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Probing of DNA structured with Nanoparticles

A Biodiction : A Unit of Dr. Divya Sharma
A Biodiction : A Unit of Dr. Divya Sharma

Probing of DNA structured with Nanoparticles: Synthesis and their Different Methods

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Probing DNA structure with Nanoparticles: Synthesis and their Different Methods Dr. Divya Sharma Assistant Professor A Biodiction (A Unit of Dr. Divya Sharma)
Introduction • In 1950s, double helical structure of DNA has been known • In the 1980s, it has become increasingly recognized that local DNA structure and dynamics can affect its function. • The DNA duplex, as a result of chemical damage or by virtue of its intrinsic sequence, may exhibit bends, loops, bulges, kinks, and other unusual structures on a few-base-pair length scale. • Characterization of local DNA structure can be done, of course, by traditional nuclear magnetic resonance or X-ray crystallographic methods. Mahtab R.,Murphy C.J. NanoBiotechnology Protocols, Methods in Molecular Biology; Vol 303
• This article describes the features of the Protein Data Bank, the standard database to search and download crystal structures, NMR structures, and some theoretical structures of biological macromolecules, including DNA: http://www.rcsb.org/pdb/ . • Rutgers University also maintains the Nucleic Acid Database for DNA/RNA sequence and structure searching: http://ndbserver.rutgers.edu/NDB/ndb.html.). • A powerful alternative approach should the DNA samples not be amenable to characterization by these methods is to bind a probe to the DNA target, and use the optical properties of the probe to infer the nature of local DNA structure or dynamics.
• Common examples of such probes include fluorescent intercalators & most unusual example of an optical probe for DNA is an inorganic nanoparticle. • Nanoparticles are materials that have diameters on the 1 to 100 nm scale and are therefore in the size range of proteins. • Nanoparticles made of inorganic materials such as semiconductors and metals have unusual, size-dependent optical properties in this size range.
• In particular, semiconductor nanoparticles are known as “Quantum dots” because they exhibit “particle-in-a-box” quantum confinement effects at the nanoscale. • CdSe and CdS nanoparticles can be made by a number of routes in the 2 to 8 nm size range, and these nanoparticles are photoluminescent in the visible, with wavelength maxima that depend on size and surface group. • Some researchers have used CdSe quantum dots as inorganic dyes for biological labeling assays. We have used CdS nanoparticles as protein- sized probes of local DNA structure.
Methods  Synthesis of “Unactivated” CdS Nanoparticles Stabilized by Polyphosphate  Activation of CdS Nanoparticles With Cd(II)  Synthesis of 2-Mercaptoethanol-Capped CdS  DNA Purification by High-Performance Liquid Chromatography and Annealing  Titrations of Cd(II)-Activated CdS With Duplex DNAs Mahtab R.,Murphy C.J. NanoBiotechnology Protocols, Methods in Molecular Biology; Vol 303
Synthesis of “Unactivated” CdS Nanoparticles Stabilized by Polyphosphate • CdS nanoparticles are prepared with reagent weights based on a final concentration of 2 × 10^–4 M . [The quantum dots prepared as described here are not “passivated,” meaning that they are not coated with a material (ZnS, or another higher- band-gap semiconductor, or silica) that will insulate the quantum dot from its environment and render its emission stable and bright regardless of the surrounding medium. In the kind of experiments described here, the intensity of the photoluminescence of the quantum dots should be sensitive to the environment. Hence, control experiments with buffer alone, and standard DNAs, are required].
Procedure: i. In a three-necked flask held over a stir/heat plate, place a stir bar and 100 mL of deionized water, and degas the water by bubbling nitrogen gas through it for 15 min. ii. Add 6.2 mg of cadmium nitrate tetrahydrate {Cd[NO3]2•4H2O} to the flask, with stirring. iii. Add 12.1 mg of sodium polyphosphate to the flask, with stirring. iv. Check the pH of the aqueous solution. Adjust the pH to 9.8 by adding small amounts of 0.1 M NaOH via a pipet.
v. Stir and add 1.6 mg of anhydrous sodium sulfide (Na2S) and dissolve it in 2 mL of water. Immediately add this solution drop-wise to the three- necked flask. The reaction mixture should become light yellow. vi. Stirring for 20 min vii. Adjust the pH of the solution to 10.3 with 0.1 M NaOH. The reaction has produced approx 4-nm CdS nanoparticles, surface capped with polyphosphate. solution should be stored under nitrogen in the dark. If one irradiates the solution with a UV blacklight, dull pinkish yellow emission will be observed. If one desires to “activate” the nanoparticles with Cd(II), the solution should remain undisturbed for 24 h.
Activation of CdS Nanoparticles With Cd(II) • The CdS solution (prepared in first method) should remain undisturbed for 24 h after its synthesis. • Prepared a solution of 0.01 M Cd(NO3)2 tetrahydrate [activates with Zn (II) and Mg (II) as well; the resulting CdS nanoparticles act similarly, but not identically, with DNA]. • Then, monitor the photoluminescence of the unactivated CdS solution. While, adding a solution Cd(NO3)2 tetrahydrate to it. • The CdS solution before activation has an emission peak maximum at approx 550 nm. • As the activation progresses, a new peak appears at approx 440 nm and the intensity of this peak increases.
• Addition of Cd(II) is continued until this new peak at 440 nm has reached its maximum intensity. • Toward the end, addition of Cd(II) is done very carefully, and the emission spectrum is checked after each addition of 1 or 2 drops, because if more Cd(II) is added than what is required for maximum activation, the photoluminescence of the activated CdS solution will decrease. • During activation the pH of the solution decreases. After activation is complete, the pH of the solution is brought back to 10.3 with 0.1 M NaOH. • The “activated” CdS solution has a very bright pinkish white glow under UV light. • The nanoparticles should not have changed in size and now are coated with a loose “web” of Cd(II). This activation procedure can be performed with other divalent metal salt solutions as well.
Synthesis of 2-Mercaptoethanol-Capped CdS • The synthesis of 2-mercaptoethanol-capped CdS produces nanoparticles that bear ⎯SCH2CH2OH groups that are ionically neutral compared with the probing DNA structure with nanoparticles activated ones. • As before, CdS nanoparticles are prepared with reagent weights based on a final concentration of 2 × 10–4 M.
Procedure: i. In a three-necked flask held over a stir/heat plate, place a stir bar and 100 mL of deionized water, and degas the water by bubbling nitrogen gas through it for 15 min. ii. Maintain a blanket flow of nitrogen through the rest of this procedure. iii. Add 6.2 mg of cadmium nitrate tetrahydrate {Cd[NO3]2•4H2O} and 1.4 μL of mercaptoethanol to the water, with stirring. iv. Insert a pH meter into the flask and check the pH of the aqueous solution. Adjust the pH to 9.8 by adding small amounts of 0.1 M NaOH via a pipet. v. Stir the solution vigorously.
vi. Weigh out 1.6 mg of Na2S and dissolve it in 2 mL of water. Immediately add this solution dropwise to the three-necked flask. The reaction mixture should remain colorless. vii. Continue stirring for 20 min. viii. Adjust the pH of the solution to 10.3 with 0.1 M NaOH. The colorless solution, which glows yellow-green when viewed under UV light, contains CdS nanoparticles surface coated with mercaptoethanol. The nanoparticle diameter should be approx. 4 nm. The solution should be stored in the dark under nitrogen. [In the synthesis of thiol-capped CdS, as in synthesis of 2-mercaptoethanol- capped CdS, other thiols may give different optical properties. For example, we have used L-cysteine as a thiol, and the resulting CdS solution appears pale yellow and glows bright yellow under UV light]
DNA Purification by High-Performance Liquid Chromatography and Annealing • Firstly, decide what sequences of DNA one wishes to probe and choose control DNAs that are allegedly “normal” compared with the “unusual” one that is of interest.  In our experiments, select sequences 5′-GGGTCCTCAGCTTGCC-3′ and complement as a “straight” duplex, 5′-GGTCCAAAAAATTGCC-3′ and complement as a “bent” duplex, the self-complementary 5′- GGTCATGGCCATGACC-3′ as a “kinked” duplex.  Also examined ssDNAs that fold up into unusual structures, such as 5′- CGGCGGCGGCGGCGGCGGCGG-3′, d(CGG)7, and 5′- CCGCCGCCGCCGCCGCCGCCG-3′, d(CCG)7. These are commercially purchased and received as a dried-down pellet (“trityl off”) on a 1-μmol scale.
• Oligonucleotides are purified by high-performance liquid chromatography (HPLC) on a C8 or C18 reverse-phase column with a triethylammonium acetate/acetonitrile gradient, collected and dried down, and redissolved in tris buffer (5 mM tris hydrochloride; 5 mM NaCl, pH 7.2) for duplex DNAs. [The ionic strength of the buffer is lower than that of a typical tris buffer, because the nanoparticles associate electrostatically with the DNA, and a salt concentration that is too high will screen the binding] • The exact nature of the HPLC gradient can vary, depending on the user’s DNA and HPLC. • For annealing duplex DNAs, equal amounts of the complementary single strands are mixed together in Eppendorf tubes and placed in a boiling water bath or a heat block. The heat is turned off and the mixture is allowed to cool down to room temperature.
• Ultraviolet (UV)-visible melting temperature experiments confirm that the duplexes are double stranded (Tm approx 50°C in the stated buffer at approx 1 mM nucleotide concentration). • For annealing unusual ssDNAs into their folded states, the literature must be consulted closely for the proper ionic strength conditions. In the case of the d(CGG) and d(CCG) triplet repeats, which are similarly purified by reverse-phase HPLC, the proper buffer is tris-EDTA. These oligonucleotides are annealed at 90°C in a heating block for 10 min, allowed to cool gradually to room temperature, and then allowed to cool down further to 4°C for 48 h to obtain the properly folded structures, which can be confirmed by circular dichroism spectroscopy and melting temperature experiments.
Titrations of Cd(II)-Activated CdS With Duplex DNAs • Binding of DNA to cationic Cd(II)-activated quantum dots is monitored by photoluminescence spectroscopy. • Then the DNA quenches the emission of nanoparticle solution, and from such data equilibrium binding constants can be obtained.
Procedure: i. Place 200 μL of a 2 × 10–4 M activated CdS solution into a quartz cuvet, and place the cuvet in a spectrofluorometer. Ensure that the size of the excitation light beam in the fluorometer matches the sample size; we have used small 400-μL cuvets instead of the standard 1-cm, 3-mL cuvets. ii. Using an excitation wavelength of 350 nm, which is absorbed by the CdS nanoparticles but not by the DNA, acquire an emission spectrum from 400–800 nm. Slit widths and detector settings will vary by instrument, but for our spectrofluorometer, use 4-nm slits. iii. Take a 5-μL aliquot of an approximately mM (nucleotide) DNA solution in tris buffer and add it to the 200 μL of CdS solution. Mix by inverting the stoppered cuvet several times, and record the emission spectrum. [The ionic strength of the buffer is lower than that of a typical tris buffer, because the nanoparticles associate electrostatically with the DNA, and a salt concentration that is too high will screen the binding]
iv. Wait 30 min, and repeat step 3 until the photoluminescence of the CdS is completely quenched. [It is important during the course of the titration to make sure that equilibrium has been reached at each DNA concentration along the way; hence, the 30-min waiting period between spectra] v. Repeat steps 3 and 4 for different DNAs. Do all of these photoluminescence titrations in a single day, and without changing the spectrofluorometer parameters. vi. Repeat steps 3 and 4 for a buffer solution without DNA, as a control for any loss of photoluminescence intrinsic to the CdS sample. Typically, this is a minor effect. DNA titration experiments with other DNAs in other buffers (e.g., the triplet repeat sequences mentioned in DNA Purification by High-performance liquid chromatography and annealing method) with the proper buffer control can be performed analogously.
Calculations: • To calculate binding constants of the DNA to the nanoparticles, first integrate the areas under the photoluminescence spectra data curves. • From Fig., one could integrate the entire area under the curves from 400 to 800 could use only the “surface-sensitive” peak at 460 nm. In the latter case, integrating the area from approx. 440–510 nm would be appropriate.
Raw photoluminescence titration data for Cd(II) activated CdS nanoparticles Raw photoluminescence titration data for Cd(II)- activated CdS nanoparticles, with a 32mer duplex DNA in tris buffer. The top spectrum is the original Cd(II)-activated CdS data; subsequent addition of DNA decreases the intensity. The peak at approx 570 nm corresponds to the “unactivated” CdS, and the approx 460 nm peak corresponds to the Cd(II)- CdS “activated” species.
• Should buffer alone quench the emission of the nanoparticles more than approx. 5% of the amount of DNA quenching, the DNA data must be corrected. I(corrected) = I(DNA) – I(buffer) I(corrected) = corrected integrated photoluminescence intensity for a given concentration of DNA; I(DNA) = raw integrated intensity for a given concentration of DNA; I(buffer) =raw integrated intensity for the same volume of buffer that goes with the given DNA concentration.
 Frisch-Simha-Eirich (FSE) adsorption isotherm, which physically corresponds to a long polymer adsorbing to a flat surface in short segments, to extract binding constants from our data. Other models, of course, may be used. The FSE isotherm takes the form. [θ exp(2K1θ)]/(1 – θ) = (KC)^1/υ θ = fractional surface coverage of DNA on the nanoparticles, is equated to fractional change in photoluminescence (i.e., θ = [I(DNA) – I0]/[I(DNAfinal) – I0], in which I(DNA) is the corrected integrated intensity of the CdS emission at a particular DNA concentration); I0 = the initial CdS photoluminescence integrated intensity without DNA; I(DNAfinal) = the corrected integrated intensity of the CdS emission at the highest [most quenched] DNA concentration); C = the DNA concentration; K1 is a constant that is a function of the interaction of adsorbed polymer segments, which we manually fit; K = the equilibrium constant for the binding of DNA to the nanoparticle; υ corresponds to the average number of segments attached to the surface, which has no physical meaning in our system, and is allowed to mathematically float.
• Plots of [θ exp(2K1θ)]/(1 – θ), with varying values for K1, vs C are constructed, and fits to a “power” function in the software (Kaleidagraph or Excel) yield values for K and υ. Generally, K1 = 0.5 gives the best fits to our data, and υ does not generally vary much. • With the oligonucleotides, as “straight,” “bent,” or “kinked,” the binding constants, obtained to 4 nm Cd(II)-CdS nanoparticles were 1000, 4200, and 7200 M^–1, respectively.
• In this case, the kinked DNA was thought to have a larger bend angle than the bent DNA, and the trend from our data suggests that the more bent the DNA, the tighter it binds to a curved surface. In the case of triplet repeat DNAs of unknown structures, we observed that they bound to our particles in much higher salt buffers, under conditions in which normal duplex DNA did not bind to the particles. • Suggested, unknown structures either were more able to wrap about a curved surface than duplex DNA, or perhaps were less sensitive to electrostatics in binding to the nanoparticles, possibly because of increased vander Waals interactions.
Conclusion • Semiconductor nanoparticles, also known as quantum dots, are receiving increasing attention for their biological applications. These nanomaterials are photoluminescent and are being developed both as dyes and as sensors. • Structural polymorphism in DNA may serve as a biological signal in-vivo, highlighting the need for recognition of DNA structure in addition to DNA sequence in biotechnology assays. • “Sensors” use of quantum dots to detect different intrinsic DNA structure. Mahtab R.,Murphy C.J. NanoBiotechnology Protocols, Methods in Molecular Biology; Vol 303
Thank you A Biodiction (A Unit of Dr. Divya Sharma)

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Probing of DNA structured with Nanoparticles

  • 1. Probing DNA structure with Nanoparticles: Synthesis and their Different Methods Dr. Divya Sharma Assistant Professor A Biodiction (A Unit of Dr. Divya Sharma)
  • 2. Introduction • In 1950s, double helical structure of DNA has been known • In the 1980s, it has become increasingly recognized that local DNA structure and dynamics can affect its function. • The DNA duplex, as a result of chemical damage or by virtue of its intrinsic sequence, may exhibit bends, loops, bulges, kinks, and other unusual structures on a few-base-pair length scale. • Characterization of local DNA structure can be done, of course, by traditional nuclear magnetic resonance or X-ray crystallographic methods. Mahtab R.,Murphy C.J. NanoBiotechnology Protocols, Methods in Molecular Biology; Vol 303
  • 3. • This article describes the features of the Protein Data Bank, the standard database to search and download crystal structures, NMR structures, and some theoretical structures of biological macromolecules, including DNA: http://www.rcsb.org/pdb/ . • Rutgers University also maintains the Nucleic Acid Database for DNA/RNA sequence and structure searching: http://ndbserver.rutgers.edu/NDB/ndb.html.). • A powerful alternative approach should the DNA samples not be amenable to characterization by these methods is to bind a probe to the DNA target, and use the optical properties of the probe to infer the nature of local DNA structure or dynamics.
  • 4. • Common examples of such probes include fluorescent intercalators & most unusual example of an optical probe for DNA is an inorganic nanoparticle. • Nanoparticles are materials that have diameters on the 1 to 100 nm scale and are therefore in the size range of proteins. • Nanoparticles made of inorganic materials such as semiconductors and metals have unusual, size-dependent optical properties in this size range.
  • 5. • In particular, semiconductor nanoparticles are known as “Quantum dots” because they exhibit “particle-in-a-box” quantum confinement effects at the nanoscale. • CdSe and CdS nanoparticles can be made by a number of routes in the 2 to 8 nm size range, and these nanoparticles are photoluminescent in the visible, with wavelength maxima that depend on size and surface group. • Some researchers have used CdSe quantum dots as inorganic dyes for biological labeling assays. We have used CdS nanoparticles as protein- sized probes of local DNA structure.
  • 6. Methods  Synthesis of “Unactivated” CdS Nanoparticles Stabilized by Polyphosphate  Activation of CdS Nanoparticles With Cd(II)  Synthesis of 2-Mercaptoethanol-Capped CdS  DNA Purification by High-Performance Liquid Chromatography and Annealing  Titrations of Cd(II)-Activated CdS With Duplex DNAs Mahtab R.,Murphy C.J. NanoBiotechnology Protocols, Methods in Molecular Biology; Vol 303
  • 7. Synthesis of “Unactivated” CdS Nanoparticles Stabilized by Polyphosphate • CdS nanoparticles are prepared with reagent weights based on a final concentration of 2 × 10^–4 M . [The quantum dots prepared as described here are not “passivated,” meaning that they are not coated with a material (ZnS, or another higher- band-gap semiconductor, or silica) that will insulate the quantum dot from its environment and render its emission stable and bright regardless of the surrounding medium. In the kind of experiments described here, the intensity of the photoluminescence of the quantum dots should be sensitive to the environment. Hence, control experiments with buffer alone, and standard DNAs, are required].
  • 8. Procedure: i. In a three-necked flask held over a stir/heat plate, place a stir bar and 100 mL of deionized water, and degas the water by bubbling nitrogen gas through it for 15 min. ii. Add 6.2 mg of cadmium nitrate tetrahydrate {Cd[NO3]2•4H2O} to the flask, with stirring. iii. Add 12.1 mg of sodium polyphosphate to the flask, with stirring. iv. Check the pH of the aqueous solution. Adjust the pH to 9.8 by adding small amounts of 0.1 M NaOH via a pipet.
  • 9. v. Stir and add 1.6 mg of anhydrous sodium sulfide (Na2S) and dissolve it in 2 mL of water. Immediately add this solution drop-wise to the three- necked flask. The reaction mixture should become light yellow. vi. Stirring for 20 min vii. Adjust the pH of the solution to 10.3 with 0.1 M NaOH. The reaction has produced approx 4-nm CdS nanoparticles, surface capped with polyphosphate. solution should be stored under nitrogen in the dark. If one irradiates the solution with a UV blacklight, dull pinkish yellow emission will be observed. If one desires to “activate” the nanoparticles with Cd(II), the solution should remain undisturbed for 24 h.
  • 10. Activation of CdS Nanoparticles With Cd(II) • The CdS solution (prepared in first method) should remain undisturbed for 24 h after its synthesis. • Prepared a solution of 0.01 M Cd(NO3)2 tetrahydrate [activates with Zn (II) and Mg (II) as well; the resulting CdS nanoparticles act similarly, but not identically, with DNA]. • Then, monitor the photoluminescence of the unactivated CdS solution. While, adding a solution Cd(NO3)2 tetrahydrate to it. • The CdS solution before activation has an emission peak maximum at approx 550 nm. • As the activation progresses, a new peak appears at approx 440 nm and the intensity of this peak increases.
  • 11. • Addition of Cd(II) is continued until this new peak at 440 nm has reached its maximum intensity. • Toward the end, addition of Cd(II) is done very carefully, and the emission spectrum is checked after each addition of 1 or 2 drops, because if more Cd(II) is added than what is required for maximum activation, the photoluminescence of the activated CdS solution will decrease. • During activation the pH of the solution decreases. After activation is complete, the pH of the solution is brought back to 10.3 with 0.1 M NaOH. • The “activated” CdS solution has a very bright pinkish white glow under UV light. • The nanoparticles should not have changed in size and now are coated with a loose “web” of Cd(II). This activation procedure can be performed with other divalent metal salt solutions as well.
  • 12. Synthesis of 2-Mercaptoethanol-Capped CdS • The synthesis of 2-mercaptoethanol-capped CdS produces nanoparticles that bear ⎯SCH2CH2OH groups that are ionically neutral compared with the probing DNA structure with nanoparticles activated ones. • As before, CdS nanoparticles are prepared with reagent weights based on a final concentration of 2 × 10–4 M.
  • 13. Procedure: i. In a three-necked flask held over a stir/heat plate, place a stir bar and 100 mL of deionized water, and degas the water by bubbling nitrogen gas through it for 15 min. ii. Maintain a blanket flow of nitrogen through the rest of this procedure. iii. Add 6.2 mg of cadmium nitrate tetrahydrate {Cd[NO3]2•4H2O} and 1.4 μL of mercaptoethanol to the water, with stirring. iv. Insert a pH meter into the flask and check the pH of the aqueous solution. Adjust the pH to 9.8 by adding small amounts of 0.1 M NaOH via a pipet. v. Stir the solution vigorously.
  • 14. vi. Weigh out 1.6 mg of Na2S and dissolve it in 2 mL of water. Immediately add this solution dropwise to the three-necked flask. The reaction mixture should remain colorless. vii. Continue stirring for 20 min. viii. Adjust the pH of the solution to 10.3 with 0.1 M NaOH. The colorless solution, which glows yellow-green when viewed under UV light, contains CdS nanoparticles surface coated with mercaptoethanol. The nanoparticle diameter should be approx. 4 nm. The solution should be stored in the dark under nitrogen. [In the synthesis of thiol-capped CdS, as in synthesis of 2-mercaptoethanol- capped CdS, other thiols may give different optical properties. For example, we have used L-cysteine as a thiol, and the resulting CdS solution appears pale yellow and glows bright yellow under UV light]
  • 15. DNA Purification by High-Performance Liquid Chromatography and Annealing • Firstly, decide what sequences of DNA one wishes to probe and choose control DNAs that are allegedly “normal” compared with the “unusual” one that is of interest.  In our experiments, select sequences 5′-GGGTCCTCAGCTTGCC-3′ and complement as a “straight” duplex, 5′-GGTCCAAAAAATTGCC-3′ and complement as a “bent” duplex, the self-complementary 5′- GGTCATGGCCATGACC-3′ as a “kinked” duplex.  Also examined ssDNAs that fold up into unusual structures, such as 5′- CGGCGGCGGCGGCGGCGGCGG-3′, d(CGG)7, and 5′- CCGCCGCCGCCGCCGCCGCCG-3′, d(CCG)7. These are commercially purchased and received as a dried-down pellet (“trityl off”) on a 1-μmol scale.
  • 16. • Oligonucleotides are purified by high-performance liquid chromatography (HPLC) on a C8 or C18 reverse-phase column with a triethylammonium acetate/acetonitrile gradient, collected and dried down, and redissolved in tris buffer (5 mM tris hydrochloride; 5 mM NaCl, pH 7.2) for duplex DNAs. [The ionic strength of the buffer is lower than that of a typical tris buffer, because the nanoparticles associate electrostatically with the DNA, and a salt concentration that is too high will screen the binding] • The exact nature of the HPLC gradient can vary, depending on the user’s DNA and HPLC. • For annealing duplex DNAs, equal amounts of the complementary single strands are mixed together in Eppendorf tubes and placed in a boiling water bath or a heat block. The heat is turned off and the mixture is allowed to cool down to room temperature.
  • 17. • Ultraviolet (UV)-visible melting temperature experiments confirm that the duplexes are double stranded (Tm approx 50°C in the stated buffer at approx 1 mM nucleotide concentration). • For annealing unusual ssDNAs into their folded states, the literature must be consulted closely for the proper ionic strength conditions. In the case of the d(CGG) and d(CCG) triplet repeats, which are similarly purified by reverse-phase HPLC, the proper buffer is tris-EDTA. These oligonucleotides are annealed at 90°C in a heating block for 10 min, allowed to cool gradually to room temperature, and then allowed to cool down further to 4°C for 48 h to obtain the properly folded structures, which can be confirmed by circular dichroism spectroscopy and melting temperature experiments.
  • 18. Titrations of Cd(II)-Activated CdS With Duplex DNAs • Binding of DNA to cationic Cd(II)-activated quantum dots is monitored by photoluminescence spectroscopy. • Then the DNA quenches the emission of nanoparticle solution, and from such data equilibrium binding constants can be obtained.
  • 19. Procedure: i. Place 200 μL of a 2 × 10–4 M activated CdS solution into a quartz cuvet, and place the cuvet in a spectrofluorometer. Ensure that the size of the excitation light beam in the fluorometer matches the sample size; we have used small 400-μL cuvets instead of the standard 1-cm, 3-mL cuvets. ii. Using an excitation wavelength of 350 nm, which is absorbed by the CdS nanoparticles but not by the DNA, acquire an emission spectrum from 400–800 nm. Slit widths and detector settings will vary by instrument, but for our spectrofluorometer, use 4-nm slits. iii. Take a 5-μL aliquot of an approximately mM (nucleotide) DNA solution in tris buffer and add it to the 200 μL of CdS solution. Mix by inverting the stoppered cuvet several times, and record the emission spectrum. [The ionic strength of the buffer is lower than that of a typical tris buffer, because the nanoparticles associate electrostatically with the DNA, and a salt concentration that is too high will screen the binding]
  • 20. iv. Wait 30 min, and repeat step 3 until the photoluminescence of the CdS is completely quenched. [It is important during the course of the titration to make sure that equilibrium has been reached at each DNA concentration along the way; hence, the 30-min waiting period between spectra] v. Repeat steps 3 and 4 for different DNAs. Do all of these photoluminescence titrations in a single day, and without changing the spectrofluorometer parameters. vi. Repeat steps 3 and 4 for a buffer solution without DNA, as a control for any loss of photoluminescence intrinsic to the CdS sample. Typically, this is a minor effect. DNA titration experiments with other DNAs in other buffers (e.g., the triplet repeat sequences mentioned in DNA Purification by High-performance liquid chromatography and annealing method) with the proper buffer control can be performed analogously.
  • 21. Calculations: • To calculate binding constants of the DNA to the nanoparticles, first integrate the areas under the photoluminescence spectra data curves. • From Fig., one could integrate the entire area under the curves from 400 to 800 could use only the “surface-sensitive” peak at 460 nm. In the latter case, integrating the area from approx. 440–510 nm would be appropriate.
  • 22. Raw photoluminescence titration data for Cd(II) activated CdS nanoparticles Raw photoluminescence titration data for Cd(II)- activated CdS nanoparticles, with a 32mer duplex DNA in tris buffer. The top spectrum is the original Cd(II)-activated CdS data; subsequent addition of DNA decreases the intensity. The peak at approx 570 nm corresponds to the “unactivated” CdS, and the approx 460 nm peak corresponds to the Cd(II)- CdS “activated” species.
  • 23. • Should buffer alone quench the emission of the nanoparticles more than approx. 5% of the amount of DNA quenching, the DNA data must be corrected. I(corrected) = I(DNA) – I(buffer) I(corrected) = corrected integrated photoluminescence intensity for a given concentration of DNA; I(DNA) = raw integrated intensity for a given concentration of DNA; I(buffer) =raw integrated intensity for the same volume of buffer that goes with the given DNA concentration.
  • 24.  Frisch-Simha-Eirich (FSE) adsorption isotherm, which physically corresponds to a long polymer adsorbing to a flat surface in short segments, to extract binding constants from our data. Other models, of course, may be used. The FSE isotherm takes the form. [θ exp(2K1θ)]/(1 – θ) = (KC)^1/υ θ = fractional surface coverage of DNA on the nanoparticles, is equated to fractional change in photoluminescence (i.e., θ = [I(DNA) – I0]/[I(DNAfinal) – I0], in which I(DNA) is the corrected integrated intensity of the CdS emission at a particular DNA concentration); I0 = the initial CdS photoluminescence integrated intensity without DNA; I(DNAfinal) = the corrected integrated intensity of the CdS emission at the highest [most quenched] DNA concentration); C = the DNA concentration; K1 is a constant that is a function of the interaction of adsorbed polymer segments, which we manually fit; K = the equilibrium constant for the binding of DNA to the nanoparticle; υ corresponds to the average number of segments attached to the surface, which has no physical meaning in our system, and is allowed to mathematically float.
  • 25. • Plots of [θ exp(2K1θ)]/(1 – θ), with varying values for K1, vs C are constructed, and fits to a “power” function in the software (Kaleidagraph or Excel) yield values for K and υ. Generally, K1 = 0.5 gives the best fits to our data, and υ does not generally vary much. • With the oligonucleotides, as “straight,” “bent,” or “kinked,” the binding constants, obtained to 4 nm Cd(II)-CdS nanoparticles were 1000, 4200, and 7200 M^–1, respectively.
  • 26. • In this case, the kinked DNA was thought to have a larger bend angle than the bent DNA, and the trend from our data suggests that the more bent the DNA, the tighter it binds to a curved surface. In the case of triplet repeat DNAs of unknown structures, we observed that they bound to our particles in much higher salt buffers, under conditions in which normal duplex DNA did not bind to the particles. • Suggested, unknown structures either were more able to wrap about a curved surface than duplex DNA, or perhaps were less sensitive to electrostatics in binding to the nanoparticles, possibly because of increased vander Waals interactions.
  • 27. Conclusion • Semiconductor nanoparticles, also known as quantum dots, are receiving increasing attention for their biological applications. These nanomaterials are photoluminescent and are being developed both as dyes and as sensors. • Structural polymorphism in DNA may serve as a biological signal in-vivo, highlighting the need for recognition of DNA structure in addition to DNA sequence in biotechnology assays. • “Sensors” use of quantum dots to detect different intrinsic DNA structure. Mahtab R.,Murphy C.J. NanoBiotechnology Protocols, Methods in Molecular Biology; Vol 303
  • 28. Thank you A Biodiction (A Unit of Dr. Divya Sharma)