Indian Patents. 218355:A PROCESS FOR THE PREPARATION OF A NANOSIZED COLLOIDAL METAL PARTICLE

Title of Invention	A PROCESS FOR THE PREPARATION OF A NANOSIZED COLLOIDAL METAL PARTICLE
Abstract	The invention relates to a biological process for the preparation of nano-sized colloidal metal particles by treating wet fungus or fungus extract with a metal ion solution of the desired metal and separating the biomass to obtain the nano-sized colloidal metal particles.

Full Text	PROCESS FOR THE PREPARATION OF A NANOSIZED COLLOIDAL METAL PARTICLE Field of the invention The present invention relates to a process for the preparation of a nano sized colloidal metal particle. More particularly, the present invention relates to a process for the preparation of a nano sized colloidal metal particle using naturally occurring bio-materials. Background of the invention Nanoparticles are extremely important materials with utility in different areas ranging from nano-technology, non-linear optics, diode lasers, smart sensors, markers in drugs, gene sequencing to catalysts. In the art, nano materials are obtained by different chemical and physical methods. Chemical methods for the preparation of nano-materials include borohydride and citrate reduction methods for the preparation of colloidal metal such a gold and silver [Handley D. A., Colloidal Gold: Principles, Methods and Applications, Hayat M. A.ed., Academic Press, San Diego CA, 1989, Vol. 1, Chapter 2]. Physical methods for the preparation of nano materials include vapour deposition, lithographic processes and molecular beam epitaxy (MBE). Reduction of metal ions by radiolysis is also frequently used for the preparation of nano-sized metal particles. However, the prior art methods described above suffer from several drawbacks. The chemical methods are environmentally hazardous and result in quick agglomeration of nano-particles leading to big particles of poor monodispersity. While specific capping agents are used in some of the above methods to restrict the size of the colloidal metal particles and to stabilise the particle size distribution, use of such capping agents makes the system complicated and user - unfriendly. The radiolysis method is quite complicated and gamma ray sources are not readily available. Accordingly, it is important to develop processes for the preparation of nano-particles which overcome the drawbacks enumerated above. Objects of the invention The main object of the invention is to provide a process for the preparation of nano sized colloidal metal particles that is environmentally friendly. It is another object of the invention to provide a process for the preparation of nano-sized colloidal metal particles that is user friendly. It is a further object of the invention to provide a process for the preparation of nano-sized colloidal metal particles that results in colloidal metal particles with improved stability in aqueous solution. It is another object of the invention to provide an economic and efficient process for the preparation of nano-sized colloidal metal particles. These and other objects of the invention are achieved by the process of the invention which uses a biological method for the preparation of nano-sized colloidal metal particles. Summary of the invention Accordingly the present invention provides a process for the preparation of nano-size colloidal metal particles, said process comprising; treating fungus such as herein described in the form of a whole cell wet solid mass or fungus extract with metal ion solution in presence of water wherein the concentration of the metal ions in the solution ranges from 0.01 to 0.2 g per gram of the wet fungus mycelial mass at a incubation temperature in the range of 15 to 40°C for a time period ranging between 2 to 120 hours, separating the biomass by known method to obtain the nano-sized colloidal metal particles. In one embodiment of the invention, the concentration of the metal ions in the solution ranges from 0.01 to 0.2 g per gram of the wet fungus mycelial mass. In another embodiment of the invention, the metal ion solution is prepared by dissolving the desired metal salt or acid in water. In yet another embodiment of the invention, the metal ions comprise metal from Group IB to VIIB of the periodic table. In a further embodiment of the invention, the metal ions are selected from the group consisting of Au, Ag, Pd, Pt, Ni, Rh and Ru. In another embodiment of the invention, the metal salt used for the preparation of the metal ion solution is selected from the group consisting of halide, carbonate and nitrate. In a further embodiment of the invention, the concentration of the metal ion per gram of the wet fungus or fungus extract is in the range of 10 to 200 mg. In a further embodiment of the invention, the concentration of the metal ion per gram of the wet fungus or fungus extract is in the range of 10 to 100 mg. In a further embodiment of the invention, the concentration of the metal ion per gram of the wet fungus or fungus extract is in the range of 25 to 100 mg. In another embodiment of the invention, the ratio of water to wet fungus or fungus extract ranges between 1:100 (w/w). In another embodiment of the invention, the fungus used is selected from different species of Fusarium oxysporum. In a further embodiment of the invention, the fungus is used in the form of a whole cell wet solid mass or a fungus extract. In another embodiment of the invention, the reaction of the fungus and the metal ion source is carried out in water. In another embodiment of the invention, the temperature for incubation is in the range of 23 - 33°C, preferably 25 - 29°C. Detailed description of the invention The process of the invention is described hereinbelow with reference to the following examples, which are illustrative and should not be construed as limiting the scope of the invention. Example 1: 10 g of wet fungus Fusarium oxysporum which was grown in a culture medium, separated from the medium by centrifugation, washed several times with water through centrifugation, was taken in an autoclaved conical flask and then 100 ml solution of 110 mg of HAuCU in water were added and the conical flask was then plugged with cotton and incubated at 27°C. The samples were collected from time to time by filtration of the solution containing the fungus inside the inoculation chamber under laminar flow condition. The samples were collected at different times between 2 and 120 hours and each sample was characterised by UV-Vis spectrscopy followed by fluorescence spectroscopy. The formation of purple coloration and the characteristic plasmon resonance band of gold ca 533 nm are the clear indication of the formation of gold nanoclusters by the reduction of HAuCU by the fungus. The samples were also characterised by TEM where the particle size is found to be in the range of 5 - 71 nm. The samples were further characterised by X - ray diffraction. The reflection at 29 = 38°C clearly indicates the (111) Bragg reflection of gold nanoclusters. The size of the nanoclusters was also determined from the line broadening of the (111) reflection X - ray and found to be 5 - 70 nm for the gold nanoparticles. The variation of particle size and percent conversion of Au3+ into Au° with the reaction time are shown in Table 1. Table 1: Percent reduction of Au3+ into Au° (Table Removed) Example 2: 10 g of wet fungus Fusarium oxysporum which was grown in a culture medium, separated from the medium by centrifugation, washed several times with water through centrifugation, was taken in an autoclaved conical flask and then a solution containing 25 mg of HAuCU in 100 ml water were added and the conical flask was then plugged with cotton and incubated at 27°C. The samples were collected from time to time by filtration of the solution containing the fungus inside the inoculation chamber under laminar flow condition. The samples were collected at different times between 2 and 72 hours and each sample was characterised by UV-Vis spectrscopy followed by fluorescence spectroscopy. The formation of purple coloration and the characteristic plasmon resonance band of gold ca 533 nm are a clear indication of the formation of gold nanoclusters by the reduction of HAuCU by the fungus. The samples were also characterised by TEM where the particle size is found to be in the range of 5 - 60 nm. The samples were further characterised by X - ray diffraction. The reflection at 29 = 38°C clearly indicates (111) Bragg reflection of gold nanoclusters. The size of the nanoclusters was also determined from the line broadening of the (111) reflection X -ray and found to be 5 - 70 nm for the gold nanoparticles. Example 3: 10 g of wet fungus Fusarium oxysporum which was grown in a culture medium, separated from the medium by centrifugation, washed several times with water through centrifugation, was taken in an autoclaved conical flask and then 250 mg of HAuCU in 100 ml water were added and the conical flask was then plugged with cotton and incubated at 27°C. The samples were collected from time to time by filtration of the solution containing the fungus inside the inoculation chamber under laminar flow condition. The samples were collected at different times between 2 and 72 hours and each sample was characterised by UV-Vis spectrscopy followed by fluorescence spectroscopy. The formation of purple coloration and the characteristic plasmon resonance band of gold ca 533 nm are the clear indication of the formation of gold nanoclusters by the reduction of HAuCU by the fungus. The samples were also characterised by TEM where the particle size is found to be in the range of 5 - 90 nm. The samples were further characterised by X - ray diffraction. The reflection at 26 = 38°C clearly indicates the (111) Bragg reflection of gold nanoclusters. Example 4: 10 g of wet fungus Fusarium oxysporum which was grown in a culture medium, separated from the medium by centrifugation, washed several times with water through centrifugation, was first inoculated at 27°C for 12 hours, filtered out and to the 100 g clear total filtrate, taken in a conical flask, 100 mg of HAuCU in water were added and kept at 27°C. The samples were collected from time to time by filtration of the solution containing the fungus inside the inoculation chamber under laminar flow condition. The samples were collected between 2 to 72 hours and each sample was characterised by UV-Vis spectrscopy followed by fluorescence spectroscopy. The formation of purple coloration and the characteristic plasmon resonance band of gold ca 533 nm are the clear indication of the formation of gold nanoclusters by the reduction of HAuCU by the fungus. The samples were also characterised by TEM where the particle size is found to be in the range of 5 - 70 nm. Example 5: 10 g of wet fungus Fusariutn oxysporum which was grown in a culture medium, separated from the medium by centrifugation, washed several times with water through centrifugation, was taken in an autoclaved conical flask and then 125 mg of AgNOs in 100 ml water were added and the conical flask was then plugged with cotton and incubated at 27°C. The samples were collected from time to time by filtration of the solution containing the fungus inside the inoculation chamber under laminar flow condition. The samples were collected between 1 to 86 hours and each sample was characterised by UV-Vis spectrscopy, fluorescence spectroscopy, TEM analysis. The evolution of the plasmon resonance band around 400nm and the brown colour is a clear indication of the formation of silver nanoclusters. The range of the silver nanoparticle size is found to be 5 - 80 nm. Example 6: 10 g of wet fungus Fusarium oxysporum which was grown in a culture medium, separated from the medium by centrifugation, washed several times with water through centrifugation, was taken in an autoclaved conical flask and then 50 mg of AgNOs in 100 ml water were added and the conical flask was then plugged with cotton and incubated at 37°C. The samples were collected from time to time by filtration of the solution containing the fungus inside the inoculation chamber under laminar flow condition. The samples were collected between 1 to 86 hours and each sample was characterised by UV-Vis spectrscopy, fluorescence spectroscopy, TEM analysis. The evolution of the plasmon resonance band around 400nm and the brown colour is a clear indication of the formation of silver nanoclusters. The range of the silver nanoparticle size is found to be 5 - 60 nm. Example 7: 10 g of wet fungus Fusarium oxysporum which was grown in a culture medium, separated from the medium by centrifugation, washed several times with water through centrifugation, was taken in an autoclaved conical flask and then 75 mg of AgNOs in 100 ml water were added and the conical flask was then plugged with cotton and incubated at 17°C. The samples were collected from time to time by filtration of the solution containing the fungus inside the inoculation chamber under laminar flow condition. The samples were collected at 1,2, 6, 19, 25, 30, 40, 46, 52 and 86 hours and each sample was characterised by UV-Vis spectrscopy, fluorescence spectroscopy, TEM analysis. The evolution of the plasmon resonance band around 400nm and the brown colour is a clear indication of the formation of silver nanoclusters. The range of the silver nanoparticle size is found to be in the range of 5 -40 nm. Example 8: 10 g of wet fungus Fusarium oxysporum which was grown in a culture medium, separated from the medium by centrifugation, washed several times with water through centrifugation, was taken in an autoclaved conical flask and then 100 mg of AgNOs in 100 ml water were added and the conical flask was then plugged with cotton and incubated at 21°C. The samples were collected from time to time by filtration of the solution containing the fungus inside the inoculation chamber under laminar flow condition. The samples were collected at 1,2, 6, 19, 25, 30, 40, 46, 52 and 86 hours and each sample was characterised by UV-Vis spectrscopy, fluorescence spectroscopy, TEM analysis. The evolution of the plasmon resonance band around 400nm and the brown colour is a clear indication of the formation of silver nanoclusters. The range of the silver nanoparticle size is found to be in the range of 5 -80 nm. Example 9: 10 g of wet fungus Fusarium oxysporum which was grown in a culture medium, separated from the medium by centrifugation, washed several times with water through centrifugation, was taken in an autoclaved conical flask and then 100 ml solution containing 100 mg of NiSC4 (nickel sulphate) were added and the conical flask was then plugged with cotton and incubated at 22°C. The samples were collected from time to time by filtration of the solution containing the fungus inside the inoculation chamber under laminar flow condition. The samples were collected at 1, 2, 6, 19, 25, 30, 40, 46, 52 and 86 hours and each sample was characterised by UV-Vis spectrscopy, TEM analysis and fluorescence spectroscopy. The evolution of the plasmon resonance band around 415nm is a clear indication of the formation of Ni- nanoclusters. The nanoparticles size is found to be in the range of 5 - lOOnm. Example 10: 10 g of wet fungus Fmarium oxysporum which was grown in a culture medium, separated from the medium by centrifugation, washed several times with water through centrifugation, was taken in an autoclaved conical flask and then 25 mg NiS(>4 in 100 ml water were added and the conical flask was then plugged with cotton and incubated at 25°C. The samples were collected from time to time by filtration of the solution containing the fungus inside the inoculation chamber under laminar flow condition. The samples were collected between 1 and 96 hours and each sample was characterised by UV-Vis spectrscopy, TEM analysis and fluorescence spectroscopy. The brown coloration, evolution of the plasmon resonance band around 415nm and TEM analysis indicated the formation of Ni-nanoclusters in the range of 10 - 100 nm. Example 11: 10 g of wet fungus Fusarium oxysporum which was grown in a culture medium, separated from the medium by centrifugation, washed several times with water through centrifugation, was taken in an autoclaved conical flask and 100 ml aqueous solutio containing 125 mg HjPtCle (chloroplatinic acid) in water were added and the conical flask was then plugged with cotton and incubated at 33°C. The samples were collected from time to time by filtration of the solution containing the fungus inside the inoculation chamber under laminar flow condition. The samples were collected between 1 and 96 hours and each sample was characterised by UV-Vis spectroscopy, fluorescence spectroscopy and TEM analysis. The evolution of the plasmon resonance band at 215nm is a clear indication of formation of Pt nano-particles in the solution. The samples were further characterised by TEM analysis where the particle size was found to be in the range of 10 - 50 nm. Advantages of the invention The main advantage of the present invention is the use of naturally occurring fungi under aqueous medium. Another major advantage of the present invention is that the colloidal nano-sized metal particles formed are quite stable in the aqueous solution. The method of the invention is also environmentally friendly and simple. The reduction process is extracellular with the formation of the nano-particles occurring in the solution and not inside the fungal cell. We Claim: 1. A process for the preparation of nano-size colloidal metal particles, said process comprising; treating fungus such as herein described in the form of a whole cell wet solid mass or fungus extract with metal ion solution in presence of water wherein the concentration of the metal ions in the solution ranges from 0.01 to 0.2 g per gram of the wet fungus mycelial mass at a incubation temperature in the range of 15 to 40°C for a time period ranging between 2 to 120 hours, separating the biomass by known method to obtain the nano-sized colloidal metal particles. 2. A process as claimed in claim 1 wherein the metal ions comprise metal from Group IB to VIIIB of the periodic table. 3. A process as claimed in claims 1 to 2 wherein the metal ions are selected from the group consisting of Au, Ag, Pd, Pt, Ni, Rh and Ru. 4. A process as claimed in claims 1 to 3 wherein the preferable concentration of the metal ion per gram of the wet fungus or fungus extract is the range of 0.01 to 0.1 g, more preferably in the range of 0.25 to 0.1 g. 5. A process as claimed in claims 1 to 4 wherein the ratio of water to wet fungus or fungus extract ranges between 1:100 (w/w) 6. A process as claimed claims 1 to 5 wherein the fungus used is selected from different naturally occurring species ofFusarium oxysporum. 7. A process as claimed in claims 1 to 6 wherein the temperature for incubation is in the range of 23-33 °C,preferably in the range of 25-29 °C. 8. A process for the preparation of nano-sized colloidal metal particles substantially as described hereinbefore and with reference to the foregoing examples.

Full Text

PROCESS FOR THE PREPARATION OF A NANOSIZED COLLOIDAL METAL PARTICLE
Field of the invention
The present invention relates to a process for the preparation of a nano sized colloidal metal particle. More particularly, the present invention relates to a process for the preparation of a nano sized colloidal metal particle using naturally occurring bio-materials. Background of the invention
Nanoparticles are extremely important materials with utility in different areas ranging from nano-technology, non-linear optics, diode lasers, smart sensors, markers in drugs, gene sequencing to catalysts. In the art, nano materials are obtained by different chemical and physical methods. Chemical methods for the preparation of nano-materials include borohydride and citrate reduction methods for the preparation of colloidal metal such a gold and silver [Handley D. A., Colloidal Gold: Principles, Methods and Applications, Hayat M. A.ed., Academic Press, San Diego CA, 1989, Vol. 1, Chapter 2]. Physical methods for the preparation of nano materials include vapour deposition, lithographic processes and molecular beam epitaxy (MBE). Reduction of metal ions by radiolysis is also frequently used for the preparation of nano-sized metal particles.
However, the prior art methods described above suffer from several drawbacks. The chemical methods are environmentally hazardous and result in quick agglomeration of nano-particles leading to big particles of poor monodispersity. While specific capping agents are used in some of the above methods to restrict the size of the colloidal metal particles and to stabilise the particle size distribution, use of such capping agents makes the system complicated and user - unfriendly. The radiolysis method is quite complicated and gamma ray sources are not readily available.
Accordingly, it is important to develop processes for the preparation of nano-particles which overcome the drawbacks enumerated above. Objects of the invention
The main object of the invention is to provide a process for the preparation of nano sized colloidal metal particles that is environmentally friendly.
It is another object of the invention to provide a process for the preparation of nano-sized colloidal metal particles that is user friendly.
It is a further object of the invention to provide a process for the preparation of nano-sized colloidal metal particles that results in colloidal metal particles with improved stability in aqueous solution.

It is another object of the invention to provide an economic and efficient process for the
preparation of nano-sized colloidal metal particles.
These and other objects of the invention are achieved by the process of the invention which uses
a biological method for the preparation of nano-sized colloidal metal particles.
Summary of the invention
Accordingly the present invention provides a process for the preparation of nano-size colloidal metal particles, said process comprising; treating fungus such as herein described in the form of a whole cell wet solid mass or fungus extract with metal ion solution in presence of water wherein the concentration of the metal ions in the solution ranges from 0.01 to 0.2 g per gram of the wet fungus mycelial mass at a incubation temperature in the range of 15 to 40°C for a time period ranging between 2 to 120 hours, separating the biomass by known method to obtain the nano-sized colloidal metal particles.
In one embodiment of the invention, the concentration of the metal ions in the solution ranges from 0.01 to 0.2 g per gram of the wet fungus mycelial mass.
In another embodiment of the invention, the metal ion solution is prepared by dissolving the desired metal salt or acid in water.
In yet another embodiment of the invention, the metal ions comprise metal from Group IB to VIIB of the periodic table.
In a further embodiment of the invention, the metal ions are selected from the group consisting of Au, Ag, Pd, Pt, Ni, Rh and Ru.
In another embodiment of the invention, the metal salt used for the preparation of the metal ion solution is selected from the group consisting of halide, carbonate and nitrate.
In a further embodiment of the invention, the concentration of the metal ion per gram of the wet fungus or fungus extract is in the range of 10 to 200 mg.
In a further embodiment of the invention, the concentration of the metal ion per gram of the wet fungus or fungus extract is in the range of 10 to 100 mg.
In a further embodiment of the invention, the concentration of the metal ion per gram of the wet fungus or fungus extract is in the range of 25 to 100 mg.
In another embodiment of the invention, the ratio of water to wet fungus or fungus extract ranges between 1:100 (w/w).
In another embodiment of the invention, the fungus used is selected from different species of Fusarium oxysporum.
In a further embodiment of the invention, the fungus is used in the form of a whole cell wet solid mass or a fungus extract.
In another embodiment of the invention, the reaction of the fungus and the metal ion source is carried out in water.
In another embodiment of the invention, the temperature for incubation is in the range of 23 - 33°C, preferably 25 - 29°C. Detailed description of the invention
The process of the invention is described hereinbelow with reference to the following examples, which are illustrative and should not be construed as limiting the scope of the invention. Example 1:
10 g of wet fungus Fusarium oxysporum which was grown in a culture medium, separated from the medium by centrifugation, washed several times with water through centrifugation, was taken in an autoclaved conical flask and then 100 ml solution of 110 mg of HAuCU in water were added and the conical flask was then plugged with cotton and incubated at 27°C. The samples were collected from time to time by filtration of the solution containing the fungus inside the inoculation chamber under laminar flow condition. The samples were collected at different times between 2 and 120 hours and each sample was characterised by UV-Vis spectrscopy followed by fluorescence spectroscopy. The formation of purple coloration and the characteristic plasmon resonance band of gold ca 533 nm are the clear indication of the formation of gold nanoclusters by the reduction of HAuCU by the fungus. The samples were also characterised by TEM where the particle size is found to be in the range of 5 - 71 nm. The samples were further characterised by X - ray diffraction. The
reflection at 29 = 38°C clearly indicates the (111) Bragg reflection of gold nanoclusters. The size of the nanoclusters was also determined from the line broadening of the (111) reflection X - ray and found to be 5 - 70 nm for the gold nanoparticles. The variation of particle size and percent conversion of Au3+ into Au° with the reaction time are shown in Table 1. Table 1:
Percent reduction of Au3+ into Au°
(Table Removed)
Example 2:
10 g of wet fungus Fusarium oxysporum which was grown in a culture medium, separated from the medium by centrifugation, washed several times with water through centrifugation, was taken in an autoclaved conical flask and then a solution containing 25 mg of HAuCU in 100 ml water were added and the conical flask was then plugged with cotton and incubated at 27°C. The samples were collected from time to time by filtration of the solution containing the fungus inside the inoculation chamber under laminar flow condition. The samples were collected at different times between 2 and 72 hours and each sample was characterised by UV-Vis spectrscopy followed by fluorescence spectroscopy. The formation of purple coloration and the characteristic plasmon resonance band of gold ca 533 nm are a clear indication of the formation of gold nanoclusters by the reduction of HAuCU by the fungus. The samples were also characterised by TEM where the particle size is found to be in the range of 5 - 60 nm. The samples were further characterised by X - ray diffraction. The
reflection at 29 = 38°C clearly indicates (111) Bragg reflection of gold nanoclusters. The size of the nanoclusters was also determined from the line broadening of the (111) reflection X -ray and found to be 5 - 70 nm for the gold nanoparticles. Example 3:
10 g of wet fungus Fusarium oxysporum which was grown in a culture medium, separated from the medium by centrifugation, washed several times with water through centrifugation, was taken in an autoclaved conical flask and then 250 mg of HAuCU in 100 ml water were added and the conical flask was then plugged with cotton and incubated at 27°C. The samples were collected from time to time by filtration of the solution containing the fungus inside the inoculation chamber under laminar flow condition. The samples were collected at different times between 2 and 72 hours and each sample was characterised by UV-Vis spectrscopy followed by fluorescence spectroscopy. The formation of purple coloration and the characteristic plasmon resonance band of gold ca 533 nm are the clear indication of the formation of gold nanoclusters by the reduction of HAuCU by the fungus. The samples were also characterised by TEM where the particle size is found to be in the range of 5 - 90 nm. The samples were further characterised by X - ray diffraction. The reflection at 26 = 38°C clearly indicates the (111) Bragg reflection of gold nanoclusters. Example 4:
10 g of wet fungus Fusarium oxysporum which was grown in a culture medium, separated from the medium by centrifugation, washed several times with water through centrifugation, was first inoculated at 27°C for 12 hours, filtered out and to the 100 g clear
total filtrate, taken in a conical flask, 100 mg of HAuCU in water were added and kept at 27°C. The samples were collected from time to time by filtration of the solution containing the fungus inside the inoculation chamber under laminar flow condition. The samples were collected between 2 to 72 hours and each sample was characterised by UV-Vis spectrscopy followed by fluorescence spectroscopy. The formation of purple coloration and the characteristic plasmon resonance band of gold ca 533 nm are the clear indication of the formation of gold nanoclusters by the reduction of HAuCU by the fungus. The samples were also characterised by TEM where the particle size is found to be in the range of 5 - 70 nm. Example 5:
10 g of wet fungus Fusariutn oxysporum which was grown in a culture medium, separated from the medium by centrifugation, washed several times with water through centrifugation, was taken in an autoclaved conical flask and then 125 mg of AgNOs in 100 ml water were added and the conical flask was then plugged with cotton and incubated at 27°C. The samples were collected from time to time by filtration of the solution containing the fungus inside the inoculation chamber under laminar flow condition. The samples were collected between 1 to 86 hours and each sample was characterised by UV-Vis spectrscopy, fluorescence spectroscopy, TEM analysis. The evolution of the plasmon resonance band around 400nm and the brown colour is a clear indication of the formation of silver nanoclusters. The range of the silver nanoparticle size is found to be 5 - 80 nm. Example 6:
10 g of wet fungus Fusarium oxysporum which was grown in a culture medium, separated from the medium by centrifugation, washed several times with water through centrifugation, was taken in an autoclaved conical flask and then 50 mg of AgNOs in 100 ml water were added and the conical flask was then plugged with cotton and incubated at 37°C. The samples were collected from time to time by filtration of the solution containing the fungus inside the inoculation chamber under laminar flow condition. The samples were collected between 1 to 86 hours and each sample was characterised by UV-Vis spectrscopy, fluorescence spectroscopy, TEM analysis. The evolution of the plasmon resonance band around 400nm and the brown colour is a clear indication of the formation of silver nanoclusters. The range of the silver nanoparticle size is found to be 5 - 60 nm. Example 7:
10 g of wet fungus Fusarium oxysporum which was grown in a culture medium, separated from the medium by centrifugation, washed several times with water through centrifugation, was taken in an autoclaved conical flask and then 75 mg of AgNOs in 100 ml
water were added and the conical flask was then plugged with cotton and incubated at 17°C. The samples were collected from time to time by filtration of the solution containing the fungus inside the inoculation chamber under laminar flow condition. The samples were collected at 1,2, 6, 19, 25, 30, 40, 46, 52 and 86 hours and each sample was characterised by UV-Vis spectrscopy, fluorescence spectroscopy, TEM analysis. The evolution of the plasmon resonance band around 400nm and the brown colour is a clear indication of the formation of silver nanoclusters. The range of the silver nanoparticle size is found to be in the range of 5 -40 nm. Example 8:
10 g of wet fungus Fusarium oxysporum which was grown in a culture medium, separated from the medium by centrifugation, washed several times with water through centrifugation, was taken in an autoclaved conical flask and then 100 mg of AgNOs in 100 ml water were added and the conical flask was then plugged with cotton and incubated at 21°C. The samples were collected from time to time by filtration of the solution containing the fungus inside the inoculation chamber under laminar flow condition. The samples were collected at 1,2, 6, 19, 25, 30, 40, 46, 52 and 86 hours and each sample was characterised by UV-Vis spectrscopy, fluorescence spectroscopy, TEM analysis. The evolution of the plasmon resonance band around 400nm and the brown colour is a clear indication of the formation of silver nanoclusters. The range of the silver nanoparticle size is found to be in the range of 5 -80 nm. Example 9:
10 g of wet fungus Fusarium oxysporum which was grown in a culture medium, separated from the medium by centrifugation, washed several times with water through centrifugation, was taken in an autoclaved conical flask and then 100 ml solution containing 100 mg of NiSC4 (nickel sulphate) were added and the conical flask was then plugged with cotton and incubated at 22°C. The samples were collected from time to time by filtration of the solution containing the fungus inside the inoculation chamber under laminar flow condition. The samples were collected at 1, 2, 6, 19, 25, 30, 40, 46, 52 and 86 hours and each sample was characterised by UV-Vis spectrscopy, TEM analysis and fluorescence spectroscopy. The evolution of the plasmon resonance band around 415nm is a clear indication of the formation of Ni- nanoclusters. The nanoparticles size is found to be in the range of 5 - lOOnm.
Example 10:
10 g of wet fungus Fmarium oxysporum which was grown in a culture medium, separated from the medium by centrifugation, washed several times with water through centrifugation, was taken in an autoclaved conical flask and then 25 mg NiS(>4 in 100 ml water were added and the conical flask was then plugged with cotton and incubated at 25°C. The samples were collected from time to time by filtration of the solution containing the fungus inside the inoculation chamber under laminar flow condition. The samples were collected between 1 and 96 hours and each sample was characterised by UV-Vis spectrscopy, TEM analysis and fluorescence spectroscopy. The brown coloration, evolution of the plasmon resonance band around 415nm and TEM analysis indicated the formation of Ni-nanoclusters in the range of 10 - 100 nm. Example 11:
10 g of wet fungus Fusarium oxysporum which was grown in a culture medium, separated from the medium by centrifugation, washed several times with water through centrifugation, was taken in an autoclaved conical flask and 100 ml aqueous solutio containing 125 mg HjPtCle (chloroplatinic acid) in water were added and the conical flask was then plugged with cotton and incubated at 33°C. The samples were collected from time to time by filtration of the solution containing the fungus inside the inoculation chamber under laminar flow condition. The samples were collected between 1 and 96 hours and each sample was characterised by UV-Vis spectroscopy, fluorescence spectroscopy and TEM analysis. The evolution of the plasmon resonance band at 215nm is a clear indication of formation of Pt nano-particles in the solution. The samples were further characterised by TEM analysis where the particle size was found to be in the range of 10 - 50 nm. Advantages of the invention
The main advantage of the present invention is the use of naturally occurring fungi under aqueous medium. Another major advantage of the present invention is that the colloidal nano-sized metal particles formed are quite stable in the aqueous solution. The method of the invention is also environmentally friendly and simple. The reduction process is extracellular with the formation of the nano-particles occurring in the solution and not inside the fungal cell.

We Claim:
1. A process for the preparation of nano-size colloidal metal particles, said process
comprising; treating fungus such as herein described in the form of a whole cell wet solid
mass or fungus extract with metal ion solution in presence of water wherein the
concentration of the metal ions in the solution ranges from 0.01 to 0.2 g per gram of the
wet fungus mycelial mass at a incubation temperature in the range of 15 to 40°C for a
time period ranging between 2 to 120 hours, separating the biomass by known method
to obtain the nano-sized colloidal metal particles.
2. A process as claimed in claim 1 wherein the metal ions comprise metal from Group IB to
VIIIB of the periodic table.
3. A process as claimed in claims 1 to 2 wherein the metal ions are selected from the group
consisting of Au, Ag, Pd, Pt, Ni, Rh and Ru.
4. A process as claimed in claims 1 to 3 wherein the preferable concentration of the metal
ion per gram of the wet fungus or fungus extract is the range of 0.01 to 0.1 g, more
preferably in the range of 0.25 to 0.1 g.
5. A process as claimed in claims 1 to 4 wherein the ratio of water to wet fungus or fungus
extract ranges between 1:100 (w/w)
6. A process as claimed claims 1 to 5 wherein the fungus used is selected from different
naturally occurring species ofFusarium oxysporum.
7. A process as claimed in claims 1 to 6 wherein the temperature for incubation is in the
range of 23-33 °C,preferably in the range of 25-29 °C. 8. A process for the preparation of nano-sized colloidal metal particles substantially as
described hereinbefore and with reference to the foregoing examples.

Documents:

0333-del-2001-abstract.pdf

0333-del-2001-claims.pdf

0333-del-2001-correspondence-others.pdf

0333-del-2001-correspondence-po.pdf

0333-del-2001-description (complete).pdf

0333-del-2001-form-1.pdf

0333-del-2001-form-18.pdf

0333-del-2001-form-2.pdf

0333-del-2001-form-3.pdf

0333-del-2001-petition-137.pdf

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Patent Number

218355

Indian Patent Application Number

333/DEL/2001

PG Journal Number

24/2008

Publication Date

13-Jun-2008

Grant Date

31-Mar-2008

Date of Filing

23-Mar-2001

Name of Patentee

COUNCIL OF SCIENTIFIC AND INDUSTRIAL RESEARCH

Applicant Address

RAFI MARG, NEW DELHI- 110 001, INDIA

Inventors:

#	Inventor's Name	Inventor's Address
1	PRIYABRATA KUKHERJEE	NATIONAL CHEMICAL LABORATORY, PUNE- 411008, MAHARASHTRA, INDIA
2	DEENDAYAL MANDAL	NATIONAL CHEMICAL LABORATORY, PUNE- 411008, MAHARASHTRA, INDIA
3	ABSAR AHMAD	NATIONAL CHEMICAL LABORATORY, PUNE- 411008, MAHARASHTRA, INDIA
4	MURALI SASTRY	NATIONAL CHEMICAL LABORATORY, PUNE- 411008, MAHARASHTRA, INDIA
5	RAJIV KUMAR	NATIONAL CHEMICAL LABORATORY, PUNE- 411008, MAHARASHTRA, INDIA

PCT International Classification Number

B22F 9/24

PCT International Application Number

N/A

PCT International Filing date

PCT Conventions:

#	PCT Application Number	Date of Convention	Priority Country
1			NA