

Publication or Identification Number Publication Date

D01

US 20070258888 A1 (FELDMANN et al.) 08.11.2007

D02

WO 2008115854 A2 (GOVERNMENT OF THE UNITED STATES OF AMERICA, UNIVERSITY OF OXFORD) 25.09.2008

D03

US 5491219 A (MANN) 13.02.1996

D04

P.E. DICKSON et al. "Properties of magnetoferritin: a novel biomagnetic nanoparticle" NANOSTRUCTURED MATERIALS, vol. 9, 1997, pages 595-598. 1997

D05

DOMINIC P.E. DICKSON "Nanostructured magnetism in living systems" JOURNAL OF MAGNETISM AND MAGNETIC MATERIALS, vol. 203, 1999, pages 46-49. Page 46, section 2 and page 48, section 3. 1999

D06

MASAKI UCHIDA et al. "A human ferritin iron oxide nanocomposite magnetic resonance contrast agent" MAGNETIC RESONANCE IN MEDICINE, vol. 60, 2008, pages 1073-1081. Summary and page 1080, conclusion section 2008

2. Statement motivated according to articles 29.6 and 29.7 of the Regulations for the execution of Law 11/1986, of March 20, on Patents on novelty and inventive activity; quotes and explanations in support of this statement The present patent application, as written, refers to a superparamagnetic magnetoferritin characterized in that the magnetite core occludes 99mTc (claims 1-3). Said superparamagnetic magnetoferritin also has chains of a biocompatible polymer covalently bonded to the surface of the magnetoferritin; wherein the biocompatible polymer is polyethylene glycol (claims 4-8). The superparamagnetic magnetoferritin synthesis method is also claimed (claims 9-12); as well as a composition comprising the magnetoferritin of the invention (claim 13) and its use for the preparation of a medicament (claim 14) for the diagnosis of cancer (claim 15) and as a contrast agent (claim 16), specifically in MRI or SPECT (claim 17). NEW AND INVENTIVE ACTIVITY: L P ARTS. 6 AND 8. Document D01 refers to a new contrast agent suitable for different imaging techniques such as MRI, SPECT, etc. (see paragraphs [0007] and [0009]). Said contrast agent comprises particles consisting of a core comprising an oxide, a mixture of oxides or hydroxides of an element selected from among other Fe (see paragraphs [0012] and [0022]). Furthermore, said core preferably contains 99Mo, this is advantageous, since 99Mo can be transformed into 99Tc by conventional reactor techniques (see paragraph [0019]). On the other hand, said contrast agent may contain polyethylene glycol in a shell to provide biocompatibility (see paragraph [0035]). Document D02 refers to a multifunctional nanoparticle that can be used in three different imaging techniques such as: magnetic resonance, optical and radioisotope. Said particle comprises: a) a metal core, b) a biocompatible envelope layer and c) a biomolecule conjugated to the biocompatible envelope layer and a multidented ligand (see paragraphs [0004] and [0005]. The metal core may be among others Fe , such as superparamagnetic iron oxide (see paragraph [0016]) The biocompatible covalent layer may be polyethylene glycol (PEG) among others (see paragraph [0020]). The biomolecule can be Either synthetic or natural molecules, which have a certain role in the biological system (DNA, immunoglobulins etc) (see paragraph [0028]). And finally, the multidentate ligand is conjugated to an image agent that is optionally radioactive, such as among other 99mTc (see paragraphs [0045] and [0046]). Document D03 describes a method of synthesis of a superparamagnetic magnetoferritin useful in imaging techniques. (see column 1 and 2) Document D04 deals with the properties of a new biomagnetic nanoparticle: magnetoferritin. Document D05 refers to the study of ferritin and its magnetoferritin derivative as a model system superparamagnetic (see page 46, section 2); and as a nano-phase magnetic material (see page 48, section 3). Document D06 describes the use as a contrast agent for RMI of a human ferritin. It is a ferritin of recombinant human H chain (rHFn) that encapsulates a mineralized magnetite (or maghemite) (see summary and page 1080, conclusion section). None of the documents considered alone or in combination reveals a superparamagnetic magnetoferritin whose 99mTc occluded magnetite core. Also in the cited documents there are no suggestions that direct the expert in the matter towards the invention defined in claims 1-17. Therefore the object of claims 1-17 meets the requirements of novelty and inventive activity in accordance with the L P articles 6 and 8. State of the Art Report Page 4/4