Host–guest complexes of the antituberculosis drugs pyrazinamide and isoniazid with cucurbit[7]uril

The potential use of cucurbit[7]uril (CB[7]) as an excipient in oral formulations for improved drug physical stability or for improved drug delivery was examined with the antituberculosis drugs pyrazinamide (pyrazine-2-carboxamide) and isoniazid (isonicotinohydrazide). Both drugs form 1:1 host–guest complexes with CB[7] as determined by ¹H nuclear magnetic resonance spectrometry, electrospray ionisation mass spectrometry and molecular modelling. Drug binding is stabilised by hydrophobic effects between the pyridine and pyrazine rings of isoniazid and pyrazinamide, respectively, to the inside cavity of the CB[7] macrocycle as well as hydrogen bonds between the hydrazide and amide groups of each drug to the CB[7] carbonyl portals. At pH 1.5, isoniazid binds CB[7] with a binding constant of 5.6 × 10⁵ M^?1, whilst pyrazinamide binds CB[7] at pH 7 with a much smaller binding constant (4.8 × 10³ M^?1). Finally, CB[7] prevents drug melting through encapsulation. Where previously pyrazinamide displays a typical melting point of 189 °C and isoniazid 171 °C, by differential scanning calorimetry, no melting or degradation at temperatures up to 280 °C is observed for either drug once bound by CB[7].     

Binding of a neutral guest to cucurbiturils: photophysics,thermodynamics and molecular modelling

Steady-state and time-resolved fluorescence techniques were used to study the thermodynamics of binding of a neutral polarity-sensitive guest, the methyl 2-naphthalenecarboxylate (2MN), with three cucurbiturils (CBn; n = 6, 7 and 8) in water. Association constants (K) were obtained from nonlinear regression analysis of the fluorescence intensity against [CB] in the 5–45°C range. 2MN complexed with CB7 exhibited a 1:1 stoichiometry (K ≈ 10³ M^? 1 at 25°C); however, it hardly did with CB6 (K < 10 M^? 1) and it did not with the larger CB8 macrocyclic ring. The (1:1) 2MN:CB7 complexation process was accompanied by a small unfavourable enthalpy change and was, therefore, entropically governed. Molecular mechanics and molecular dynamics calculations in the presence of water were also used to study the geometry of the complexes formed and the driving forces responsible for their formation. The results were compared with those previously obtained for the complexation of the same guest, 2MN, with natural α-, β- and γ-cyclodextrins.     

Complexation and Fluorescence of Tricyclic Basic Dyes Encapsulated in Cucurbiturils

Tricyclic basic dyes (proflavine, acridine orange, pyronine, pyronine Y, oxonine, thionine and methylene blue) often form one‐to‐one or two‐to‐one complexes with CB[7] and CB[8], respectively. In the case of pyronine Y, the complexes with CB[7] and CB[8] have a one‐to‐one and three‐to‐one stoichiometry, respectively. The binding constants for CB[7] complexes range from 3.07×10⁶ to 1.70×10⁷ m ^?1. In the case of CB[8], the association constant varies between 3.24×10¹³ and 2.50×10¹⁶ m ^?2. Overall, these binding constants are four orders of magnitude higher than those reported for the same dyes in β and γ‐cyclodextrins. Formation of the host–guest complexes leads to an increase in the fluorescence quantum yields in the case of CB[7], while the dimeric or trimeric dye encapsulated in CB[8] are remarkably less fluorescent than the same dye in diluted solutions.     

Effect of cucurbit[n]urils on tropicamide and potential application in ocular drug delivery

The supramolecular interactions of the ocular drug tropicamide (TR) with cucurbit[7]uril (CB7) and cucurbit[8]uril (CB8) were investigated in aqueous solutions by using ¹H NMR, ESI-MS and UV–vis spectroscopic techniques. The results indicate a 1:1 binding stoichiometry of TR with CB7 and CB8. The binding constants of TR in its protonated form were higher (e.g. K = 4 × 10⁶ M^? 1 with CB8) than in its neutral form (e.g. K = 1.4 × 10⁴ M^? 1 with CB8), which led to a complexation-induced increase in its pK _a value of ca. 0.5 and 2 units with CB7 and CB8, respectively. In the presence of about 1% (w/v) CB8, the ionisation degree of 0.1% (w/v) TR was increased from 2% to 62% at neutral pH. The increase in the pK _a value and thus stabilisation of the protonated TR species at neutral pH is discussed in the context of supramolecular drug delivery of ophthalmologic drugs.     

A Comparative Study of Complexation of β-Cyclodextrin,Calix[4]arenesulfonate and Cucurbit[7]uril with Dye Guests: Fluorescence Behavior and Binding Ability

The complexation behaviors of acridine red (AR), neutral red (NR) and rhodamine B (RhB) dye guest molecules by three kinds of supramolecular hosts, including β-cyclodextrin (β-CD), calix[4]arene tetrasulfonate (C4AS) and cucurbit[7]uril (CB[7]), have been investigated by means of fluorescence spectra in aqueous citrate buffer solution (pH 6.0). The results obtained show that the three hosts, possessing different types of cavity, lead to various complexation-induced fluorescence of dye guests, and present different binding ability and molecular selectivity. The complexation stability constants decrease in the order of NR > AR > RhB for C4AS and CB[7] hosts, while in the order of RhB > AR > NR for β-CD host. Particularly, CB[7] displays the strongest binding ability with NR (K _S = 33300 M^? 1), and provides the molecular selectivity of 4.8 for NR/AR pairs. Although the binding ability of C4AS for present dye guests is weaker than CB[7], but the molecular selectivity of the two hosts are nearly equivalent. β-CD shows stronger binding ability with RhB (K _S = 5880 M^? 1) as comparison with CB[7] and C4AS. Furthermore, the solvent effects and salt effects during the course of complexation have also been investigated.     

Encapsulation of a β-carboline in cucurbit[7]uril

Inclusion of a biological photosensitizer and prototype of β-carbolines, norharmane (NHM), into the cavity of cucurbit[7]uril (CB[7]) has been investigated for the first time, by using ¹H NMR and UV–visible spectroscopy, and ab initio calculations. Protonated NHM forms a very stable host–guest complex with CB[7] in aqueous solution, with a binding constant of (9.0 ± 0.5) × 10⁴ M^?1. The encapsulation of NHM into CB[7] has driven the prototropic equilibrium of NHM to protonated NHM (NHMH⁺) at neutral pH. A pH titration for the host–guest complex revealed a moderate shift of the acid–base equilibrium in the ground-state (from 7.2 to 7.9), which may be caused by the low polarity microenvironment of the CB[7] cavity. The CB[7] provides a binding pocket for the hydrophobic molecule, and the polar, carbonyl-lined portals offering an anchoring site for the positive charge of the cationic species NHMH⁺.     

Cucurbit[7]uril complexations of bis(isoquinolinium)alkane dications in aqueous solution

The 1:1 and 2:1 host–guest complexation of a series of 1,n-bis(isoquinolinium)alkane dications (Iq(CH₂)_nIq²⁺, n = 2, 4, 5, 6, 8, 9, 10 and 12, and Iq(p-xylene)Iq²⁺) by cucurbit[7]uril (CB[7]) in aqueous solution has been investigated by ¹H NMR spectroscopy and ESI mass spectrometry. The site of binding of the first CB[7] is dependent on the nature of the central linker group, with encapsulation of the p-xylene group or the polymethylene chain when n = 6–10.With shorter (n = 2–5) or longer (n = 12) chains, the first CB[7] binds over an isoquinolinium group. With a second CB[7], the binding of the central group is abandoned in favour of the CB[7] hosts encapsulating the two cationic isoquinolinium termini. The 1:1 and 2:1 host–guest stability constants are related to modes of binding and the nature of the central linkers, and are compared with dicationic guests bearing different terminal groups.     

Light- and pH-regulated Water-soluble Pseudorotaxanes Comprising a Cucurbit[7]uril and a Flavylium-based Axle

A linear double pyridinium-terminated thread comprising a central chalcone moiety is shown to provide two independent binding sites with similar affinity for cucurbit[7]uril (CB7) macrocycles in water as judged from NMR, UV-Visible and fluorescence spectroscopies. Association results in [2] and [3]pseudorotaxanes, which are both pH and photosensitive. Switching from the neutral chalcone to the cationic flavylium form upon irradiation at 365 nm under acidic conditions provided an enhanced CB7 association (K_1:1 increases from 1.2×10⁵ M⁻¹ to 1.5×10⁸ M⁻¹), limiting spontaneous on-thread cucurbituril shuttling. This co-conformational change in the [2]pseudorotaxane is reversible in the dark with k_obs=4.1×10⁻⁴ s⁻¹. Threading the flavylium moiety into CB7 leads to a dramatic increase in the fluorescence quantum yield, from 0.29 in the free axle to 0.97 in the [2]pseudorotaxane and 1.0 in the [3]pseudorotaxane.     

Crystal structure,interaction with DNA,and bovine serum albumin of the cobalt(II) complex of demethylcantharate and 2,2′-bipyridine

A new cobalt(II) complex [Co(DCA)(bipy)(H₂O)] (DCA?=?demethylcantharate, 7-oxabicyclo[2.2.1]heptane-2,3-dicarboxylate, C₈H₈O₅; bipy?=?2,2′-bipyridine, C₁₀H₈N₂) was synthesized from cobalt acetate, demethylcantharidin, and bipy. This complex was characterized by elemental analysis, molar conductance, infrared spectra, and X-ray single-crystal diffraction. It crystallized in orthorhombic crystal system and Pbca space group. The DNA binding of the complex was investigated by electronic absorption spectra and viscosity measurements. The complex binds to DNA via partial intercalation with binding constant K _b of 4.02?×?10⁴?L?M^?1. The complex could quench the intrinsic fluorescence of bovine serum albumin through static quenching. The binding constant K _A was 7.28?×?10⁶?L?M^?1 and binding site was one.     

Determination of L‐Cystine by a New Sensitive Cucurbit[7]uril/palmatine Probe

In the presence of cucurbit[7]uril (CB[7]), the CB[7] could react with palmatine, which served as a sensitive fluorescence probe, to form host‐guest stable complexes and the fluorescence intensity of the complexes was greatly enhanced. The fluorescence intensity decreased linearly with an increasing number of L‐cystine in the inclusion system. The experimental results show that there exists a competition between L‐cystine and palmatine for the CB[7] hydrophobic cavity and L‐cystine occupies the space of CB[7] cavity, leading palmatine molecules to be forced to reside in the aqueous environment. Based on the fluorescence quenching of the CB[7]/palmatine complexes resulting from complex formation between CB[7] and L‐cystine, a spectrofluorimetric method for the determination of L‐cystine in aqueous solution in the presence of CB[7] was developed. The linear relationship between the corresponding values of the fluorescence quenching ΔF and L‐cystine concentration was obtained in the range of 6.0 to 1.5×10³ ng·mL^?1, with a correlation coefficient (r) of 0.9996. The detection limit was 2.0 ng·mL^?1. The application of the present method to the determination of L‐cystine in tablets gave satisfactory results. This paper also discussed the mechanism of the fluorescence indicator probe.     

Imidazo[1,2-a]pyridine-substituted coumarin as a selective ratiometric sensor for Cu2+ ion

A novel fluorescent chemosensor, (E)-7-(diethylamino)-3-((2-phenylimidazo[1,2-a]pyridin-3-ylimino)methyl)-2H-chromen-2-one 1a, has been synthesised and characterised. This chemosensor displayed an extreme selective fluorescence emission only with Cu²⁺ ion over all other metal ions examined. The Job’s plot experiment analysis suggested the binding ratio of the chemosensor 1a with Cu²⁺ was 1:1 metal-to-ligand ratio. The association constant for Cu²⁺ towards receptor 1a obtained from Benesi–Hildebrand plot was found to be 4.859 × 10³ M^?1 with a detection limit 4.6 × 10^?8 M. Fluorescence enhancement caused by Cu²⁺ binding with chemosensor 1a attributed to combinational effect of intramolecular charge transfer and chelation-enhanced fluorescence occurred at pH 8.0.     

Photophysical properties of aqueous solutions of a styryl dye in the presence of cucurbit[<Emphasis Type="Italic">n</Emphasis>]uril (<Emphasis Type="Italic">n</Emphasis> = 5, 6, 8)

Photophysical properties of aqueous solutions of the styryl dye 4-[(E)-2-(3,4-dimethoxyphenyl)-1-ethylpyridinium] perchlorate (1) in the presence of cucurbit[n]urils (CB[n]; n = 5, 6, 8) have been studied by fluorescent spectroscopy methods. The fluorescence intensity of a 10^–6 mol L^–1 solution of 1 increases by a factor of 12.6 upon the formation of 1 : 1 inclusion complexes with CB[6] or 1.3 in complexes with CB[8]. Upon the formation of inclusion complexes, the average lifetime of the electronically excited state of 1 increases to about 1 ns for both CB[6] and CB[8]. On the basis of fluorescence anisotropy measurements, the rotational relaxation times were estimated to be 408, 314, and 183 ps for the complexes with CB[6], CB[8], and for unbound 1, respectively. Using the fluorescence titration method developed for the case of poorly soluble cavitands, the binding constant of 1 with CB[6] was determined to be 1.1 × 10⁵ L mol^–1. The addition of CB[5] does not lead to changes in the photophysical properties of a solution of 1, indicating the absence of complexes between CB[5] and 1. It has been found on the basis of the experimental data that the fluorescence rate constant of 1 decreases about twice in the complex with CB[8], but doubles in the complex with CB[6].     

A rare case for binding a diquat salt by two cyclo[6]aramides

The non-aggregational cyclo[6]aramide has demonstrated 2:1 host–guest complexation towards diquat with very strong binding ability (K₁ = 5.41 × 10⁴ M^? 1, K₂ = 4.33 × 10⁶ M^? 1). The donor–acceptor binding process of the macrocycle and the quaternary salt was investigated by ¹H NMR, ESI mass spectrometry and UV–vis spectroscopy. The binding mode is supported by both experiments and theoretical simulations. This work provides the first example of using recently developed H-bonded aromatic oligoamide macrocycles for binding diquat in solution.     

Host–guest interactions of 6-benzyladenine with normal and modified cucurbituril: 1H NMR,UV absorption spectroscopy and phase solubility methods

Guest–host inclusion complexes between 6-benzyladenine (6-BA), cucurbit[7]uril (Q[7]), symmetrical tetramethylcucurbit[6]uril (TMeQ[6]) and meta-hexamethyl-substituted cucurbit[6]uril (HMeQ[6]) in aqueous solution were investigated by ¹H NMR, UV absorption spectroscopy and phase solubility studies. The ¹H NMR spectra analysis revealed that the hosts selectively bound the phenyl moiety of the guests. Absorption spectroscopic analysis defined the stability of the host–guest inclusion complexes. A host:guest ratio of 1:1 was measured quantitatively as (5.63 ± 0.26) × 10⁴, (1.94 ± 0.17) × 10³ and (2.89 ± 0.23) × 10³ mol L^? 1 for the Q[7]-6-BA, TMeQ[6]-6-BA and HMeQ[6]-6-BA systems, respectively. Phase solubility diagrams were analysed through rigorous procedures to obtain estimates of the complex formation constants for Q[n]-6-BA complexation. The formation constants were (1.29 ± 0.24) × 10⁴ L mol^? 1 for Q[7]-6-BA, (3.20 ± 0.17) × 10³ L mol^? 1 for TMeQ[6]-6-BA and (3.52 ± 1.01) × 10³ L mol^? 1 for TMeQ[6]-6-BA. Furthermore, phase solubility studies showed that 6-BA solubility increased as a function of Q[7], TMeQ[6] and HMeQ[6] concentrations. The thermodynamic parameters of the complex formation were also determined. The formation of inclusion complexes between 6-BA and Q[7] was enthalpy controlled, suggesting that hydrophobic and van der Waals interactions were the main driving forces. Our results demonstrated that the complexation of 6-BA with Q[n] could be used to improve the solubility of 6-BA.     

Synthesis,characterization, molecular modeling,and DNA interaction studies of a Cu(II) complex containing drug of chronic hepatitis B: adefovir dipivoxil

A new copper(II) complex [Cu(adefovir)₂Cl₂], where adefovir = adefovir dipivoxil drug, was synthesized and characterized by using different physicochemical methods. Binding interaction of this complex with calf thymus DNA (ct-DNA) has been investigated by multi-spectroscopic techniques and molecular modeling study. The complex displays significant binding properties of ct-DNA. The results of fluorescence and UV–vis absorption spectroscopy indicated that, this complex interacted with ct-DNA in a groove-binding mode, and the binding constant was 4.3(±0.2) × 10⁴ M^?1. The fluorimeteric studies showed that the reaction between the complex and ct-DNA is exothermic (ΔH = 73.91 kJ M^?1; ΔS = 357.83 J M^?1 K^?1). Furthermore, the complex induces detectable changes in the CD spectrum of ct-DNA and slightly increases its viscosity which verified the groove-binding mode. The molecular modeling results illustrated that the complex strongly binds to the groove of DNA by relative binding energy of the docked structure ?5.74 kcal M^?1. All experimental and molecular modeling results showed that the Cu(II) complex binds to DNA by a groove-binding mode.     

Determination of Paraquat by Cucurbit[7]uril Sensitized Fluorescence Quenching Method

A method for the determination of paraquat by cucurbit[7]uril (CB[7]) fluorescence quenching was developed. The assay was based on the reaction of the CB[7] with acridine orange. The fluorescence intensity of acridine orange regularly increased with the addition of CB[7]. However, while an appropriate amount of paraquat was added to the CB[7]- acridine orange system, the fluorescence intensity of the system was quenched which was employed to determine paraquat. Under the optimum conditions, a linear range of 3.0–800 nmol L^?1 and a detection limit of 1.61 nmol L^?1 for paraquat were obtained. The simple strategy reported here offers great practical potential for the determination of pesticide residues in agricultural products.     

Determination of Tryptophan using a p-Sulfonated Calix [4,6,8]arene Modified Gold Electrode

The ability of p-sulfonated calix[n]arenes (n = 4, 6, 8) to form complexes with tryptophan was studied. The electrochemical properties of these complexes immobilized on gold surfaces were examined by cyclic voltammetry. Parameters affecting the performance of the modified electrodes including the arene concentration, scan rate, applied potential, and pH were optimized. Under the optimal conditions, the method had a linear response to tryptophan between 1 × 10^?7 M and 1 × 10^?5 M with a detection limit of 3 × 10^?8 M. The interaction of the tryptophan–p-sulfonated calix[4]arene complex was more stable than the tryptophan–p-sulfonated calix[6]arene and p-sulfonated calix[8]arene complexes. Molecular modeling calculations indicated that electrostatic interactions and structural matching effects were predominant stabilizing factors. The modified electrodes demonstrated good reproducibility and high selectivity, illustrating their effectiveness for analytical measurements.     

Cucurbit[7]uril/CuCl promoting decomposition of 4-nitrobenzenediazonium in aqueous solution

The host-guest complex between cucurbit[7]uril and 4-nitro-benzendiazonium is decomposed into a nitrobenzene/4-nitrophenol mixture in a high total yield in the presence of CuCl.     

MECHANISM OF THE PHOTOSENSITIZED REDOX REACTIONS OF ACRIDINE ORANGE IN AQUEOUS SOLUTIONS-A SYSTEM OF INTEREST IN THE PHOTOCHEMICAL STORAGE OF SOLAR ENERGY†

-We have carried out a very detailed study, using fluorescence and optical flash photolysis techniques, of the photoreduction of methyl viologen (MV²⁺) by the electron donor ethylene diamine tetraacetic acid (EDTA) in aqueous solution sensitized by the dye acridine orange (AOH⁺). A complete mechanism has been proposed which accounts for virtually all of the known observations on this reaction. This reaction is novel in that both the triplet and the singlet state of AOH⁺ appear to be active photochemically. We have shown that mechanisms previously proposed for this reaction are probably incorrect due to an artifact. At pH 7 the fluorescence quantum yield φ_s of AOH⁺ is 0.26 ± 0.02 and the fluorescence lifetime is 1.8 ± 0.2 ns. φ_s is pH dependent and reaches a maximum of 0.56 at pH 4. The fluorescence of AOH⁺ is quenched by MV²⁺ at concentrations above 1 mM and the quenching obeys Stern-Volmer kinetics with a quenching rate constant of (1.0 ± 0.1) × 10¹⁰M^?1 s^?1. The quenching of the AOH⁺ excited singlet state by MV²⁺ almost certainly returns the AOH⁺ to its ground state with no photochemistry occurring. EDTA also quenches the fluorescence of AOH· with Stern-Volmer kinetics but with a smaller rate constant (6.4 ± 0.5) × 10⁸M^?1s^?1 at pH 7. In this case the quenching is reactive resulting in the formation of semireduced AOH. In the presence of MV²⁺, flash irradiation of AOH⁺ does result in the reversible formation of the semireduced MV? which absorbs at 603 nm. We attribute this to a photochemical reaction of the triplet state of AOH⁺ with MV²⁺. The initial quantum yield for formation of MV? (φ_MV:)₀ was found to be constant at 0.10 ± 0.05 for [MV²⁺] from 5 × 10^?5 to 1.0 × 10^?3 with [AOH⁺] = 8 × 10^?6M. Previous workers had found that (φ_MV:)₀ appears to decrease with decreasing [AOH⁺]; however, on careful investigation, we found this was most probably due to quenching of the triplet state of AOH⁺ by trace amounts of oxygen. When EDTA is added to a mixture of AOH ⁺ and MV²⁺ at pH 7, the photochemical formation of MV? becomes irreversible as the [EDTA] is increased. The quantum yield for the irreversible formation of MV? exceeds 0.10 becoming as large as 0.16 for [EDTA] = 0.014M. This fact requires that an alternative photochemical process must be operative and we present evidence that this is a reaction of EDTA with the excited singlet state of AOH⁺ to produce the semi-reduced AOH- which then reacts with MV²⁺ to produce MV?. The full kinetic scheme was tested by computer simulation and found to be totally consistent. This also enabled the processing of a full set of rate constants. When colloidal PtO₂ was added to the optimal mixture [EDTA] = 3.4 × 10^?2M; [MV²⁺] = 5 × 10^?4M; [AOH⁺] = 4 × 10^?5M; pH6 H₂ gas was produced at a rate of 0.2μmol H₂h^?1. Thus, acridine orange should serve as an effective sensitizer in reactions designed to use solar energy to photolyze water.     

Synthesis,structure and spectroscopic studies on DNA binding,BSA interaction of a nickel(II) complex containing l–methionine Schiff base and 1,10-phenanthroline

A new nickel(II) complex, [Ni(o-van-L-met)(phen)(CH₃OH)] (o-van-L-met = Schiff base derived from o-vanillin and l-methionine, phen = 1,10–phenanthroline), has been synthesized and characterized by elemental analyses, IR spectra, and single-crystal X-ray diffraction. The crystal structure shows nickel is six-coordinate in a distorted octahedral geometry. In this crystal, molecules form a 2-D plane structure via hydrogen bonds and π–π interactions. The interaction of the complex with calf thymus DNA (CT-DNA) was investigated by absorption, fluorescence, circular dichroism (CD), spectroscopies, and viscosity measurement. The complex binds to CT-DNA in an intercalative mode with a binding constant of (4.7 ± 0.5) × 10⁴ M^?1. The interaction of the complex with bovine serum albumin (BSA) was also studied by the multispectroscopic methods. Results illustrated that the nickel(II) complex can effectively quench the intrinsic fluorescence of BSA via a static quenching mechanism and cause conformational changes. The binding constant K_b was (6.3 ± 1.6) × 10⁴ M^?1 and the binding site number n was 0.96 ± 0.04; its bind site was located within subunit IIA of BSA.