Preferential Binding of Epirubicin Hydrochloride with Single Nucleotide Mismatched DNA and Subsequent Sequestration by a Mixed Micelle

Abstract: Targeting mismatched base pairs containing DNA using small molecules and exploring the underlying mechanism involved during the binding interactions is one of the fundamental aspects of drug design. These molecules in turn are used in nucleic acid targeted therapeutics and cancer diagnosis. In this work, we systematically delineate the binding of the anticancer drug, epirubicin hydrochloride (EPR) with 20-mer duplex DNA, having both natural nucleobase pairing and thermodynamically least stable non-Watson−Crick… Show more

“…It must be stated here, the probe (here NR) does not show any loss in fluorescence signal during the experiment as evident from Figure S12. Only NR displays a typical single component diffusion with a time constant ∼72 μs as evident from the recorded autocorrelation function trace (Figure 5a), which is well corroborated with a previously reported drug, Epirubicin Hydrochloride, from our group [41] . On the contrary, the longer lag time component of the diffusion arises from the fibrillar binding site as evident from Figure 5a, and Table S5.…”

“…Only NR displays a typical single component diffusion with a time constant ~72 μs as evident from the recorded autocorrelation function trace (Figure 5a), which is well corroborated with a previously reported drug, Epirubicin Hydrochloride, from our group. [41] On the contrary, the longer lag time component of the diffusion arises from the fibrillar binding site as evident from Figure 5a, and Table S5. From Figure 5a, Table 1, and Table S5, it is observed that the longer lag-time component and corresponding relative amplitude increases which attributes the binding of NR to Trypsin Fib.…”

“…K B , T , r H , and η are the Boltzmann constant, absolute temperature, hydrodynamic radius of the fluorescent probe, and viscosity of the medium, respectively. For the elimination of mismatches of refractive index and viscosity of the experimental medium, we have used a ratio method as mentioned in an earlier report [41,43] . To estimate the accurate hydrodynamic radius ( r H ), we used equation (2) with Rhodamine 6G as a standard fluorescent probe having a known diffusion coefficient ( D t =426 μm 2 s −1 ) [42] …”

“…For the elimination of mismatches of refractive index and viscosity of the experimental medium, we have used a ratio method as mentioned in an earlier report. [41,43] To estimate the accurate hydrodynamic radius (r H ), we used equation (2) with Rhodamine 6G as a standard fluorescent probe having a known diffusion coefficient (D t = 426 μm 2 s À 1 ). [42] (2)…”

“…Fluorescence Lifetime Imaging Microscopy (FLIM) images and FCS data were recorded in PicoQuant, MicroTime 200 confocal setup with an inverted optical microscope (Olympus IX-71), the details are mentioned elsewhere. [41,46] Here, NR and ThT were used for FCS and FLIM studies with excitation lasers of 530 nm and 405 nm, respectively. In the case of FCS, a dichroic mirror (DC/470/532 DCXR, Chroma) and a band-pass filter (HQ532lp, Chroma) was used.…”

Macrocyclic Cavitand β‐Cyclodextrin Inhibits the Alcohol‐Induced Trypsin Aggregation

“…It must be stated here, the probe (here NR) does not show any loss in fluorescence signal during the experiment as evident from Figure S12. Only NR displays a typical single component diffusion with a time constant ∼72 μs as evident from the recorded autocorrelation function trace (Figure 5a), which is well corroborated with a previously reported drug, Epirubicin Hydrochloride, from our group [41] . On the contrary, the longer lag time component of the diffusion arises from the fibrillar binding site as evident from Figure 5a, and Table S5.…”

“…Only NR displays a typical single component diffusion with a time constant ~72 μs as evident from the recorded autocorrelation function trace (Figure 5a), which is well corroborated with a previously reported drug, Epirubicin Hydrochloride, from our group. [41] On the contrary, the longer lag time component of the diffusion arises from the fibrillar binding site as evident from Figure 5a, and Table S5. From Figure 5a, Table 1, and Table S5, it is observed that the longer lag-time component and corresponding relative amplitude increases which attributes the binding of NR to Trypsin Fib.…”

“…K B , T , r H , and η are the Boltzmann constant, absolute temperature, hydrodynamic radius of the fluorescent probe, and viscosity of the medium, respectively. For the elimination of mismatches of refractive index and viscosity of the experimental medium, we have used a ratio method as mentioned in an earlier report [41,43] . To estimate the accurate hydrodynamic radius ( r H ), we used equation (2) with Rhodamine 6G as a standard fluorescent probe having a known diffusion coefficient ( D t =426 μm 2 s −1 ) [42] …”

“…For the elimination of mismatches of refractive index and viscosity of the experimental medium, we have used a ratio method as mentioned in an earlier report. [41,43] To estimate the accurate hydrodynamic radius (r H ), we used equation (2) with Rhodamine 6G as a standard fluorescent probe having a known diffusion coefficient (D t = 426 μm 2 s À 1 ). [42] (2)…”

“…Fluorescence Lifetime Imaging Microscopy (FLIM) images and FCS data were recorded in PicoQuant, MicroTime 200 confocal setup with an inverted optical microscope (Olympus IX-71), the details are mentioned elsewhere. [41,46] Here, NR and ThT were used for FCS and FLIM studies with excitation lasers of 530 nm and 405 nm, respectively. In the case of FCS, a dichroic mirror (DC/470/532 DCXR, Chroma) and a band-pass filter (HQ532lp, Chroma) was used.…”

Macrocyclic Cavitand β‐Cyclodextrin Inhibits the Alcohol‐Induced Trypsin Aggregation

New anticancer Pt and Pd complexes with binicotinic acid and oxalate derivatives as ligands: Synthesis, cytotoxicity, binding mode on DNA and HSA and molecular docking

Disruption of aggregates of a Zn2+-complex of a schiff base in water by surfactants: Insights from fluorescence spectroscopy in ensemble and single molecule levels