Toward Understanding the Binding Synergy of Trastuzumab and Pertuzumab to Human Epidermal Growth Factor Receptor 2.

Human epidermal growth factor receptor 2 (HER2) is overexpressed in breast, gastric, esophageal, ovarian, and endometrial cancer. Combination therapy using trastuzumab and pertuzumab antibodies targeting HER2 has shown better survival outcomes in breast cancer patients. In the quest to understand the synergistic effect observed due to combination therapy, trastuzumab, pertuzumab, and their F(ab')2 fragments were labeled with radioisotope and fluorescent probes. Detailed in vitro studies to understand binding synergism in HER2 overexpressing cell lines were done. Antibodies and their F(ab')2 fragments prepared by enzyme digestion with pepsin were radiolabeled with iodine-125. In vitro binding studies to evaluate immunoreactivity, specificity, affinity, and binding synergism between radiolabeled trastuzumab, pertuzumab, and their F(ab')2 fragments were carried out. Synergism was observed by 20-30% enhanced uptake of radiolabeled pertuzumab and its F(ab')2 fragments in the presence of excess of unlabeled trastuzumab or F(ab')2-trastuzumab. However, uptake of radiolabeled trastuzumab was not enhanced in the presence of excess pertuzumab or its fragments; rather inhibition or competition in binding to HER2 was observed. Studies using fluorescent antibodies by flow cytometry confirmed enhanced binding of pertuzumab in the presence of trastuzumab. Live cell tracking was done to give insights into the binding synergy and fate of fluorescent antibodies . Colocalization of antibodies on HER2 followed by internalization in the cells was observed. The radiolabeled immunoconjugates served as an important tool for experimental characterization of interaction between pertuzumab and trastuzumab to HER2. Studies with fluorescent antibodies corroborated the binding data and provided evidence of colocalization and internalization of both the antibodies in HER2-positive cells.

Determining Metal Ion Complexation Kinetics with Fluorescent Ligands by Using Fluorescence Correlation Spectroscopy.

Fluorescence correlation spectroscopy (FCS) has been extensively used to measure equilibrium binding constants (K) or association and dissociation rates in many reversible chemical reactions across chemistry and biology. For the majority of investigated reactions, the binding constant was on the order of ∼100 M-1 , with dissociation constants faster or equal to 103  s-1 , which ensured that enough association/dissociation events occur during the typical diffusion-determined transition time of molecules through the FCS detection volume. However, complexation reactions involving metal ions and chelating ligands exhibit equilibrium constants exceeding 104  M-1 . In the present paper, we explore the applicability of FCS for measuring reaction rates of such complexation reactions, and apply it to binding of iron, europium and uranyl ions to a fluorescent chelating ligand, calcein. For this purpose, we exploit the fact that the ligand fluorescence becomes strongly quenched after binding a metal ion, which results in strong intensity fluctuations that lead to a partial correlation decay in FCS. We also present measurements for the strongly radioactive ions of 241 Am3+ , where the extreme sensitivity of FCS allows us to work with sample concentrations and volumes that exhibit close to negligible radioactivity levels. A general discussion of the applicability of FCS to the investigation of metal-ligand binding reactions concludes our paper.

Single-Molecule Orientation Imaging Reveals Two Distinct Binding Configurations on Amyloid Fibrils.

Fluorescence readouts for an amyloid fibril sensor critically depend on its molecular interaction and local environment offered by the available structural motifs. Here we employ polarized points accumulation for imaging in nanoscale topography with intramolecular charge transfer probes transiently bound to amyloid fibrils to investigate the organization of fibril nanostructures and probe binding configurations. Besides the in-plane (θ ≈ 90°) mode for binding on the fibril surface parallel to the long fibril axis, we also observed a sizable population of over 60% out-of-plane (θ < 60°) dipoles for rotor probes experiencing a varying degree of orientational mobility. Highly confined dipoles exhibiting an out-of-plane configuration probably reflect tightly bound dipoles in the inner channel grooves, while the weakly bound ones on amyloid enjoy rotational flexibility. Our observation of an out-of-plane binding mode emphasizes the pivotal role played by the electron donor amino group toward fluorescence detection and hence the emergence of anchored probes alongside conventional groove binders.

Inter-molecular interaction kinetics: tale of photon anti-bunching and bunching in fluorescence correlation spectroscopy (FCS).

Molecular interactions are fundamental to any chemical or biological processes, and their rates define the operational sequence and control for any desirable product. Here, we deliberate on a recently developed novel fluorescence spectroscopic method, which combines fluorescence photon anti-bunching, photon bunching, time-correlated single-photon counting (TCSPC), and steady-state fluorescence spectroscopy, to study composite chemical reactions with single molecule sensitivity. The proposed method captures the full picture of the multifaceted quenching kinetics, which involves static quenching by ground state complexation and collisional quenching in the excited state under dynamic exchange of fluorophore in a heterogeneous media, and which cannot be seen by steady-state or lifetime measurements alone. Photon correlation in fluorescence correlation spectroscopy (FCS) provides access to interrogate interaction dynamics from picosecond to seconds, stitching all possible stages of dye-quencher interaction in a micellar media. This is not possible with the limited time window available to conventional ensemble techniques like TCSPC, flash photolysis, transient absorption, stop-flow, etc. The basic premises of such unified global analysis and sanctity of extracted parameters critically depends on the minimum but precise description of reaction scheme, for which careful inspection of ensemble spectroscopy data for photo-physical behaviour is very important. Though in this contribution we discussed and demonstrated the merits of photon antibunching and bunching spectroscopy for dye-quencher interaction in cationic cetyltrimethylammonium bromide (CTAB) micellar solution by photo-induced electron transfer mechanism and the influence of micellar charge and microenvironment on the interaction kinetics, but in principal similar arguments are equally applicable to any other interaction mechanisms which alter fluorescence photon correlations, like Förster resonance energy transfer (FRET), proton transfer, isomerisation, etc.

Confined ultrafast torsional dynamics of Thioflavin-T in a nanocavity.

The influence of confinement in the supramolecular ß-cyclodextrin nanocavity on the excited state torsional dynamics of the amyloid fibril sensor, Thioflavin-T, is explored using subpicosecond fluorescence up-conversion spectroscopy. In the presence of ß-cyclodextrin, the emission intensity and the fluorescence lifetime of Thioflavin-T significantly increases, indicating the confinement effect of the nanocage on the photophysical behaviour of the dye. Detailed time-resolved fluorescence studies show an appreciable dynamic Stokes' shift for the dye in the ß-cyclodextrin nanocavity. Analysis of the time-resolved area normalized emission spectra (TRANES) indicates the formation of an emissive TICT state. The rate of formation of the TICT state, as calculated from the time dependent changes in the peak frequency and the width of the emission spectra, is found to be substantially slower in the ß-cyclodextrin nanocavity compared to that in bulk water. Present results indicate that ultrafast torsional motion in Thioflavin-T is significantly retarded due to confinement by the ß-cyclodextrin nanocavity.

Picosecond to Second Fluorescence Correlation Spectroscopy for Studying Solute Exchange and Quenching Dynamics in Micellar Media.

Numerous studies have been devoted to understand the reaction kinetics in micelles, where the accessible kinetic time window is often limited by the dynamic range of the employed spectroscopic technique. This is usually accompanied by a selection of probes that comfortably explore time scales where slow solute exchange kinetics is negligible, as compared to the fast excited state reactions. This has led to an undervaluation of the role played by dynamic partitioning of hydrophilic solutes in microheterogeneous media. Here, we employ fluorescence correlation spectroscopy (FCS) and the zwitterionic dye Rhodamine 110 to quantitatively explore the impact of solute exchange on the photoinduced electron transfer between this dye and N,N-dimethylaniline in micellar media. Our study elucidates the coupling and interplay between the kinetics of photophysics, quenching, and solute exchange through a quantitative unified molecular-state quenching-kinetic model that describes the steady-state ensemble and FCS data from subnanosecond photon antibunching to millisecond diffusions.

Identifying the bond responsible for the fluorescence modulation in an amyloid fibril sensor.

An ultrafast intramolecular bond twisting process is known to be the responsible mechanism for the sensing activity of the extensively used amyloid fibril sensor thioflavin T (ThT). However, it is not yet known which one of the two possible single bonds in ThT is actually involved in the twisting process. To resolve this fundamental issue, two derivatives of ThT have been designed and synthesized and subsequently their photophysical properties have been studied in different solvents. It is understood from the present study that the rotation around the central C-C single bond, and not that around the C-N single bond, is primarily responsible for the sensor activity of ThT. Detailed viscosity-dependent fluorescence studies revealed that the ThT derivative with restricted C-N bond rotation acts as a better sensor than the derivative with free C-N bond rotation. The better sensory activity is directly correlated with a shorter excited-state lifetime. Results obtained from the photophysical studies of the ThT derivatives have also been supported by the results obtained from quantum chemical calculations.

Binding Constant Determined from the Angstrom-Scale Change in Hydrodynamic Radius of Transferrin upon Binding with Europium Using Dual-Focus Fluorescence Correlation Spectroscopy.

Monitoring the binding of a large fluorescently tagged molecule to a small solute by fluorescence correlation spectroscopy (FCS) is rather uncommon because the binding-related change in diffusion coefficient is very small. Here, we use a high-precision variant of FCS, namely, dual-focus FCS (2fFCS), for measuring the angstrom-scale change of the hydrodynamic radius of the bilobal metal transport protein transferrin (Tf) upon binding europium ions. Applying a sequential 1:2 complexation model, we use these measurements for determining the binding constants (K). Our results show a 0.7 Å change of the protein's hydrodynamic radius upon 1:1 Tf-Eu complex formation and a second change of 1.8 Å upon subsequent binding of a second europium ion. More than one unit variation in logK indicates an intrinsic dissimilarity in metal affinity of the C- and N-lobes of Tf, which agrees well with earlier reported ensemble spectroscopy results.

Ruthenium(II) complexes of bipyridine-glycoluril and their interactions with DNA.

Nine complexes of the type [Ru(N-N)(2)(BPG)]Cl(2) 1-4, [Ru(N-N)(BPG)(2)]Cl(2) 5-8, and [Ru(BPG)(3)]Cl(2) 9 where N-N is 2,2'-bipyridine (bpy), 1,10-phenanthroline (phen), dipyrido[3,2-d:2',3'-f]quinoxaline (dpq), dipyrido[3,2-a:2',3'-c]phenazine (dppz), which incorporates bipyridine-glycoluril (BPG-4b,5,7,7a-tetrahydro-4b,7a-epiminomethanoimino-6H-imidazo[4,5-f][1,10]phenanthroline-6,13-dione) as the ancillary ligand, have been synthesized and characterized. These complexes with the peripheral polypyridyl ligands have the ability to form conjugates with DNA. The DNA binding (absorption spectroscopy, steady-state and time-resolved emission measurements, steady-state emission quenching measurements) and cleavage (under dark and irradiated conditions) by these complexes has been studied to investigate the influence of the ancillary ligand. The binding ability of these complexes to DNA is dependent on the planarity of the intercalative polypyridyl ligand, which is further affected by the ancillary bipyridine-glycoluril ligand. The complexes 3, 4, 7, and 8 bind to CT-DNA with binding constants on the order of 10(4) M(-1). Time-resolved emission measurements on the DNA-bound complexes 1, 3, 5-7, and 9 show monoexponential decay of the excited states, whereas complexes 2, 4, and 8 show biexponential decay with short- and long-lived components. Interaction of complexes 2-9 with plasmid pBR322 DNA studied by gel electrophoresis experiments reveals that all complexes cleave DNA efficiently at micromolar concentrations under dark and anaerobic conditions probably by a hydrolytic mechanism. Complexes 3, 4, 7, 8, and [Ru(bpy)(2)(dppz)](2+) show extensive DNA cleavage in the presence of light with a shift in mobility of form I of DNA probably due to the high molecular weight of DNA-complex conjugates. However, the extent of the cleavage is augmented on irradiation in the case of complexes 3, 4, 7, and 8, which include the planar dpq and dppz ligands, suggesting a combination of hydrolytic and oxidative mechanism for the DNA scission. Molecular mechanics calculations of these systems corroborate the DNA binding and cleavage mechanisms.

Influence of confined water on the photophysics of dissolved solutes in reverse micelles.

The photophysical parameters of two probes with largely different hydrophobic character, namely, coumarin 1 and coumarin 343, are investigated in sodium bis-(2-ethylhexyl)sulfosuccinate (AOT)/hexane/water reverse micelles at various water/AOT molar ratio w(0). Correlation of photophysical parameters such as fluorescence quantum yield, fluorescence lifetime, and emission maxima with w(0) indicate distinctly different trends below and above w(0) approximately 7 for both probes. The variation of the average rotational correlation times obtained from fluorescence anisotropy decays for both probes in reverse micelles further corroborate the above observation. Similar studies were also performed in nonaqueous reverse micelles with acetonitrile as polar solvent. Similar to aqueous reverse micelles, breaks in the photophysical parameters with increasing acetonitrile/AOT molar ratios w'(0) were also observed in these cases, although at a much lower w'(0) value of 3. The present results indicate that around w(0) approximately 7 for aqueous reverse micelles (and around w'(0) approximately 3 for nonaqueous reverse micelles) a distinct change occurs in the probe microenvironment, which is rationalized on the basis of the relative populations of interfacial and core water. We propose that until the ionic head groups and counterions are fully solvated by polar solvents, that is, up to w(0) approximately 7 (or w'(0) approximately 3), the interfacial water population dominates. Above these molar ratios coalescence of excess water molecules with each other to form truncated H-bonded water clusters leads to a sizable population of core water. This is further substantiated by changes in the IR absorption spectra for the O--D stretching mode of diluted D(2)O in reverse micelles with varying w(0). Critical comparison of the present results with relevant literature reports provide clear support for the proposals made on water structure in reverse micelles. The role of relative size of the probe and the reverse micelles for differences in polar solvent to AOT ratios (w(0)=7 and w'(0)=3) in the observed breaks in the two types of reverse micelles is also discussed.

Single-molecule fluorescence studies reveal long-range electron-transfer dynamics through double-stranded DNA.

Complex dynamics of combined long-range fluorescence resonance energy transfer (FRET) and short-range electron transfer (ET) processes in a single double-stranded DNA (dsDNA) molecule (see figure) reveals that FRET remains almost unaltered in the presence of ET. Present systems also demonstrate the potential for long-range ET studies through the base stack in single dsDNA molecules.

Modulation in the solute location in block copolymer-surfactant supramolecular assembly: a time-resolved fluorescence study.

Effect of cosurfactant concentration on the location of a dissolved solute in a block copolymer-surfactant supramolecular system has been investigated using time-resolved fluorescence anisotropy and dynamic Stokes' shift measurements. Pluronic F88 and cosurfactant CTAC have been used to form a supramolecular assembly. The anion of coumarin 343 dye has been used as the solute/probe. It is seen that as the CTAC concentration is increased in the F88-CTAC supramolecular assembly, the microviscosity around the probe gradually increases. The result suggests that the probe undergoes a gradual migration from micellar surface to the interior of the micelle as the concentration of the CTAC is increased. This is also supported by the dynamic Stokes' shift results. It is seen that as the CTAC concentration is increased in the system, the observed Stokes' shift gradually increases due to the movement of the probe away from the bulk water. By comparing the present results with those reported in another pluronic-surfactant system, namely, P123-CTAC, it is indicated that the extent of modulation in the position of the probe in such supramolecular systems is largely determined by the composition of the pluronic, especially on the length of its hydrophilic ethyleneoxide block.

Ultrafast torsional dynamics of protein binding dye thioflavin-T in nanoconfined water pool.

Photophysical properties and ultrafast excited state torsional dynamics of the protein binding dye, Thioflavin-T, have been investigated in a nanoconfined water pool of reverse micelles using both steady-state fluorescence and the femtosecond fluorescence upconversion technique. It is seen that due to the confined environment in the reverse micelle, the fluorescence yield of Thioflavin-T is dramatically enhanced approximately 250-fold as compared to that in bulk water. The fluorescence yield decreases nonlinearly with the increase in the water pool size of the reverse micelles. Fluorescence lifetime of Thioflavin-T is also seen to decrease sharply with an increase in the water pool size. The results have been rationalized on the basis of the effect of confinement on the ultrafast torsional motion in the Thioflavin-T. The rate constants for the torsional motion in Thioflavin-T molecule in confined water pool have been estimated.

Fluorescence spectroscopic investigation to identify the micelle to gel transition of aqueous triblock copolymer solutions.

Steady-state and time-resolved fluorescence anisotropy measurements using probes coumarin 153 (C153) and 4-heptadecylumbelliferon (HUF) have been carried out to understand the micelle to gel transition of an aqueous triblock copolymer P123 ((EO)(20)-(PO)(70)-(EO)(20)) (EO = ethylene oxide; PO = propylene oxide) solution. Anisotropy results with a normal fluorescent probe, C153, do not show a characteristic change due to the micelle to gel transition. However, the probe HUF having a long hydrocarbon chain that helps its strong association with the micelle shows an increase in anisotropy above the sol-gel transition point. This difference has been explained as invoking a substantial contribution from the micellar structural fluctuations to the depolarization of HUF as its hydrocarbon chain is embedded in the micellar structure, which is not sensed significantly by the normal probe C153. That the extent of change in anisotropy for HUF upon gelation is not that large is possibly caused by the collective motion of the physically interconnected nodes, as observed from the dynamic light scattering studies, which acts in favor of a relatively faster depolarization in the gel phase. Similar studies in other copolymers, such as P85 ((EO)(26)-(PO)(40)-(EO)(26)) and F127 ((EO)(100)-(PO)(65)-(EO)(100)), further demonstrate the potential of probes latched with hydrocarbon chains in displaying a characteristic change for the micelle to gel transition which otherwise remains obscured for normal fluorescent probes.

Photophysical properties of coumarin-7 dye: role of twisted intramolecular charge transfer state in high polarity protic solvents.

Photophysical studies on coumarin-7 (C7) dye in different protic solvents reveal interesting changes in the properties of the dye on increasing the solvent polarity (Deltaf; Lippert-Mataga solvent polarity parameter) beyond a critical value. Up to Deltaf approximately 0.31, the photophysical properties of the dye follow good linear correlations with Deltaf. For Deltaf > approximately 0.31, however, the photophysical properties, especially the fluorescence quantum yields (Phi(f)), fluorescence lifetimes (tau(f)) and nonradiative rate constants (k(nr)), undergo large deviations from the above linearity, suggesting an unusual enhancement in the nonradiative decay rate for the excited dye in these high polarity protic solvents. The effect of temperature on the tau(f) values of the dye has also been investigated to reveal the mechanistic details of the deexcitation mechanism for the excited dye. Studies have also been carried out in deuterated solvents to understand the role of solute-solvent hydrogen bonding interactions on the photophysical properties of the dye. Observed results suggest that the fluorescence of the dye originates from the planar intramolecular charge transfer (ICT) state in all the solvents studied and the deviations in the properties in high polarity solvents (Deltaf > approximately 0.31) arise due to the participation of a new deexcitation channel associated with the formation of a nonfluorescent twisted intramolecular charge transfer (TICT) state of the dye. Comparing present results with those of a homologous dye coumarin 30 (C30; Photochem. Photobiol., 2004, 80, 104), it is indicated that unlike in C30, the TICT state of the C7 dye does not experience any extra stability in protic solvents compared to that in aprotic solvents. This has been attributed to the presence of intramolecular hydrogen bonding between the NH group (in the 3-benzimidazole substituent) of the C7 dye and its carbonyl group, which renders an extra stability to the planar ICT state, making the TICT state formation relatively difficult. Qualitative potential energy diagrams have been proposed to rationalize the differences observed in the results with C7 and C30 dyes in high polarity protic solvents.

Effect of electrostatic interaction on the location of molecular probe in polymer-surfactant supramolecular assembly: a solvent relaxation study.

Effect of electrostatic interaction on the location of a solubilized molecular probe with ionic character in a supramolecular assembly composed of a triblock copolymer, P123 ((ethylene oxide) 20-(propylene oxide) 70-(ethylene oxide) 20) and a cosurfactant cetyltrimethylammonium chloride (CTAC) in aqueous medium has been studied using steady-state and time-resolved fluorescence measurements. Coumarin-343 dye in its anionic form has been used as the molecular probe. In the absence of the surfactant, CTAC, the probe C343 prefers to reside at the surface region of the P123 micelle, showing a relatively less dynamic Stokes' shift, as a large part of the Stokes' shift is missed in the present measurements due to faster solvent relaxation at micellar surface region. As the concentration of CTAC is increased in the solution, the percentage of the total dynamic Stokes' shift observed from time-resolved measurements gradually increases until it reaches a saturation value. Observed results have been rationalized on the basis of the mixed micellar structure of the supramolecular assembly, where the hydrocarbon chain of the CTAC surfactant dissolves into the nonpolar poly(propylene oxide) (PPO) core of the P123 micelle and the positively charged headgroup of CTAC resides at the interfacial region between the central PPO core and the surrounding hydrated poly(ethylene oxide) (PEO) shell or the corona region. The electrostatic attraction between the anionic probe molecule and the positively charged surface of the PPO core developed by the presence of CTAC results in a gradual shift of the probe in the deeper region of the micellar corona region with an increase in the CTAC concentration, as clearly manifested from the solvation dynamics results.

Ultrafast bimolecular electron transfer dynamics in micellar media.

Ultrafast photoinduced bimolecular electron transfer (ET) dynamics between 7-aminocoumarin derivatives and N,N-dimethylaniline (DMAN) has been studied in neutral (TX100), cationic (DTAB) and anionic (SDS) micellar media. A very fast decay time constant (tau(fast)) shorter than approximately 10 ps has been observed for the coumarins in the presence of DMAN in all of the three micellar media. In this time scale, reactants in the micellar phase undergo ET interactions without involving diffusion or reorientation of the reactants and thus can be envisaged as equivalent to nondiffusive bimolecular ET reaction. The fastest ET rates estimated as the inverse of the shortest lifetime components of the fluorescence decay (k(et) congruent with tau(fast)(-1)) nicely follow the predicted Marcus inversion behavior with reaction exergonicity (-DeltaG degrees), irrespective of the nature of micelles considered. Onset of inversion in ET rates occur at approximately 0.61 eV lower exergonicity in SDS and TX100 micelles compared with that in DTAB micelle and are rationalized following two-dimensional ET (2DET) theory. These differences suggest the possibility of tuning Marcus inversion by proper selection of micelles. Interestingly, ET rates (k'(et)) obtained from the conventional Stern-Volmer analysis of the relatively longer time constants of the fluorescence decays also exhibit similar Marcus correlation with DeltaG degrees, showing clear inversion behavior. Fitting of Marcus correlation curves for k(et) and k'(et) indicate two largely different values for the electronic coupling parameters. In micellar media, as the interacting donor-acceptor molecules are on an average expected to be separated by an intervening surfactant chain and the reorientation rate of the reactants is quite slow, it is predicted that the ultrafast ET (k(et)) component arises because of the surfactant separated donor-acceptor pairs that are orientated perfectly to give the maximum electronic coupling. The slower ET (k'(et)) is predicted to arise because of those pairs where the donor-acceptor orientations are not very suitable but good enough to give a sizable electronic coupling.

A nanoreactor for tuning the chemical reactivity of a solute.

Present results demonstrate that the redox potential and hence the chemical reactivity of a solute dissolved in a polymer-surfactant supramolecular assembly, considered as a nanoreactor, can be tuned substantially by changing the composition of the supramolecular assembly. It is understood from detailed study that, on changing the polymer-surfactant composition of the supramolecular assembly, the probe undergoes a change in its location in these nanoreactors and accordingly its physical and chemical properties can be modulated.

Effects of block size of pluronic polymers on the water structure in the corona region and its effect on the electron transfer reactions.

Effects of constituent block size of triblock copolymers on the nature of the water molecules in the corona region of their micelles have been investigated using time-resolved fluorescence measurements. The physical nature of the water molecules in the micellar corona region of the block copolymer, Pluronic F88 ([ethylene oxide (EO)]103-[propylene oxide (PO)]39-EO103), has been studied using a solubilized coumarin dye. Solvent reorientation time and rotational correlation time have been measured and compared with another block copolymer, Pluronic P123 (EO20-PO70-EO20), which has a different composition of the constituent PO and EO blocks. It is noted that due to the presence of larger number of EO blocks in F88 as compared with P123, the corona region of the former micelle is more hydrated than that of the latter. The solvent reorientation time and rotational correlation time are found to be relatively shorter for F88 as compared with P123. This indicates that the water molecules in the corona of the F88 micelle are more labile than those of P123, which is also supported from the estimated number of water molecules associated with each EO unit, measured from the size of each type of micelle and its aggregation number. To understand the effect of block size on the chemical reactions in these microheterogeneous media, electron transfer reactions have been carried out between different coumarin acceptors and N, N-dimethylaniline donor. The electron transfer results obtained in F88 micelles have been compared with those obtained in P123, and the results are rationalized on the basis of the relative hydration of the two triblock copolymer micelles.

Quantitative distinction between competing intramolecular bond twisting and solvent relaxation dynamics: an ultrafast study.

Often an intramolecular relaxation process takes place in a time scale similar to that of the solvent relaxation process. Under these circumstances the dynamic Stokes' shift of the probe can be modulated by the combined effect of these two relaxation processes. In the present article we have studied ultrafast solvent relaxation using three different coumarin dyes and proposed a methodology for the quantitative separation of the dynamics of two competing processes, namely, solvent relaxation and bond twisting, that take place simultaneously in the present systems.