RESUMO
Compaction of calf thymus DNA (ct-DNA) by two cationic gemini surfactants, 12-4-12 and 12-8-12, in the absence and presence of negatively charged SiO2 nanoparticles (NPs) (â¼100 nm) has been explored using various techniques. 12-8-12 having a longer hydrophobic spacer induces a greater extent of ct-DNA compaction than 12-4-12, which becomes more efficient with SiO2 NPs. While 50% ct-DNA compaction in the presence of SiO2 NPs occurs at â¼77 nM of 12-8-12 and â¼130 nM of 12-4-12, but a conventional counterpart surfactant, DTAB, does it at its concentration as high as â¼7 µM. Time-resolved fluorescence anisotropy measurements show changes in the rotational dynamics of a fluorescent probe, DAPI, and helix segments in the condensed DNA. Fluorescence lifetime data and ethidium bromide exclusion assays reveal the binding sites of surfactants to ct-DNA. 12-8-12 with SiO2 NPs has shown the highest cell viability (≥90%) and least cell death in the human embryonic kidney (HEK) 293 cell lines in contrast to the cell viability of ≤80% for DTAB. These results show that 12-8-12 with SiO2 NPs has the highest time and dose-dependent cytotoxicity compared to 12-8-12 and 12-4-12 in the murine breast cancer 4T1 cell line. Fluorescence microscopy and flow cytometry are performed for in vitro cellular uptake of YOYO-1-labeled ct-DNA with surfactants and SiO2 NPs using 4T1 cells after 3 and 6 h incubations. The in vivo tumor accumulation studies are carried out using a real-time in vivo imaging system after intravenous injection of the samples into 4T1 tumor-bearing mice. 12-8-12 with SiO2 has delivered the highest amount of ct-DNA in cells and tumors in a time-dependent manner. Thus, the application of a gemini surfactant with a hydrophobic spacer and SiO2 NPs in compacting and delivering ct-DNA to the tumor is proven, warranting its further exploration in nucleic acid therapy for cancer treatment.
Assuntos
Nanopartículas , Dióxido de Silício , Humanos , Animais , Camundongos , Dióxido de Silício/química , Tensoativos/química , Células HEK293 , DNA/genética , DNA/química , Nanopartículas/químicaRESUMO
The present work elucidates binding interactions of sodium dodecyl sulphate (SDS) with the conjugated gold nanoparticles (AuNPs)-bovine serum albumin (BSA), unfolded by each of two gemini surfactants, 1,4-bis(dodecyl-N,N-dimethylammonium bromide)-butane (12-4-12,2Br-) or 1,8-bis(dodecyl-N,N-dimethylammonium bromide)-octane (12-8-12,2Br-). Initially, at a low concentration of SDS there is a relaxation of bioconjugates from their compressed form due to the formation of catanions between SDS and gemini surfactants. On moving towards higher concentrations of SDS, these relaxed unfolded bioconjugates renature by removal of residual bound gemini surfactants. Mixed assemblies of SDS and gemini surfactants formed during refolding of bioconjugates are characterized by DLS and FESEM measurements. A step-by-step process of refolding observed for these denatured protein bioconjugates is exactly the inverse of their unfolding phenomenon. Parameters concerning nanometal surface energy transfer (NSET) and Förster's resonance energy transfer (FRET) phenomenon were employed to develop a binding isotherm. Moreover, there remains an inverse relationship between α-helix and ß-turns of bioconjugates during the refolding process. Significantly, in the presence of 12-8-12,2Br-, SDS induces more refolding as compared to that for 12-4-12,2Br-. Bioconjugation shows an effect on the secondary structures of refolded BSA, which has been explored in detail through various studies such as Fourier transform infrared spectroscopy, fluorescence, and circular dichroism (CD). Therefore, this approach vividly describes the refolding of denatured bioconjugates, exploring structural information regarding various catanions formed during the process that would help in understanding distance-dependent optical biomolecular detection methodologies and physicochemical properties.
RESUMO
This work demonstrates binding interactions of two cationic gemini surfactants, 12-4-12,2Br- and 12-8-12,2Br- with gold nanoparticles (AuNPs)-conjugated bovine serum albumin (BSA) presenting binding isotherms from specific binding to saturation binding regions of surfactants. The binding isotherm has been successfully constructed using Förster's resonance energy transfer (FRET) and nanometal surface energy transfer (NSET) parameters calculated based on fluorescence quenching of donor, tryptophan (Trp) residue by acceptor, AuNP. Energy transfer efficiency (ET) changes due to alteration in the donor-acceptor distance when surfactants interact with bioconjugates. A solid reverse relationship between α-helix and ß-turn contents of BSA-AuNPs-conjugates is noted while interacting with surfactants. 12-8-12,2Br- shows stronger binding interactions with BSA-bioconjugates than 12-4-12,2Br-. The effect of bioconjugation on secondary/tertiary structures of BSA in the absence and presence of a surfactant is studied through circular dichroism, fluorescence, and Fourier transform infrared spectroscopic measurements. Motional restrictions imposed by AuNPs on Trp residues of folded and unfolded BSA have been investigated using red edge emission shift (REES) measurements. Finally, the molecular docking results present the modes of interactions of 12-4-12,2Br- and 12-8-12,2Br-, and Au-nanoclusters (Au92) with BSA. An approach to describe the binding isotherms of surfactants using AuNPs-bioconjugates as optical-based molecular ruler and possible effects of AuNPs on microenvironment and conformations of the protein is presented.
Assuntos
Ouro/química , Nanopartículas Metálicas/química , Simulação de Acoplamento Molecular/métodos , Análise Espectral/métodos , Tensoativos/química , Cátions , Microscopia Eletrônica de Transmissão e VarreduraRESUMO
The present work highlights the effect of urea on solvation dynamics and the rotational relaxation of Coumarin 480 (C-480) in the Stern layer of aqueous micelles of cationic gemini surfactants, 12-4(OH) n -12 (n = 0, 1, 2). UV-visible absorption, steady-state fluorescence and fluorescence anisotropy, time-resolved fluorescence and fluorescence anisotropy, and dynamic light scattering measurements have been carried out for this study. The formation of micelles becomes disfavored in the presence of urea at high concentration. Solvation dynamics is bimodal in nature with fast solvation as a major component. The average solvation time increases, reaches a maximum, and then decreases with increasing concentration of urea because the degree of counterion dissociation also follows the same order with the addition of urea in the micellar solution. With increased degree of counterion dissociation, the extent of clustering of water molecules is increased, resulting in slower solvation process. The -OH group present in the spacer group of gemini surfactant controls the rate of solvation by shielding the water molecules from the probe molecules forming hydrogen bond. The microviscosity of micelles is decreased with increasing concentration of urea, as a result of which the rotational relaxation process becomes faster. In the presence of the -OH group in the spacer group, the microviscosity of micelles is enhanced, resulting in longer rotational relaxation time. Rotational relaxation process is bimodal in nature with the major contribution from the fast component to the fluorescence depolarization. Slow rotational relaxation is mainly due to the lateral diffusion of C-480 molecules along the surface of the micelle. The tumbling motion of the micelle as a whole is much slower than the lateral diffusion of C-480. Wobbling motion of C-480 becomes faster with increasing concentration of urea as a result of decreased microviscosity of micelles. The alignment of C-480 molecules in micelles might change with changing microviscosity.
RESUMO
The binding interactions of three gemini surfactants having different spacer groups (12-4-12, 12-8-12, and 12-4(OH)-12) with a high concentration (150 µM) of bovine serum albumin (BSA) at various regions of binding isotherms have been studied by means of steady-state fluorescence and fluorescence anisotropy, time-correlated single-photon counting fluorescence of trans-2-[4-(dimethylamino)styryl]benzothiazole, small-angle neutron scattering (SANS), and dynamic light scattering (DLS) measurements. The fluorescence resonance energy transfer phenomenon between the twisted intramolecular charge transfer fluorescent molecule, trans-2-[4-(dimethylamino)styryl]benzothiazole as an acceptor, and tryptophan 213 (Trp-213) of BSA as a donor has been successfully used to probe the binding interactions of gemini surfactants with protein at all regions of binding isotherms. The increasing order of energy transfer efficiency at a higher concentration range of surfactants is 12-8-12 > 12-4-12 > 12-4(OH)-12. Stronger binding of micelles of gemini surfactant molecules having a comparatively more hydrophobic spacer group with the hydrophobic segments of the protein results in closer approach of trans-2-[4-(dimethylamino)styryl]benzothiazole molecules solubilized in micelles to Trp-213. The average excited-state lifetimes become shorter with a trend of increase in contribution from the fast component and decrease in contribution from the slow component to the decay with increasing concentration of a surfactant. The nonradiative rate constant of trans-2-[4-(dimethylamino)styryl]benzothiazole increases with increasing concentration of a surfactant because the average microenvironment around it in protein-surfactant aggregates is more polar as compared to that in native protein. SANS and DLS measurements were carried out for the study of the structural deformations in the protein, on enhancement of the concentration of the gemini surfactants. The necklace and bead model has been used for the analysis of SANS data for the protein-surfactant complexes. At a higher concentration range, 12-8-12 and 12-4-12 have a slightly smaller fractal dimension and a larger correlation length as compared to 12-4(OH)-12. DLS data show that the increasing order of hydrodynamic diameter for the complexes of protein with three gemini surfactants in their high concentration range is 12-4(OH)-12 < 12-4-12 < 12-8-12.
RESUMO
Solvation dynamics and rotational relaxation of coumarin 480 in aqueous micelles of cationic gemini surfactants with diethyl ether (EE) spacer group (m-EE-m) and tails with varying tail lengths (m = 12, 14, and 16) have been studied. Studies have been carried out by measuring UV-visible absorption, steady-state fluorescence and fluorescence anisotropy, time-resolved fluorescence and fluorescence anisotropy, 1H NMR spectroscopy, and dynamic light scattering. Effects of hydrocarbon tail length and hydrophilicity of spacer group on solvation dynamics and rotational relaxation processes at inner side of the Stern layer of micelles have been studied. With increasing hydrophobicity of tails of surfactants, water molecules in the Stern layer become progressively more rigid, resulting in a decrease in the rate of solvation process with slow solvation as a major component. With increasing hydrophilicity of the spacer group of gemini surfactant, the extent of free water molecules is decreased, thereby making the duration of the solvation process longer. Solvation times in the micelles of gemini surfactants with hydrophilic spacer are almost 4 times longer compared to those in the micelles of their conventional counterpart. Rotational relaxation time increases with increasing tail length of surfactant as a result of increasing microviscosity of micelles with fast relaxation as a major component. With increasing hydrophilicity of the spacer group, the anisotropy decay becomes slower due to the formation of more compact micelles. Rotational relaxation in gemini micelles is also slower compared to that in their conventional counterpart. The anisotropy decay is found to be biexponential with lateral diffusion of the probe along the surface of the micelle as a slow component. Rotational motion of micelle as a whole is a very slow process, and the motion becomes further slower with increasing size of the micelle. The time constants for wobbling motion and lateral diffusion of the probe become longer with increasing microviscosity of micelles.
RESUMO
Solvation dynamics and rotational relaxation of coumarin 153 (C-153) in mixed micelles of non-ionic surfactant, Triton X-100 and a series of cationic gemini surfactants, 12-s-12, 2Br with varying polymethylene spacer chain length (s = 3, 6, 8, 12) at different bulk mole fractions of a surfactant were studied. Studies were carried out by means of UV-Vis absorption, steady-state fluorescence and fluorescence anisotropy, time-resolved fluorescence and fluorescence anisotropy, and dynamic light scattering measurements. While micropolarity of the environment around C-153 in mixed micelles increased, the microviscosity decreased with increasing amount of a gemini surfactant. This is because the thickness of the Stern layer of micelles increases as a result of greater extent of penetration of water molecules. Solvation dynamics and rotational relaxation of C-153 become faster with increasing mole fraction of a gemini surfactant in the mixed micelles. Increasing the thickness of the Stern layer leads to an increase in the number of water molecules hydrogen bonded among themselves, resulting in an increase in polarity and microfluidity of the environment. At a given bulk mole fraction of a surfactant, the microviscosity of micelles decreases with increasing the spacer chain length of the gemini surfactant resulting in an increase in the rate of the rotational relaxation process. However, at a given bulk mole fraction of a surfactant, solvation dynamics becomes slower with increasing spacer chain length from s = 3 to 8 because of the increasing degree of counter ion dissociation. The slow rotational relaxation process is mainly due to the lateral diffusion of C-153 along the surface of the micelles. Rotationalmotion of the micelle as a whole is much slower than the lateral diffusion of C-153.
RESUMO
The present work demonstrates the solvation dynamics and rotational relaxation of Coumarin 153 (C-153) in the micelles of a series of cationic gemini surfactants, 12-s-12, 2Br(-) containing a hydrophobic polymethylene spacer with s = 3, 4, 6, 8, 12. Steady-state and time-correlated single-photon counting (TCSPC) fluorescence spectroscopic techniques have been used to carry out this study. Steady-state and TCSPC fluorescence data suggest that C-153 molecules are located at the Stern layer of micelles. While probe molecules feel more or less the same micropolarity in the micellar phase, the microviscosity of micelles decreases with spacer chain length. Solvation dynamics at the Stern layer is bimodal in nature with fast solvation as a major component. Counter ions and water molecules bonded with the polar headgroups of surfactant molecules are responsible for the slow component. Average solvation time increases with spacer chain length because of the increased degree of counter ion dissociation. Some water molecules are involved in the solvation of counter ions themselves, resulting in the decrease in "free" water molecules to be available for the solvation of C-153. The hydrophobic spacer chain also has an effect on increasing the solvation time with increasing chain length. The average rotational relaxation time for C-153 decreases with spacer chain length with a rapid decrease at s > 4. The anisotropy decay of C-153 in micelles is biexponential in nature. The slow rotational relaxation is due to the lateral diffusion of C-153 in micelles. Lateral diffusion is much faster than the rotational motion of a micelle as a whole. The rotational motion of the micelle as a whole becomes faster with the decreasing size of micelles.
Assuntos
Calcitriol/análogos & derivados , Cumarínicos/química , Micelas , Rotação , Solventes/química , Tensoativos/química , Água/química , Anisotropia , Calcitriol/química , Propriedades de Superfície , ViscosidadeRESUMO
The solvation dynamics and rotational relaxation of Coumarin 480 (C-480) have been investigated in the micelles of a series of gemini surfactants, 12-4(OH)n-12 (n = 0, 1, and 2), with increasing hydroxyl group substitution within the spacer group. Steady-state and time-correlated single photon counting (TCSPC) fluorescence spectroscopic techniques have been used to carry out such study. Steady-state and TCSPC fluorescence data support the location of probe molecule at the Stern layer. The solvation dynamics is found to be slower on hydroxyl substitution of spacer group due to the formation of hydrogen bonds between water molecules and hydroxyl group(s) of spacer group. Such kind of hydrogen bonding protects the probe molecule from its contact with water molecules and also results in restricted mobility of water molecules. The average rotational relaxation time increases on increasing number of substituted hydroxyl group on a spacer group. It is because of formations of more and more close packed micelles and larger extent of intermolecular hydrogen bonding interactions between C-480 and hydroxyl group(s). For micelles of each of 12-4-12 and 12-4(OH)-12, the slow rotational relaxation is dominated by the lateral diffusion of the fluorophore along the spherical surface of the micelle. However, for 12-4(OH)2-12, the slow rotational relaxation is mainly due to the rotational motion of the micelle as a whole. Because of high microviscosity of micelles of 12-4(OH)2-12 and greater extent of hydrogen bonding interactions with C-480, the relaxation time corresponding to the lateral diffusion of the fluorophore is very high in this case.
Assuntos
Cumarínicos/química , Hidróxidos/química , Micelas , Quinolizinas/química , Tensoativos/química , Cátions/química , Ligação de Hidrogênio , Solventes/química , Espectrometria de Fluorescência , Propriedades de Superfície , Água/químicaRESUMO
The dipolar nature of trans-2-[4-(dimethylamino)styryl]benzothiazole (DMASBT) in its twisted intramolecular charge transfer (TICT) excited state makes it useful as a surface probe for phenomena such as premicellar and micellar aggregation of non-ionic Brij surfactants. The process of micellization of Brij 35, Brij 58, Brij 78, and Brij 98 through the formation of smaller premicellar aggregates results in a progressive change in the nature of the DMASBT molecule and its location in the aggregates, reflecting the changes in its photophysical properties, which have been studied using steady-state fluorescence, fluorescence anisotropy, and time-correlated single-photon counting measurements. The microenvironment polarity around the DMASBT probe in the micellar phase is greater than that in corresponding premicellar phases. The orders of premicellar as well as micellar concentrations are Brij 35 > Brij 58 > Brij 98 > Brij 78. The lower fluorescence anisotropies observed in the case of Brij 78 aggregates compared to those in other Brijs studied could be due to the accessibility of a nonrigid environment as a result of a folded conformation of a part of the nonpolar long chain of surfactant molecules near the core of aggregates. Three different locations of DMASBT were noted for Brijs 35, Brij 78, and Brij 98, whereas for Brij 58 only two locations are observed. The micropolarity of the environment around DMASBT in aggregation states has been determined.
Assuntos
Corantes Fluorescentes/química , Tensoativos/química , Benzotiazóis/química , Micelas , Espectrometria de Fluorescência , Estirenos/químicaRESUMO
The guest-host concentration has already been proved to be a very important factor in the drug delivery process. In the present work we demonstrate the formation of compound induced gamma-cyclodextrin nanotubular suprastructure. The nanotubes formed are found to be highly sensitive to the concentration of the guest molecule. The increasing concentration of the compound in solution initiates a competition toward their existence inside the core of the nanotubes affecting the extent of nanotubular cluster formation. The hydrogen bonding responsible for the building of the cyclodextrin nanotubes is found to be partially disrupted because of this increasing competition. The continuous replacement of the guest molecules inside the nanochannels is supposed to be responsible for the instability in some of the hydrogen bondings that develop during the primary and the secondary interactions between the formed nanotubes resulting into fragmentation of the suprastructures. The steady state and time-resolved fluorescence experiments coupled with fluorescence anisotropy and atomic force microscopy illustrate the guest concentration dependence of the formation of the gamma-cyclodextrin nanotubes.
Assuntos
Sistemas de Liberação de Medicamentos , Nanotubos , gama-Ciclodextrinas/química , Microscopia de Força Atômica , Estrutura Molecular , Espectrometria de FluorescênciaRESUMO
Photophysical changes of a cylindrical compound undergoing twisted intramolecular charge transfer may be used as a surface probe to study the different phases of premicellar aggregate formation. The probe molecule, trans-2-[4-(dimethylamino)styryl] benzothiazole (DMASBT), attaches itself to the premicellar and the micellar aggregates of cationic, anionic, and neutral surfactants in different orientations because of its dipolar nature in the excited state. The micelle formation is preceded by a few typical rearrangements of the surfactant molecules. These events need proper inspection that can only be done by compounds that sense environmental changes by residing in the vicinity of the surface of those aggregates. Steady-state and time-resolved fluorescence spectroscopy coupled with steady-state fluorescence anisotropy measurements serve as a very useful tool to monitor premicellar aggregate formation. The dipolar interaction of DMASBT with the surface of the aggregate and its extraordinary capability to sense the polarity of the environment make it a very efficient molecule to use for the purpose.