WO2014016465A1 - Biosensor con nanoparticulas metálicas - Google Patents
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- WO2014016465A1 WO2014016465A1 PCT/ES2013/070549 ES2013070549W WO2014016465A1 WO 2014016465 A1 WO2014016465 A1 WO 2014016465A1 ES 2013070549 W ES2013070549 W ES 2013070549W WO 2014016465 A1 WO2014016465 A1 WO 2014016465A1
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- G01N2201/06113—Coherent sources; lasers
-
- Y—GENERAL TAGGING OF NEW TECHNOLOGICAL DEVELOPMENTS; GENERAL TAGGING OF CROSS-SECTIONAL TECHNOLOGIES SPANNING OVER SEVERAL SECTIONS OF THE IPC; TECHNICAL SUBJECTS COVERED BY FORMER USPC CROSS-REFERENCE ART COLLECTIONS [XRACs] AND DIGESTS
- Y10—TECHNICAL SUBJECTS COVERED BY FORMER USPC
- Y10S—TECHNICAL SUBJECTS COVERED BY FORMER USPC CROSS-REFERENCE ART COLLECTIONS [XRACs] AND DIGESTS
- Y10S977/00—Nanotechnology
- Y10S977/902—Specified use of nanostructure
- Y10S977/932—Specified use of nanostructure for electronic or optoelectronic application
- Y10S977/953—Detector using nanostructure
- Y10S977/954—Of radiant energy
Definitions
- the present invention relates to the field of biotechnology, specifically to the field of biosensors, more specifically to the field of biosensors with metal nanoparticles as a signal transduction system.
- a biosensor is an analysis device composed of two fundamental elements: a biological receptor (an antibody, a DNA probe, or a cell ”) prepared to specifically detect a substance taking advantage of the specificity of biomolecular interactions and a transducer or sensor , capable of interpreting the biological recognition reaction produced by the receptor and "translating it” into a quantifiable, optical or electrical signal.
- a biological receptor an antibody, a DNA probe, or a cell
- a transducer or sensor capable of interpreting the biological recognition reaction produced by the receptor and "translating it” into a quantifiable, optical or electrical signal.
- biosensors The progress in the field of biosensors is based on the experience acquired over the years about the properties and recognition capacity of various biomolecules. As recognition elements, numerous biological instruments have been used, from the simplest as enzymes or antibodies, to the most complex products of genetic engineering. On the other hand, the latest advances in microelectronics, nanotechnology and the unique properties of certain materials have been key to this type of device.
- the present invention proposes a new biosensor based on the properties of light to heat conversion of metal particles.
- a first aspect of the present invention relates to a biosensor for the visual detection of an analyte comprising:
- a recognition molecule capable of recognizing the target analyte
- a second recognition molecule capable of recognizing the target analyte
- the biosensor for the visual detection of an analyte comprises:
- a recognition molecule capable of recognizing the target analyte, immobilized on a support with a thermosensitive surface
- a second recognition molecule capable of recognizing the target analyte, attached to the surface of a metal nanoparticle having a surface plasmon band; where the detection of the analyte is performed visually by the color change in the areas of the support in which the analyte is present, produced as a result of the heat generated by the metal nanoparticles when irradiated with the external light source.
- a second aspect of the present invention relates to a biosensor for the visual detection of an analyte comprising:
- a recognition molecule capable of recognizing the target analyte
- a second recognition molecule capable of recognizing the target analyte, optionally bound to a tag molecule
- a third aspect of the present invention relates to a biosensor for the visual detection of an analyte as defined in the second aspect of the invention, which comprises:
- a recognition molecule capable of recognizing the target analyte
- a second recognition molecule capable of recognizing the target analyte, bound to one or more biotin molecules; Y and. Metal nanoparticles with surface plasmon band functionalized with streptavidin, avidin or similar molecules, which specifically recognize biotin molecules; where the detection of the analyte is performed visually by the color change in the areas of the support in which the analyte is present, produced as a result of the heat generated by the metal nanoparticles when irradiated with the external light source.
- a fourth aspect of the present invention relates to a biosensor for the visual detection of an analyte as defined in the second aspect of the invention, which comprises:
- a recognition molecule capable of recognizing the target analyte
- a second recognition molecule where the molecule is an antibody (detection antibody), capable of recognizing the target analyte; and d. Metal nanoparticles with surface plasmon band functionalized with anti-Fc antibodies that bind to the detection antibody; where the detection of the analyte is carried out visually by the color change in the areas of the support in which the analyte is present produced as a result of the heat generated by the metal nanoparticles when irradiated with the external light source.
- an antibody detection antibody
- Metal nanoparticles with surface plasmon band functionalized with anti-Fc antibodies that bind to the detection antibody
- the recognition molecules are selected from the list consisting of antibodies, peptides, enzymes, polysaccharides, nucleic acids (DNA, RNA), aptamers or peptide nucleic acids (PNAs).
- DNA molecules and antibodies Preferably DNA molecules and antibodies.
- the external light source is a laser, where the laser has a wavelength equal to the maximum wavelength of the surface plasmon band of the metal nanoparticle.
- the metal nanoparticle is selected from the list consisting of: a. Gold nanoparticles;
- the metal nanoparticle is a triangular gold nanoprism.
- the surface of the support comprises a heat-sensitive paper or a cellulose membrane, cellulose nitrate or cellulose acetate.
- the heat-sensitive paper has a second support selected from the list consisting of cellulose membranes, cellulose nitrate, cellulose acetate, polystyrene, ceramic, silicon or glass.
- a fifth aspect of the present invention relates to the use of a biosensor according to the first aspect of the invention, for the visual detection of an analyte comprising:
- step b Incubate the support of step a) with functionalized metal nanoparticles with a second recognition molecule (detection biomolecule) of the analyte; Y
- a sixth aspect of the invention relates to the use of a biosensor for the visual detection of an analyte as defined in the second aspect of the invention, for the detection of an analyte comprising: to. Add the sample, where the analyte to be determined is present, to a support that the recognition molecule (capture biomolecule) of the analyte is immobilized;
- step b Incubate the support of step a) with a second recognition molecule (detection biomolecule) of the analyte optionally labeled with a label;
- step b) Incubate the support of step b) with metal nanoparticles functionalized with a biomolecule that specifically recognizes the detection biomolecule or the label with which the detection biomolecule was modified; Y
- a preferred embodiment of the sixth aspect of the invention relates to the use of a biosensor for the detection of an analyte comprising:
- step b Incubate the support of step a) with a second recognition molecule (detection biomolecule) of the analyte labeled with at least one biotin molecule;
- SUBSTITUTE SHEET RULE 26 b Incubate the support of step a) with a second recognition molecule (detection biomolecule) that should be an antibody; C. Incubate the support of step b) with metal nanoparticles functionalized with an anti-Fc antibody; Y
- a seventh aspect of the invention relates to the use of a biosensor as defined in the first aspect of the invention, for the detection of an analyte comprising:
- step b Extract the analyte bound to the nanoparticles from the sample of step a), preferably through a centrifugation process;
- stage b Add the extraction of stage b, to a support that presents the recognition molecule (capture biomolecule) of the analyte;
- An eighth aspect of the present invention relates to the use of a biosensor according to any of the above embodiments or aspects, for the detection of additives, drugs, pathogenic microorganisms, food components, pesticides, toxic compounds or in demand analysis. oxygen biochemistry
- Figure 1 Scheme of the recognition system of the present invention.
- Figure 2 Fig. 2a. CEA recognition + Anti-CEA antibody 3C6-nanoprisms.
- Fig. 2b Recognition of anti-CEA antibody 3C6-biotin + streptavidin-nanoprisms.
- Figure 3 Fig. 3a. Recognition Anti-CEA antibody 3C1 + CEA + Anti-CEA antibody 3C6-aanoprisms.
- Fig. 3b Recognition Anti-CEA antibody 3C1 + CEA + Anti-CEA antibody 3C6-biotin + streptavidin-nanoprisms.
- Figure 4 Recognition of anti-CEA antibody 3C1 + CEA + Anti-CEA antibody 3C6 gold nanoparticles.
- Figure 5 Recognition of anti-CEA antibody 3C1 + CEA + Anti-CEA antibody 3C6 - gold nanoprisms with different irradiation times, and different distance between the surface and the laser.
- Fig. 5a Irradiation time 10 seconds at a greater distance.
- Fig. 5b irradiation time 2 seconds at a smaller distance.
- Figure 6 Recognition of anti-CEA antibody 3C1 + CEA + Anti-CEA antibody 3C6-nanoprisms (in PBS buffer and blood plasma samples).
- Figure 7 Recognition of anti-CEA antibody 3C1 + CEA + Anti-CEA antibody 3C6 - gold nanoprisms in blood plasma samples and infrared chamber detection.
- Figure 8 This figure shows the three design schemes of the biosensor described in example 5.
- the present invention relates to a biosensor comprising (i) a recognition molecule (capture biomolecule), capable of recognizing the target analyte; (ii) a support with a heat sensitive surface; (iii) an external light source; (iv) a second recognition molecule (detection biomolecule), capable of recognizing the target analyte and (v) a metal nanoparticle that has a surface plasmon band, characterized in that the detection of the analyte is performed visually by the change of color in the areas of the support in which the analyte is present, produced as a result of the heat generated by the metal nanoparticles when irradiated with the external light source.
- the biosensor of the present invention uses as a signal transduction system, the light-to-heat conversion properties of metal nanoparticles.
- the basis for the use of this system as a biosensor tide is due to the presence of the surface plasmon absorption band. These absorption bands occur when the frequency of the incident light on the nanoparticle is in resonance with the frequency of collective oscillation of the electrons in the conduction band of the particle, producing its excitation. This phenomenon is known as "localized surface plasmon resonance" (LSPR).
- the position in the spectrum of the resonance band depends decisively on the shape, size and structure (hollow or solid) of the particle, as well as the dielectric medium where the particle is located.
- the LSPR leads to high molar extinction coefficients ( ⁇ 3x10 11 M "1 cm “ 1 ), with an efficiency equivalent to 106 fluorophore molecules and a strong increase in the local electric field near the nanoparticle.
- Metal nanoparticles such as gold, silver or copper nanoparticles, have this surface plasmon resonance effect. These particles to be irradiated by an external light source with the appropriate frequency and high intensity, such as a laser, are able to release some of the energy absorbed in the form of heat, producing a localized increase in the temperature around its surface.
- This controlled heat generation is the basis of the new detection system that has been developed.
- This generated heat causes a noticeable change in a properly selected thermosensitive surface.
- the inventors of the present invention have discovered that surprisingly a limit of detection of the order of peak beats is obtained in the experiments carried out using as a means of detection the color change in the areas of the support in which the analyte is present produced by the metal nanoparticles when irradiated with the external light source.
- example 4 of the present invention illustrates how a lower order detection limit was obtained, and therefore of a higher sensitivity, using the visual detection of the present invention to that achieved in the experiments performed using an infrared camera such as detection medium
- SUBSTITUTE SHEET RULE 26 characteristics: (i) high sensitivity, (ii) high selectivity or specificity, so that the biosensor interacts exclusively with the analyte of interest and not with others of similar properties; (iii) high reliability, so that there are no noise problems in the transduction system due to the sample to be analyzed; (iv) low production cost; (v) short analysis time that allows quick actions if necessary; (vi) unnecessary pretreatment of the sample, which saves time, materials and reagents; (vii) simple operation, so that qualified personnel are not required in the use of the biosensor; (viii) ability to perform real-time analyzes, and (ix) portable so that it is possible to perform on-site analyzes.
- a biosensor for the visual detection of an analyte comprising:
- a recognition molecule capable of recognizing the target analyte
- a second recognition molecule capable of recognizing the target analyte
- a metal nanoparticle that has a surface plasmon band where the detection of the analyte is performed visually by the color change in the areas of the support in which the analyte is present, produced as a result of the heat generated by the metal nanoparticles when irradiated with the external light source.
- the biosensor for the visual detection of an analyte comprises:
- a recognition molecule capable of recognizing the target analyte
- b A support with a thermosensitive surface where to immobilize the recognition molecule (capture biomolecule) of stage a);
- a second recognition molecule capable of recognizing the target analyte
- the biosensor comprises:
- a recognition molecule capable of recognizing the target analyte, immobilized on a support with a thermosensitive surface
- a second recognition molecule capable of recognizing the target analyte, attached to the surface of a metal nanoparticle that has a surface plasmon band; where the detection of the analyte is performed visually by the color change in the areas of the support in which the analyte is present, produced as a result of the heat generated by the metal nanoparticles when irradiated with the external light source.
- the present invention is understood as a source of light external to all that source of electromagnetic radiation with energy between 380 nm and 1100 nm, with the ability to excite the LSPR band of metallic particles of gold, silver, copper or any of its alloys or rusty states.
- the external light source can be monochromatic or polychromatic, preferably monochromatic.
- SUBSTITUTE SHEET RULE 26 In the context of the present invention, it is understood as a metal nanoparticle that presents a surface plasmon band to that mono- or polycrystalline grouping of metal atoms in any of its oxidation states, or any of its alloys, which have all their geometric dimensions between 1 and 1000 nm, preferably between 1 and 200 nm.
- said metal atoms are noble metals.
- said metal atoms are gold, silver or copper atoms. In an even more preferred embodiment of the invention, they are gold or silver atoms with a tubular or triangular shape.
- recognition molecule or capture biomolecule to any molecule capable of specifically recognizing, through any type of chemical or biological interaction, a particular analyte.
- the molecules used as recognition elements in the biosensors of the present invention must possess sufficiently selective affinity to recognize a particular analyte, in the presence of other compounds, in addition to remaining stable over time and conserving their structure as well as their biological activity. once immobilized on the support and on the surface of the nanoparticles.
- peptides In the developed system antibodies, peptides, enzymes, proteins, polysaccharides, nucleic acids (DNAs), aptamers or peptide nucleic acids (PNAs) can be used as recognition molecules.
- DNAs nucleic acids
- PNAs peptide nucleic acids
- bioreceptors are nucleic acids, antibodies or antibody fragments, and the antibodies or fragments thereof have given rise to the greatest number of techniques useful for diagnosis. The reason lies in the flexibility of the immune system to produce a number
- SUBSTITUTE SHEET RULE 26 practically unlimited antibodies with different selectivities and a high affinity for their corresponding antigen.
- monoclonal antibodies or fragments thereof from virtually any molecule regardless of their size.
- one of the advantages offered by antibodies is due to the structural homogeneity of these proteins, which is independent of their specificity. This allows standardizing procedures related to their use as immunochemical reagents, such as their preservation or their immobilization on the transducer surface.
- antibody fragments Fab or single chain Fv fragment
- Fab or single chain Fv fragment can be prepared as recognition molecules that retain the structure and ability of antigen recognition; as well as recombinant antibodies, such as second generation monoclonal antibodies or minibodies.
- aptamers are molecules that due to their small size and low immunogenicity can substitute for antibodies in certain applications.
- Aptamers are single chain nucleic acids that have well-defined three-dimensional shapes, which allows them to bind to the target molecule in a similar way as antibodies. Aptamers combine the optimal characteristics of small molecules (low immunogenicity, high diffusion, etc.) and antibodies (high specificity and affinity, and chemical stability). Another advantage over monoclonal antibodies is that they are chemically synthesized instead of being expressed biologically.
- Nucleic acids are capable of detecting single base variations in a complementary sequence of DNA.
- SUBSTITUTE SHEET (RULE 26 which reduces electrostatic repulsion during hybridization, establishing stronger bonds; In addition to presenting a minor non-specific adsorption.
- the sensor recognition element (capture biomolecule) will normally be immobilized on a support with a thermosensitive surface, either by physical retention inside a matrix (entrapment), physical adsorption on a matrix by ionic or hydrophobic interactions, or binding by covalent bond.
- thermal paper will be used as a heat-sensitive surface which, due to its sensitivity to heat, will give rise to a developing signal after being subjected to an increase in temperature.
- Thermal paper is considered to be paper that consists of a thermal layer where it incorporates a dye, a sensitizer and a color developer (regardless of the chemical components with which it has been made) capable of reacting with each other giving rise to an image, after being subjected to an increase in temperature.
- any intelligent polymer will be used as a thermosensitive surface, which after being subjected to an external stimulus, such as a temperature change, gives rise to a response in the polymer properties such as: contraction, bending, color change, of state, luminescence, etc.
- Types of temperature sensitive polymers can be: PNIPAM, poly (N-isopropylacrylamide), poly (N-vinylpiperidine), poly (N-vinylcaprolactam) or poly (N-isopropylacrylamide).
- the support with a thermosensitive surface of the system comprises at least one thermosensitive support where molecular recognition takes place, such as a cellulose membrane or derivatives thereof (cellulose nitrate, cellulose acetate, etc.) or heat sensitive paper.
- a thermosensitive support where molecular recognition takes place such as a cellulose membrane or derivatives thereof (cellulose nitrate, cellulose acetate, etc.) or heat sensitive paper.
- the support with a thermosensitive surface of the system comprises two supports.
- a first support where the capture biomolecule will have been immobilized which may be a cellulose membrane or derivatives thereof (cellulose nitrate, cellulose acetate, etc.), or other materials such as polystyrene, ceramics, silicon or glass.
- To this first support will be attached a second support.
- SUBSTITUTE SHEET RULE 26 support consisting of a thermosensitive surface that will result in the developer signal being subjected to an increase in temperature.
- a second aspect of the present invention relates to a biosensor for visual detection comprising:
- a recognition molecule capable of recognizing the target analyte
- a second recognition molecule capable of recognizing the target analyte, optionally bound to a tag molecule
- Metal nanoparticles with surface plasmon band functionalized with biomolecules that specifically recognize the detection biomolecule or the label with which the detection biomolecule was modified; where the detection of the analyte is performed visually by the color change in the areas of the support in which the analyte is present, produced as a result of the heat generated by the metal nanoparticles when irradiated with the external light source.
- the biosensor of the second aspect of the invention does not comprise any type of instrumentation capable of detecting the conversion of light to heat of the Metal nanoparticles when irradiated with the external light source.
- molecule labels are understood to be those that are recognized by affinity for a ligand-protein interaction or by molecular recognition by hybridization between strands of nucleic acids.
- the detection biomolecule is modified with an antigen, hormone, vitamin, polyhistidine tail, or lectin domains, among others. It is therefore understood that NPs are functionalized with antibodies, aptamers, receptors, binding proteins, tricarboxylic acids
- both the detection biomolecule and the NP of gold are functionalized with complementary chains of nucleic acids present in nature (deoxyribonucleic acid or DNA, ribonucleic acid or RNA) or artificial (peptide nucleic acid or PNA, morpholinos , etc.) or combinations of both (DNA-DNA, PNA-DNA, DNA-PNA, PNA-PNA, etc)
- a third aspect of the present invention relates to a biosensor for visual detection as defined in the second aspect of the invention, comprising: a.
- a recognition molecule capture biomolecule, capable of recognizing the target analyte;
- a second recognition molecule capable of recognizing the target analyte, bound to one or more biotin molecules
- e Metal nanoparticles with surface plasmon band functionalized with streptavidin, avidia or similar molecules, which specifically recognize biotin molecules; where the detection of the analyte is carried out visually by the color change in the areas of the support in which the analyte is present produced as a result of the heat generated by the metal nanoparticles when irradiated with the external light source.
- a fourth aspect of the present invention relates to a biosensor for visual detection as defined in the second aspect of the invention, comprising: a.
- a recognition molecule capture biomolecule, capable of recognizing the target analyte;
- a second recognition molecule capable of recognizing the target analyte
- the proposed device is a "sandwich" recognition system, between a “recognition” molecule, capture biomolecule (either a protein such as an antibody, a DNA probe, PNA, etc.), immobilized on the support where the recognition of the analyte will take place, and a second detection molecule, detection biomolecule (a second antibody, or a complementary DNA probe) attached to the surface of the metal nanoparticle either directly or directly indirect hint through the reading protein and / or tag.
- a “recognition” molecule either a protein such as an antibody, a DNA probe, PNA, etc.
- capture biomolecule either a protein such as an antibody, a DNA probe, PNA, etc.
- detection biomolecule a second antibody, or a complementary DNA probe
- the device of the present invention allows the analysis of multiple samples in a single test with a sensitivity limit of the order of picograms.
- the detection of an analyte in a given sample can be carried out by immobilizing the recognition molecule (capture bimolecule) on a support in a first stage, for example in a cellulose nitrate membrane . Then a second step is carried out by adding the sample, where the analyte to be determined is present, to the support, leaving enough time for antigen-antibody recognition to occur. Finally, in a third stage, the support is incubated with the nanoparticles functionalized with the second recognition molecule (detection biomolecule).
- the recognition molecule capture bimolecule
- the support is placed on a heat-sensitive surface, as long as the support no longer has a heat-sensitive surface, to be irradiated with the external light source, for example a near-infrared emission laser, resulting from this It forms analyte detection.
- the external light source for example a near-infrared emission laser
- the test consists of one more stage.
- the support in the case of using the device as defined in the third aspect of the invention, in the third stage the support is incubated with a solution of the recognition molecule (detection biomolecule), for example a labeled secondary antibody with biotin
- a fourth incubation stage is carried out with the nanoparticles functionalized with streptavidin, and finally, once the support of the excess nanoparticles has been washed, it is irradiated with the emission laser.
- the nanoparticle has been functionalized with anti-Fc antibodies after the incubation stage with the sample, for the capture of the analyte to be determined, a third stage of incubation with an antibody is carried out. as detection biomolecule. After performing the corresponding washes, in a fourth stage, the functionalized nanoparticles are added with the anti-Fc antibody, finally, once the support is washed, it is irradiated with the emission laser. where the analyte is detected when the thermopile detects light to heat conversion of the metal nanoparicles when they are radiated with the external light source.
- thermopile biosensor 1 comprises:
- a recognition molecule capable of recognizing the target analyte, immobilized on a support with a heat sensitive surface; b. An external light source; and
- thermosensor 2 A second recognition molecule capable of recognizing the target analyte, bound to the surface of a metal nanoparticle havlng a surface plasmon band.
- thermosensor 2 a biosensor comprising:
- a recognition molecule capable of recognizing the target analyte
- a second recognition molecule capable of recognizing the target analyte, optionally bound to a label molecule
- thermopile To thermopile;
- thermopile biosensor 2 as it has been defined, comprising:
- a recognition molecule capable of recognizing the target analyte
- thermopile biosensor 1 comprises: a. A recognition molecule (capture biomolecule), capable of recognizing the target analyte, immobilized on a support with a thermosensitive surface;
- thermosensor 2 A second recognition molecule (detection biomolecule), capable of recognizing the target analyte, attached to the surface of a metal nanoparticle that has a surface plasmon band.
- thermosensor 2 a biosensor comprising:
- a recognition molecule capable of recognizing the target analyte
- a second recognition molecule capable of recognizing the target analyte, optionally bound to a tag molecule
- thermopile Y
- thermopile biosensor 2 as defined herein, comprising:
- a recognition molecule capable of recognizing the target analyte
- C An external light source
- d A second recognition molecule (detection biomolecule), capable of recognizing the target analyte, bound to one or more biotin molecules; and.
- a thermopile; Y A second recognition molecule (detection biomolecule), capable of recognizing the target analyte, bound to one or more biotin molecules; and.
- a thermopile; Y A thermopile
- thermopile biosensor 2 as defined herein, comprising:
- a recognition molecule capable of recognizing the target analyte
- a second recognition molecule capable of recognizing the target analyte
- thermopile Y
- the proposed device is a "sandwich" recognition system, between a “recognition” molecule, capture biomolecule (either a protein such as an antibody, a DNA probe, PNA, etc.), immobilized on the support where the recognition of the analyte will take place, and a second detection molecule, detection biomolecule (a second antibody, or a complementary DNA probe) attached to the surface of the metal nanoparticle either directly or directly indirect hint through the reading protein and / or tag.
- capture biomolecule either a protein such as an antibody, a DNA probe, PNA, etc.
- detection biomolecule a second antibody, or a complementary DNA probe
- the present invention specifically refers in the last two proposed aspects, to a universal detection system.
- biotin-labeled detection biomolecules and functionalizing the metal nanoparticles with streptavidin; the same nanoparticles conjugated with this protein can be used, for the recognition of different analytes, based on the avidin-biotin interaction avoiding, in this way, having to prepare the nanoparticle-biomolecule detection conjugate for each analyte to be determined.
- the detection system based on the functionalization of the metal nanoparticles with an anti-Fc antibody, capable of recognizing the Fe region of any other antibody, may use the same nanoparticles for the recognition of different analytes, provided that the detection biomolecule of this system be an antibody.
- the present invention relates to the following analyte detection procedures.
- Method for the detection of an analyte comprising:
- step b Incubate the support of step a) with functionalized metal nanoparticles with a second analyte recognition molecule (detection biomolecule);
- thermopile capable of detecting the conversion of light to heat of the metal nanoparticles when irradiated with the external light source.
- step b Incubate the support of step a) with a second recognition molecule (detection biomolecule) of the analyte bound to at least one tag molecule;
- step b) Incubate the support of step b) with functionalized metal nanoparticles with at least one molecule that specifically binds to the tag; d. Irradiate the support of stage c) or d) with the external light source; and e. Carry out the detection of the analyte through the use of a thermopile capable of detecting the conversion of light to heat of the metal nanoparticles when irradiated with the external light source.
- the tag molecule is biotin and the molecule that specifically binds to the tag is avidin or streptavidin or the tag molecule is avidin or streptavidin and the molecule that specifically binds to the tag is biotin.
- step b Incubate the support of step a) with a second recognition molecule (detection biomolecule) which is a detection antibody;
- a second recognition molecule detection biomolecule
- step b) Incubate the support of step b) with metal nanoparticles functionalized with anti-Fc antibodies;
- thermopile capable of detecting the conversion of light to heat of the metal nanoparticles when irradiated with the external light source.
- step b Extract the analyte with the nanoparticles from the sample in step a); C. Add the extraction of stage b, to a support that has the analyte recognition molecule immobilized (capture biomolecule);
- thermopile capable of detecting the conversion of light to heat of the metal nanoparticles when irradiated with the external light source.
- the biosensors of the present invention can be used, but not limited to, for the detection of additives, drugs, pathogenic microorganisms, food components, pesticides, toxic compounds or in the analysis of biochemical oxygen demand.
- the biosensors of the present invention can be used for the detection of any type of analyte both qualitatively and quantitatively.
- Gold spherical nanoparticles of 1-16 nm in diameter are obtained with a surface plasmon band at 519 nm.
- - Synthesis of triangular gold nanoprisms The synthesis of triangular gold nanoprisms was carried out following the method described by Pelaz et al. "Tailoring the synthesis and heating ability of gold nanoprisms for bioapplications", Langmuir 2012, 28, 8965-70.
- a 2mM solution of tetrachloroauric acid is mixed with 120 ml of a 0.5mM Na 2 S 2 03 solution, leaving under stirring for 9 minutes, after which a second addition of a volume between 20-50ml of the 0.5mM Na 2 S 2 0 3 solution is made.
- Gold nanotriangles of size between 100-160 nm are obtained, which have a surface plasmon band between 750-1075 nm.
- the nanoprisms must be passivated, by joining a polyethylene glycol (HS-PEG-COOH, 5000g / mol).
- 10ml of the nanoprism solution is incubated with 1 mg of PEG in a pH12 NaOH solution, overnight. Finally, these nanoprisms are centrifuged for 15 minutes at 10,000 rpm to remove excess reagents.
- an aqueous solution of CuS0 4 is added to 9 mL of an aqueous solution of CTAB (cetyl trimethyl ammonium bromide) with a variable concentration of 0.01-0.1 M.
- CTAB cetyl trimethyl ammonium bromide
- 0.5 mL is added of a 0.1 M aqueous solution of sodium ascorbate on the solution of Cu (ll) -CTAB.
- the solutions were heated for 5 minutes at 55 ° C. Once this time is over, 0.2 mL of 0.5 M sodium hydroxide is added, producing the immediate appearance of a yellow color in the solution.
- the solutions are kept at 55 ° C another 10 min and allowed to cool to room temperature.
- the solutions After 30 minutes, the solutions turn to a reddish purple, light yellow, or dark yellow color depending on the concentration of CTAB used.
- the particles are centrifuged at 6000 rpm for 15 minutes, and then resuspended in water. This process is repeated twice for the removal of the surfactant. At this point the solution nanocubes have a brick red color in all cases. Copper nanocubes with an approximate size of 420 nm are obtained, with different changes in their geometry according to the amount of CTAB surfactant used in the synthesis.
- nanoparticles synthesized with various recognition elements such as antibodies, DNA or PNA were functionalized.
- recognition elements such as antibodies, DNA or PNA
- functionalization we present some examples of functionalization.
- Functionalization was carried out through immobilization of the antibody on the carboxyl groups present on the surface of the nanoparticle, through carbodiimide chemistry.
- an activation of 0.5 mg of nanoparticle is carried out with 1.5 pmoles of EDC and 3.5 umoles of sulfo-NHS, in a final volume of 1 ml of MES pH 6 10mM, for 30 minutes at 37 ° C.
- Excess reagents can be removed both by centrifugation at 6000 rpm for 5 minutes, after which the particles are suspended in 10mM pH6 MES; or by using a gel filtration column.
- the carboxyl groups of the nanoparticles are activated, they are incubated with 2.5 pg of antibody in a final volume of 1 ml of 10mM pH6 MES for 1 hour at 37 ° C. After antibody binding, the surface of the nanoparticle is blocked with 50mM of 750 Da amine PEG (D-methoxy-n-amino polyethylene glycol). Finally, the nanoparticles are purified after several centrifugation cycles at 6000 rpm for 5 minutes.
- Functionalization was carried out through the immobilization of streptavidin molecules on the carboxyl groups present on the surface of the nanoparticle, through the chemistry of carbodiimide.
- an activation of 0.5 mg of nanoparticles is carried out with 1.5 umoles of EDC (1-ethyl-3- (3- dimethylaminopropyl) carbodiimide) and 3.5 umoles of sulfo-NHS (sulfo-N-hydroxysuccinimide), in a final volume 1 ml of MES pH 6 10mM, for 30 minutes at 37 ° C.
- Excess reagents can be removed both by centrifugation at 6000 rpm for 5 minutes, after which the particles are suspended in 10mM pH6 MES; or by using a gel filtration column. Once the carboxyl groups of the nanoparticles are activated, they are incubated with 1.25 pg of streptavidin in a final volume of 1 ml of 10mM pH6 MES for 1 hour at 37 ° C. After protein binding, the surface of the nanoparticle is blocked with 50mM of 750 Da amine PEG (a-methoxy-amino-amino polyethylene glycol). Finally, the nanoparticles are purified after several centrifugation cycles at 6000 rpm for 5 minutes.
- Example 3 Detection of the CEA marker in a sample using the biosensor of the present invention.
- the gold nanoprisms were synthesized and characterized (both by scanning and scanning electron microscopy and by ultraviolet-visible spectroscopy), they were functionalized with anti-CEA monoclonal antibodies, Ab3C6 (Monoclonal anti-carcinoembryonic mouse antigen 4CA30-3C6, HyTest) and also with streptavidin protein.
- Ab3C6 Monoclonal anti-carcinoembryonic mouse antigen 4CA30-3C6, HyTest
- streptavidin protein streptavidin protein.
- the corresponding biomolecule was immobilized at different concentrations (the CEA marker or the biotin-conjugated antibody) on a nitrocellulose membrane; After incubating with the functionalized nanoparticles, the membranes deposited on the thermosensitive surface were irradiated with the laser.
- the sensor recognition element in this case the anti-CEA antibody Ab3C1, Monoclonal mouse anti-carcinoembryonic antigen 4CA30-3C1, HyTest was immobilized on the sensor surface following various methodologies. It was joined by covalent bonds to glass surfaces, as well as by physical adsorption on different cellulose and nitrocellulose membranes. The results obtained using nitrocellulose membranes with the antibody adsorbed on the surface are shown below. The two strategies described above were tested; the nanoprisms functionalized with the antibody were used directly and the nanoprisms functionalized with streptavidin were used after adding the anti-CEA antibody 3C6 conjugated to biotin. Different samples were analyzed with a decreasing concentration of the CEA tumor marker diluted in PBS.
- the membranes were deposited on the heat-sensitive surface, in this case on thermal paper, to be irradiated for a few seconds with a near-infrared emission laser (with a 1000 nm wavelength).
- the anti-CEA 3C1 + CEA + Anti-CEA 3C6-Nanoprism antibody is illustrated in Figure 3a.
- the recognition of anti-CEA antibody 3C1 + CEA + Anti-CEA antibody 3C6-Biotin + Streptavidin-Nanoprisms is illustrated in Figure 3b.
- the signal produced on the thermosensitive surface generated by the irradiation of the nanoprisms once the recognition of the analyte is produced is more intense for the 3C1 -CEA- Antibody system.
- Ab3C6-nanoprmasms than for the Antibody 3C1 -CEA-Ab3C6 Biotin-Streptavidin-gold nanoprimas system but in both cases a concentration of 0.5 ng CEA / ml is detected.
- Figure 5 illustrates the recognition of anti-CEA 3C1 + CEA + Ab antibody anti-CEA 3C6-gold nanoprisms with different irradiation times, and different distance between the surface and the laser.
- an irradiation time of 10 seconds is used at a distance of 0.5cm; an irradiation time of 2 seconds 0.1 cm was used in Figure 5b.
- the same “sandwich” experiment (Ab3C1 + CEA + Ab3C6-Nanoprisms of gold) was carried out for the detection of the CEA tumor marker in blood plasma samples, to check the specificity of the system as well as the analyte detection limit In a complex sample.
- Example 4 Comparative example using an infrared camera as a detection means.
- the same samples prepared for example 3 were used for the present experiment.
- the sensor recognition element in this case the anti-CEA antibody Ab3C1
- Different samples were then analyzed with a decreasing concentration of the CEA tumor marker diluted in blood plasma.
- a near infrared emission laser was used, at a wavelength of 1000 nm to irradiate the nanoparticles.
- a thermal infrared detection camera IR camera
- IR camera thermal infrared detection camera
- the temperature increase was checked, with the IR camera, after irradiating the samples prepared for the detection of the CEA antigen in blood plasma at different concentrations. After being irradiated for a few seconds with the laser, the IR camera recorded a temperature increase of 2-3 ° C for the 0.05ng CEA / ml sample, but no signal was obtained in the case of the 0.01 ng CEA / ml sample . For these same analyte concentrations if a signal had been seen in the case of thermal paper, after the samples were irradiated with the laser.
- thermosensitive surface such as thermal paper, which using the infrared camera as a means of detection.
- Figure 7 compares the recognition of anti-CEA antibody 3C1 + CEA + Ab anti-CEA 3C6-gold nanoprisms between visual detection by means of thermal paper (figure 7a) and the IR camera as a detection system (figure 7b).
- Example 5 Thermopile detection experiments:
- thermopile capable of transforming the temperature increase, generated in a certain area around it, into a quantifiable electrical signal.
- both the concentrated and the diluted sample were irradiated with the laser (at a power of 350mW) on the membrane and on the glass cover.
- the first problem that was found is that if the laser directly hits the battery, a very high background signal is obtained (so a sufficiently high temperature increase was necessary to be distinguishable from the background signal). A response is also obtained if only the membrane is irradiated or covered without nanoparticles (the glass gives a higher signal than the nitrocellulose membrane).
- the diluted sample a response very similar to the control was obtained, while with the concentrate the temperature increase could be perfectly measured.
- the sample was 3-4 cm away from the laser, so the sensitivity will be lower than if it is directly in contact with the laser.
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EP13771551.2A EP2878950B1 (en) | 2012-07-26 | 2013-07-26 | Biosensor comprising metallic nanoparticules |
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BR112015001725-8A BR112015001725B1 (pt) | 2012-07-26 | 2013-07-26 | Métodos para a detecção de um analito em uma amostra |
CN201380045995.7A CN104813158B (zh) | 2012-07-26 | 2013-07-26 | 带有金属纳米颗粒的生物传感器 |
RS20170739A RS56289B1 (sr) | 2012-07-26 | 2013-07-26 | Biosenzor koji sadrži nanočestice metala |
US14/417,006 US10197566B2 (en) | 2012-07-26 | 2013-07-26 | Biosensor comprising metal nanoparticles |
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WO2015188814A1 (de) * | 2014-06-13 | 2015-12-17 | Leibniz-Institut Für Neue Materialien Gemeinnützige Gesellschaft Mit Beschränkter Haftung | Spezifische proteinmarkierung sowie verfahren zur identifizierung der statistischen verteilung der proteinstöchiometrie |
KR101685076B1 (ko) * | 2015-06-03 | 2016-12-09 | 연세대학교 산학협력단 | 광전도성 바이오센서 |
US9857320B2 (en) | 2014-06-24 | 2018-01-02 | Leibniz-Institut Fuer Neue Materialien Gemeinnuetzige Gesellschaft Mit Beschraenkter Haftung | Device and method for the stoichiometric analysis of samples |
US9966223B2 (en) | 2014-03-12 | 2018-05-08 | Leibniz-Institut Fuer Neue Materialien Gemeinnuetzige Gmbh | Device for correlative scanning transmission electron microscopy (STEM) and light microscopy |
US20180299436A1 (en) * | 2017-01-20 | 2018-10-18 | Shenzhen New Industries Biomedical Engineering Co., Ltd. | A method, kit and system for preparing an antibody pair and the use of the kit |
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RU2684276C1 (ru) * | 2018-03-05 | 2019-04-05 | федеральное государственное автономное образовательное учреждение высшего образования "Российский университет дружбы народов" (РУДН) | Флуоресцентный оптический ДНК-сенсор |
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ES2553027A1 (es) * | 2014-06-03 | 2015-12-03 | Consejo Superior De Investigaciones Cientificas | Un sistema para aplicaciones de biodetección |
US10502734B2 (en) | 2014-06-03 | 2019-12-10 | Consejo Superior De Investigaciones Cientificas | System for biodetection applications |
WO2015188814A1 (de) * | 2014-06-13 | 2015-12-17 | Leibniz-Institut Für Neue Materialien Gemeinnützige Gesellschaft Mit Beschränkter Haftung | Spezifische proteinmarkierung sowie verfahren zur identifizierung der statistischen verteilung der proteinstöchiometrie |
US11499967B2 (en) | 2014-06-13 | 2022-11-15 | Leibniz-Institut Fuer Neue Materialien Gemeinnuetzige Gesellschaft Mit Beschraenkter Haftung | Specific protein marker and method for identifying the statistic distribution of protein stoichiometry |
US9857320B2 (en) | 2014-06-24 | 2018-01-02 | Leibniz-Institut Fuer Neue Materialien Gemeinnuetzige Gesellschaft Mit Beschraenkter Haftung | Device and method for the stoichiometric analysis of samples |
KR101685076B1 (ko) * | 2015-06-03 | 2016-12-09 | 연세대학교 산학협력단 | 광전도성 바이오센서 |
US20180299436A1 (en) * | 2017-01-20 | 2018-10-18 | Shenzhen New Industries Biomedical Engineering Co., Ltd. | A method, kit and system for preparing an antibody pair and the use of the kit |
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EP2878950A1 (en) | 2015-06-03 |
JP6305402B2 (ja) | 2018-04-04 |
ES2641441T3 (es) | 2017-11-10 |
CN104813158B (zh) | 2018-02-13 |
ES2440368A2 (es) | 2014-01-28 |
EP2878950B1 (en) | 2017-04-26 |
ES2440368R1 (es) | 2014-05-08 |
ES2440368B1 (es) | 2015-03-06 |
RU2015102212A (ru) | 2016-09-20 |
WO2014016465A9 (es) | 2015-03-12 |
BR112015001725A2 (pt) | 2017-07-04 |
PL2878950T3 (pl) | 2017-11-30 |
JP2015522828A (ja) | 2015-08-06 |
HK1213055A1 (zh) | 2016-06-24 |
LT2878950T (lt) | 2017-12-27 |
RU2658052C2 (ru) | 2018-06-19 |
BR112015001725B1 (pt) | 2022-08-09 |
SI2878950T1 (sl) | 2017-11-30 |
PT2878950T (pt) | 2017-08-01 |
RS56289B1 (sr) | 2017-12-29 |
CY1119325T1 (el) | 2018-02-14 |
DK2878950T3 (da) | 2017-08-14 |
HRP20171128T1 (hr) | 2017-11-03 |
US10197566B2 (en) | 2019-02-05 |
CN104813158A (zh) | 2015-07-29 |
US20150293084A1 (en) | 2015-10-15 |
HUE033318T2 (en) | 2017-11-28 |
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