FIELD OF INVENTION
The disclosed technology is generally related to rotaxanes. More specifically, the disclosed technology is related to viologen-based rotaxanes.
BACKGROUND
Motivated by the desire to understand the structure-property relationships of biomolecules including DNA, RNA and membranes and the roles they play in life processes, chemists have striven to manipulate molecular-scale phenomena, resulting from noncovalent bonding interactions, in ever-increasingly complex and organized situations.[1-4] By employing noncovalent bonding interactions, synthetic foldamers,[5-8] which are promising candidates for mimicking the behavior of biomacromolecules under different kinds of stimuli—and mechanical interlocked molecules[9-11] (MIMs), which are the result of the formation of mechanical bonds and have already found applications in drug delivery[12, 13] and molecular electronics[14-17]—have been developed and investigated in some detail. Foldamers and MIMs, both utilizing intra- and intermolecular interactions in order to regulate the shapes of molecules, however, seldom result in their paths' crossing.
Foldameric rotaxanes,[18-21] which lie at the intersection between synthetic foldamers and MIMs, have made their ways into chemists' sights recently. Usually expressed in the context of oligorotaxanes, in which the dumbbell component is threaded by multiple ring components in order to regulate the folded secondary structure, they can exhibit remarkable physicochemical properties[22-26] in response to external stimuli. For example, it has already been[22, 23, 25] demonstrated that mechanical responses of oligorotaxanes toward external forces can be controlled by the mobile rings trapped along their one-dimensional dumbbell components, representing a new class of entropy-dominated molecules and materials.
To date, syntheses and properties of a family of foldameric oligorotaxanes which rely on the presence of donor-acceptor recognition between electron-rich 1,5-dioxanaphthalene (DNP) units and electron-deficient cyclobis(paraquat-p-phenylene) (CBPQT4+) rings have been disclosed.[28] Moreover radical-pairing interactions associated with BIPY(.+) radical cations—the mono reduced state of dicationic BIPY2+ units—can be utilized in the preparation of MIMs based on a template-directing strategy.[29-33]
Foldameric oligorotaxanes make it possible to prepare functional materials by scaling[11,27] the concerted mechanical actuation of MIMs into the macroscopic regime where applications can be sought and witnessed. For the development of new applications and novel molecular devices and materials, there is a need for new rotaxanes that can be used to prepare nanoactuators.
SUMMARY OF THE INVENTION
Disclosed herein are viologen-based rotaxanes to prepare nanoactuators. In some embodiments, the nanoaccuator comprises a rotaxane, wherein the rotaxane comprises a threading component and at least two macrocylic components; wherein the threading component comprises a oligoviologen; and wherein the threading component is threaded through each of the macrocylic components. In another embodiment, the nanoaccuator comprises a rotaxane, wherein the rotaxane comprises a threading component; wherein the threading component comprising a linear subchain having a formula L-V—[B—V]n-L′, and at least two macrocycle components; wherein each of the at least two macrocycle components are threaded onto the threading component; and wherein V is a viologen subunit, B is a bridging subunit; wherein L and L′ are linking subunits, and wherein n is an integer. The nanoactuator may further comprise a first stopper subunit, S, and a second stopper subunit, S′, and wherein the threading component has a formula of S-L-V—[B—V]n-L′-S′. In some embodiments, the at least two macrocylic components are CBPQT macrocylic components.
In some embodiments, the oligoviologen comprises a viologen subunit. The viologen subunits may be BIPY subunits. The oligoviolgen may further comprise bridging subunits linking the viologen subunits. The bridging subunit may be a paraxylene subunit. In particular embodiments, the oligoviologen comprises four or five viologen subunits.
The nanoactuator may further comprise a first stopper subunit and a second stopper subunit, wherein the first stopper subunit and the second stopper subunit prevent the at least two macrocylic components from unthreading from the threading component. In some embodiments, the threading component further comprises a first linking subunit and a second linking subunit, wherein the first linking subunit links a first end of the oligoviologen to the first stopper subunit and the second linking subunit links a second end of the oligoviologen to the second stopper subunit.
In some embodiments, the first linking subunit, the second linking subunit, or both the first linking subunit and the second linking subunit comprise an alkyl subunit. In particular embodiments, the first linking subunit, the second linking subunit, or both the first linking subunit and the second linking subunit comprise a C3-9 alkyl subunit. In some embodiments, the first linking subunit, the second linking subunit, or both the first linking subunit and the second linking subunit comprise a polyethylene oxide subunit. In particular embodiments, the first linking subunit, the second linking subunit, or both the first linking subunit and the second linking subunit comprise a (O—CH2—CH2)1-3 polyethylene oxide subunit.
In some embodiments, the first stopper subunit, the second stopper subunit, or both the first stopper subunit and the second stopper subunit comprise a triazole stopper subunit. In some embodiments, the first stopper, the second stopper, or both the first stopper and the second stopper comprise a triazole stopper moiety having a formula of R—C2N3—R′, S′, wherein R and R′ are bulky moieties capable of preventing dethreading of the macrocyclic components. In particular embodiments, the first stopper subunit, the second stopper subunit, or both the first stopper subunit and the second stopper subunit comprise a (CH3)3C—CH2—O—C(═O)—C2N3—C(═O)—O—CH2—C(CH3)3 triazole stopper subunit.
In some embodiments, the rotaxane is complexed with an anion. In particular embodiments, the rotaxane is complexed with PF6− or CF3C(═O)O−.
In some embodiments, the rotaxane is cationic. In some embodiments, the rotaxane is in a radical electronic state. In some embodiments, the rotaxane is in a radical cationic electronic state. In some embodiments, the rotaxane is capable of reversible oxidation and reduction.
In some embodiments, reducing the rotaxane contracts the nanoreactor and/or oxidizing the rotaxane extends the nanoactuator. In some embodiments, the nanoactuator is capable of reversible contraction and extension.
Another aspect of the invention is a method of actuating a nanoactuator, the method comprising oxidizing or reducing a nanoactuator as described above. In some embodiments, oxidizing the nanoactuator expands the nanoactuator. In some embodiments, reducing the nanoactuator contracts the nanoactuator.
Another aspect of the invention is a method of preparing a nanoactuator, the method comprising providing an oligoviologen and a CBPQT ring capable of forming an inclusion complex, wherein the oligoviologen is threaded through the CBPQT ring. The method may further comprise stoppering the oligoviologen. In some embodiments, the CBPQT is provided in excess of the oligoviologen. In some embodiments, the oligoviologen and the CBPQT is provided in the presence of Zn dust and/or MeCN. In some embodiments, the oligoviologen is stoppered by a Cu-free alkyne-azide cycloaddition.
BRIEF DESCRIPTION OF THE DRAWINGS
Non-limiting embodiments of the present invention will be described by way of example with reference to the accompanying figures, which are schematic and are not intended to be drawn to scale. In the figures, each identical or nearly identical component illustrated is typically represented by a single numeral. For purposes of clarity, not every component is labeled in every figure, nor is every component of each embodiment of the invention shown where illustration is not necessary to allow those of ordinary skill in the art to understand the invention.
FIG. 1 shows structural formulae of the oligorotaxanes 3R|4BP.16PF6 and 3R|5BP.18PF6 composed of only positively charged components.
FIG. 2 shows structural formulas and graphical representations of the oligopseudorotaxanes 4V4(.+)⊂2CBPQT2(.+) and 5V5(.+)⊂2CBPQT2(.+) formed as a result of radical-pairing interactions.
FIG. 3A shows UV/Vis/NIR Absorption spectrophotometric titration of 4V4(.+) by CBPQT2(.+). Solvent: MeCN; black: [4V4(.+)]=10 μM; purple: (CBPQT2(.+))/(4V4(.+))=10.
FIG. 3B shows an enlargement of the spectra shown in FIG. 3A from 800 to 1500 nm. The rising peak intensity observed at 1120 nm upon titration indicates the formation of the trisradical inclusion complexes.
FIG. 4A shows UV/Vis/NIR Absorption spectrophotometric titration experiment of 5V5(.+) by CBPQT2(.+) 298 K. Solvent: MeCN; black: [5V5(.+)]=10 μM; purple: c (CBPQT2(.+))/c (5V5(.+))=12.
FIG. 4B shows the simulated curve for the determination of the binding constant between 5V5(.+) and CBPQT2(.+).
FIG. 5A shows cyclic voltammograms of 4V8+ and an equimolar mixture of 4V8+ and CBPQT4+. A glassy carbon working electrode, a platinum counter electrode, and a Ag/AgCl reference electrode were used in the characterization of 0.1 mM MeCN solutions of the oligoviologens at 298 K with 0.1 M TBAPF6 serving as the electrolyte. A scan rate of 200 mV s−1 was used in all analyses.
FIG. 5B shows cyclic voltammograms of 5V10+ and an equimolar mixture of 5V10+ and CBPQT4+. A glassy carbon working electrode, a platinum counter electrode, and a Ag/AgCl reference electrode were used in the characterization of 0.1 mM MeCN solutions of the oligoviologens at 298 K with 0.1 M TBAPF6 serving as the electrolyte. A scan rate of 200 mV s−1 was used in all analyses.
FIG. 6A shows a simulated co-conformation of the oligopseudorotaxane 4V4(.+)⊂2CBPQT2(.+) in different binding modes stabilized by radical-pairing interactions. The numbers (before the slash, in kcal mol−1) show their relative energies, demonstrating that the co-conformation with the greatest number (after the slash) of (BIPY.+)2 pairs have the highest stability.
FIG. 6B shows a simulated co-conformation of the oligopseudorotaxane 4V4(.+)⊂2CBPQT2(.+) in different binding modes stabilized by radical-pairing interactions. The numbers (before the slash, in kcal mol−1) show their relative energies, demonstrating that the co-conformation with the greatest number (after the slash) of (BIPY.+)2 pairs have the highest stability.
FIG. 6C shows a simulated co-conformation of the oligopseudorotaxane 4V4(.+)⊂2CBPQT2(.+) in different binding modes stabilized by radical-pairing interactions. The numbers (before the slash, in kcal mol−1) show their relative energies, demonstrating that the co-conformation with the greatest number (after the slash) of (BIPY.+)2 pairs have the highest stability.
FIG. 6D shows a simulated co-conformation of the oligopseudorotaxane 4V4(.+)⊂2CBPQT2(.+) in different binding modes stabilized by radical-pairing interactions. The numbers (before the slash, in kcal mol−1) show their relative energies, demonstrating that the co-conformation with the greatest number (after the slash) of (BIPY.+)2 pairs have the highest stability.
FIG. 7A shows a simulated co-conformation of the oligopseudorotaxane 5V5(.+)⊂2CBPQT2(.+) in different binding modes stabilized by radical-pairing interactions. The numbers (black, in kcal mol−1) show their relative energies, demonstrating that the co-conformation with the greatest number (red) of (BIPY.+)2 pairs have the highest stability.
FIG. 7B shows a simulated co-conformation of the oligopseudorotaxane 5V5(.+)⊂2CBPQT2(.+) in different binding modes stabilized by radical-pairing interactions. The numbers (black, in kcal mol−1) show their relative energies, demonstrating that the co-conformation with the greatest number (red) of (BIPY.+)2 pairs have the highest stability.
FIG. 7C shows a simulated co-conformation of the oligopseudorotaxane 5V5(.+)⊂2CBPQT2(.+) in different binding modes stabilized by radical-pairing interactions. The numbers (black, in kcal mol−1) show their relative energies, demonstrating that the co-conformation with the greatest number (red) of (BIPY.+)2 pairs have the highest stability.
FIG. 7D shows a simulated co-conformation of the oligopseudorotaxane 5V5(.+)⊂2CBPQT2(.+) in different binding modes stabilized by radical-pairing interactions. The numbers (black, in kcal mol−1) show their relative energies, demonstrating that the co-conformation with the greatest number (red) of (BIPY.+)2 pairs have the highest stability.
FIG. 8 shows syntheses of oligorotaxanes 3R|4BP16+ and 3R|5BP18+ by radical templation using Cu-free alkyne-azide cycloadditions.
FIG. 9A shows partial UV/Vis/NIR absorption spectra of MeCN solution of 4V4(.+) (c=10 μM) with 2 equiv, 10 equiv of CBPQT2(.+) and oligorotaxane 3R|4BP8(.+).
FIG. 9B shows enlargement of the corresponding spectra in FIG. 9A from 800 to 1400 nm, indicating that mechanical bonds enhance molecular recognition.
FIG. 9C shows a partial UV/Vis/NIR absorption spectra of MeCN solution of 5V5(.+) (c=10 μM) with 2 equiv, 12 equiv of CBPQT2(.+) and oligorotaxane 3R|5BP9(.+).
FIG. 9D shows enlargement of the corresponding spectra in FIG. 9C from 800 to 1400 nm, indicating that mechanical bonds enhance molecular recognition.
FIG. 10A shows a cyclic voltammogram of oligorotaxanes 3R|4BP16+. A glassy carbon working electrode, a platinum counter electrode, and a Ag/AgCl reference electrode were used in the characterization of 0.1 mM MeCN solutions of the oligoviologens at 298 K with 0.1 M TBAPF6 serving as the electrolyte. A scan rate of 200 mV s−1 was used in all the analyses.
FIG. 10B shows a cyclic voltammogram of oligorotaxanes 3R|5BP18+. A glassy carbon working electrode, a platinum counter electrode, and a Ag/AgCl reference electrode were used in the characterization of 0.1 mM MeCN solutions of the oligoviologens at 298 K with 0.1 M TBAPF6 serving as the electrolyte. A scan rate of 200 mV s−1 was used in all the analyses.
FIG. 10C shows a cyclic voltammogram of 4V8+ with 2 equiv of CBPQT4+. A glassy carbon working electrode, a platinum counter electrode, and a Ag/AgCl reference electrode were used in the characterization of 0.1 mM MeCN solutions of the oligoviologens at 298 K with 0.1 M TBAPF6 serving as the electrolyte. A scan rate of 200 mV s−1 was used in all the analyses.
FIG. 10D shows a cyclic voltammogram of 5V10+ with 2 equiv of CBPQT4+. A glassy carbon working electrode, a platinum counter electrode, and a Ag/AgCl reference electrode were used in the characterization of 0.1 mM MeCN solutions of the oligoviologens at 298 K with 0.1 M TBAPF6 serving as the electrolyte. A scan rate of 200 mV s−1 was used in all the analyses.
FIG. 10E shows a cyclic voltammogram of 4V8+ with 7 equiv of CBPQT4+. A glassy carbon working electrode, a platinum counter electrode, and a Ag/AgCl reference electrode were used in the characterization of 0.1 mM MeCN solutions of the oligoviologens at 298 K with 0.1 M TBAPF6 serving as the electrolyte. A scan rate of 200 mV s−1 was used in all the analyses.
FIG. 10F shows a cyclic voltammogram of 5V10+ with 7 equiv of CBPQT4+. A glassy carbon working electrode, a platinum counter electrode, and a Ag/AgCl reference electrode were used in the characterization of 0.1 mM MeCN solutions of the oligoviologens at 298 K with 0.1 M TBAPF6 serving as the electrolyte. A scan rate of 200 mV s−1 was used in all the analyses.
FIG. 11A shows an oligorotaxane with donor-acceptor interactions.
FIG. 11B shows an oligorotaxane where radical-pairing interactions stabilize the contracted form under reducing conditions and electrostatic repulsions favor the expanded form under oxidizing conditions.
FIG. 12 shows a scheme for one-step synthesis of 4BP.8PF6 from 1.6PF6.
FIG. 13 shows a scheme for one-step synthesis of 5BP.10PF6 from 3.8PF6.
FIG. 14 shows a scheme for the synthesis of 3R|4BP.16PF6 from templated by radical-pairing interactions
FIG. 15 shows a scheme for the synthesis of 3R|5BP.18PF6 from templated by radical-pairing interactions
FIG. 16 show a 1H NMR spectrum (500 MHz, CD3COCD3, 298K) of oligorotaxane 3R|4BP.16PF6.
FIG. 17A shows a 1H-1H gCOSY spectrum (500 MHz, CD3COCD3, 298K) of oligorotaxane 3R|4BP.16PF6.
FIG. 17B shows a 1H-1H gCOSY spectrum (500 MHz, CD3COCD3, 298K) of oligorotaxane 3R|4BP.16PF6.
FIG. 18 shows a 1H NMR spectrum (500 MHz, CD3COCD3, 298K) of oligorotaxane 3R|5BP.18PF6.
FIG. 19A shows a 1H-1H gCOSY spectrum (500 MHz, CD3COCD3, 298K) of oligorotaxane 3R|5BP.18PF6.
FIG. 19B shows a 1H-1H gCOSY spectrum (500 MHz, CD3COCD3, 298K) of oligorotaxane 3R|5BP.18PF6.
FIG. 20 shows a partial 1H NMR spectrum (400 MHz, CD3COCD3, 233K) of oligorotaxane 3R|5BP.18PF6.
FIG. 21A shows a analytical RP-HPLC chromatograms (H2O-MeCN, 0.1% TFA, 0-100% MeCN in 60 min, λ=254 nm) of 3R|4BP.16PF6.
FIG. 21B shows a analytical RP-HPLC chromatograms (H2O-MeCN, 0.1% TFA, 0-100% MeCN in 60 min, λ=254 nm) of 3R|5BP.18PF6. The higher charged oligorotaxane 3R|5BP.18PF6 has a shorter retention time on the column.
FIG. 22A shows an experimental HRMS (ESI) spectra of 3R|4BP.16PF6. Calculated for C176H188F78N22O8P13: 1540.6775 [M-3PF6]3+.
FIG. 22B shows a simulated HRMS (ESI) spectra of 3R|4BP.16PF6. Calculated for C176H188F78N22O8P13: 1540.6775 [M-3PF6]3+.
FIG. 22C shows an experimental and simulated HRMS (ESI) spectra of 3R|5BP.18PF6. Calculated for C194H204F90N24O8P15: 1724.7741 [M-3PF6]3+.
FIG. 22D shows a simulated HRMS (ESI) spectra of 3R|5BP.18PF6. Calculated for C194H204F90N24O8P15: 1724.7741 [M-3PF6]3+.
FIG. 23A shows determination of binding stoichiometry of CBPQT2(.+) with respect to 4V4(.+) in MeCN using the method of continuous variation with a Job plot showing the intensity of the trisradical absorption band attributable to 4V4(.+)⊂2CBPQT2(.+) host-guest complex against χ, which represents the CBPQT2(.+):4V4(.+) molar ratio.
FIG. 23B shows determination of binding stoichiometry of CBPQT2(.+) with respect to 4V4(.+) in MeCN using the method of continuous variation with absorption spectroscopy data used in the Job plot. The spectra were recorded at 298 K with [CBPQT2(.+)]+[4V4(.+)]=50 μM.
FIG. 24A shows determination of binding stoichiometry of CBPQT2(.+) with respect to 5V5(.+) in MeCN using the method of continuous variation with a Job plot showing the intensity of the trisradical absorption band attributable to 5V5(.+)⊂2CBPQT2(.+) host-guest complex against χ, which represents the CBPQT2(.+):5V5(.+) molar ratio. (b) Absorption spectroscopy data used in the Job plot. The spectra were recorded at 298 K with [CBPQT2(.+)]+[5V5(.+)]=50 μM.
FIG. 24B shows determination of binding stoichiometry of CBPQT2(.+) with respect to 5V5(.+) in MeCN using the method of continuous variation with absorption spectroscopy data used in the Job plot. The spectra were recorded at 298 K with [CBPQT2(.+)]+[5V5(.+)]=50 μM.
FIG. 25A shows a UV/Vis/NIR Absorption spectrophotometric titration experiment of 4V4(.+) by CBPQT2(.+) at 298 K. Solvent: MeCN; black: [4V4(.+)]=10 μM; purple: c (CBPQT2(.+))/c (4V4(.+))=10.
FIG. 25B shows a simulated curve for the determination of the binding constant between 4V4(.+) and CBPQT2(.+) from the data displayed in FIG. 25A.
FIG. 26A shows a UV/Vis/NIR Absorption spectrophotometric titration experiment of 5V5(.+) by CBPQT2(.+) 298 K. Solvent: MeCN; black: [5V5(.+)]=10 μM; purple: c (CBPQT2(.+))/c (5V5(.+))=12.
FIG. 26B shows a simulated curve for the determination of the binding constant between 5V5(.+) and CBPQT2(.+) from the data displayed in FIG. 25A.
FIG. 27 shows a UV/Vis/NIR spectra of 3R|4BP.16PF6 recorded at different temperatures ranging from 20° C. to 80° C. in MeCN at a concentration of 100 μM. The arrows in the figure denote the changing trend of the absorption intensities.
FIG. 28 shows a cyclic voltammogram titration of 4V4(.+)⊂2CBPQT2(.+). A glassy carbon working electrode, a platinum counter electrode, and a Ag/AgCl reference electrode were used in the characterization of 0.1 mM MeCN solutions of the 4V8+ at 298 K with 0.1 M TBAPF6 serving as the electrolyte. A scan rate of 200 mV s−1 was used in all the analyses.
FIG. 29 shows a cyclic voltammogram titration of 5V5(.+)⊂2CBPQT2(.+). A glassy carbon working electrode, a platinum counter electrode, and a Ag/AgCl reference electrode were used in the characterization of 0.1 mM MeCN solutions of the 5V10+ at 298 K with 0.1 M TBAPF6 serving as the electrolyte. A scan rate of 200 mV s−1 was used in all the analyses.
FIG. 30 shows a DPV profile of 3R|4BP.16PF6. The ratio of the area under each peak (from right to left) is 1:1:2.
FIG. 31 shows a DOSY Spectrum (500 MHz, CD3CN, 298 K) of 3R|4BP.16PF6.
FIG. 32A shows a Cw-EPR spectra (X-Band) of the reference compound BnV.+ (top line) and the oligorotaxane 3R|4BP8(.+) (bottom line) in MeCN at RT. Modulation Amplitude: 0.1 G. Microwave frequency: 9.8240. Power: 0.395 mW.
FIG. 32B shows a Cw-EPR spectra (X-Band) of 3R|4BP8(.+) in frozen MeCN at 4.1 K. Concentration: 0.2 mM. Modulation Amplitude: 0.1 G. Microwave frequency: 9.8240. Power: 0.395 mW.
FIG. 33A shows the molecular length of 4V8+ measured on the simulated co-conformations.
FIG. 33B shows the molecular length of 4V4(.+)⊚2CBPQT2(.+) measured on the simulated co-conformations.
DEFINITIONS
“Bridging subunit” (B) means a subunit that links viologen subunits to form an oligoviologen. Bridging subunit include p-xylene briding subunits.
“Linking subunit” (L) means a subunit capable of linking an oligioviologen with a stopper subunit. An oligoviologen and one or more linking subunits may together form the threading component of a rotaxane or pseudorotaxe.
“Macrocyclic component” (MC) means a molecule that has at least one ring (cycle) large enough to allow it to be threaded onto a linear subchain of another molecule. Macrocylic components include cyclobis(paraquat-p-phenylene) (CBPQT).
“Nanoacuator” means a molecular component responsible for moving or controlling a mechanism or system. When a control signal is received, the nanoactuator responds with mechanical motion. For example, when an electrochemical signal is received by a nanoactuator, the nanoactuator may respond by extending or contracting.
“Oligoviologen” (OV) means a component having different numbers of viologen subunits (V) linked with a bridging subunit. Oligoviologens may include 4,4′-bipyridinium (BIPY) subunits are linked by p-xylene bridging subunits. Oligoviologens may be described by the number of viologen subunits. For example, 4V may describe an oligoviologen having four BIPY subunits linked with three p-xylene bridging subunits or 5V may describe an oligoviologen having five BIPY subunits linked with four p-xylene bridging subunits. Oligoviologens may be threading components for a rotaxane or a pseudorotaxe.
“Pseudorotaxane” means a rotaxane-like molecular assembly in which the threading component(s) has(have) ends small enough to permit threading or dethreading of the macrocyclic component(s). A pseudorotaxane may be an “oligopseudorotaxane” when it comprises an oligomeric threading component. Pseudorotaxes may include unstoppered oligoviolgen threading components threaded through one or more macrocyclic components. Particular psuedorotaxens include 4V⊂2CBPQT and 5V⊂2CBPQT.
“Rotaxane” means a complex molecular assembly comprising at least one molecule with a linear section threaded through at least one macrocyclic part of another or the same molecule, and having end-groups large enough to prevent dethreading of the macrocyclic component. A rotaxane may be an “oligorotaxane” when it comprises an oligomeric threading component. Rotaxes may include stoppered oligoviolgen threading components threaded through one or more macrocyclic components. Particular rotaxanes include 3R|4BP and 3R|5BP.
“Stopper subunit” (S) means a group bulky enough to prevent dethreading of a given macrocyclic component from a threading component or its translocation to another linear section of the threading component.
“Threading component” (TC) means a molecule with at least one linear section onto which at least one macrocyclic component is threaded. A threading component may be an “oligomeric threading component” when it comprises repeating subunits.
“Viologen subunit” (V) means a subunit that is derivative of 4,4′-bipyridine (C10H8N2). Viologens include 4,4′-bipyridinium (BIPY) subunits.
DETAILED DESCRIPTION
Provided herein are nanoactuators capable of receiving a control signal and responding with mechanical motion. The nanoactuators disclosed herein comprise foldameric rotaxanes based on a strategy for creating foldameric oligorotaxanes composed of only positively charged components. The rotaxanes comprise threading components comprised of oligoviologens in which different numbers of 4,4′-bipyridinium (BIPY2+) subunits are linked by p-xylene bridges, and the treading components are shown to be capable of being threaded by cyclobis(paraquat-p-phenylene) (CBPQT4+) rings following the introduction of radical-pairing interactions under reducing conditions. UV/Vis/NIR Spectroscopic and electrochemical investigations suggest that the reduced oligopseudorotaxanes fold into highly ordered secondary structures as a result of the formation of BIPY.+ radical cation pairs. Furthermore, by installing bulky stoppers at each end of the oligopseudorotaxanes by means of Cu-free alkyne-azide cycloadditions, their analogous oligorotaxanes, which retain the same stoichiometries as their progenitors, can be prepared. Solution-state studies of the oligorotaxanes indicate that their mechanically interlocked structures lead to the enforced interactions between the dumbbell and ring components, allowing them to fold (contract) in their reduced states and unfold (expand) in their fully oxidized states as a result of Coulombic repulsions. This electrochemically controlled reversible folding and unfolding process, during which the oligorotaxanes experience length contractions and expansions, is reminiscent of the mechanisms of actuation associated with muscle fibers.
There are a number of potential application for these rotaxanes. Examples of application include, but are not limited to, electrochemically responsive artificial molecular muscles, electronic information storage devices, functional molecular actuators, organic molecular switches, semiconducting organic radical materials, shape memory materials.
A number of advantages can be realized from these rotaxanes. The actuations of the oligorotaxanes can be achieved by both chemical and electrochemical stimuli. The actuation of the oligorotaxanes are less influenced by changes in concentrations in solution. Introduction of the mechanical bond further regulates the co-conformations of the oligorotaxanes. Radical-pairing interactions provide stronger conformational control than analogous donor-acceptor based systems. Moreover, coulombic repulsions force the secondary structures of the oligorotaxanes to extend, improving the working efficiency.
Herein we describe a new class of functional foldameric oligorotaxanes composed of only positively charged components whose construction rely on the interactions between the oligoviologens threads and the CBPQT4+ ring under reducing conditions. Structural formulae of exemplary rotaxes are provided in FIG. 1. This design is based on the consideration that, unlike the donor-acceptor-based examples wherein the folded secondary structures are “permanent” aside from the influence of solvent and temperature, the radical-pairing interactions enable the co-conformations of the resulting oligorotaxanes to be switched reversibly between folded and unfolded states by altering the external potential. Specifically, in their oxidized states, the positively charged dumbbells apparently become extended and the CBPQT4+ rings are repelled from each other and also from the dumbbells as a result of Coulombic repulsion. Upon reduction back to their radical states, however, solution studies indicate the formation of folded structures driven by radical-pairing interactions. This reversible process, which switches the interactions of bipyridinium units between being repulsive and attractive and giving rise to the extension and contraction of the oligorotaxane chains, can lead to drastic changes in their lengths. This property makes it possible for us to control the operation of artificial molecular motors. The relative movements of the components in these oligorotaxanes, at the behest of external stimuli, are reminiscent of the actions of macroscopic springs.[34] In addition, these molecular-level movements, resembling those of the workings of muscle tissue, can potentially be developed further in the context of artificial molecular muscles that respond to electrochemical stimuli.[35-39]
Precise designs of molecular components are necessary in order to optimize noncovalent bonding interactions required for the efficient production of MIMs employing template-directed strategies. We have demonstrated that strong intra- and intermolecular radical-pairing interactions come into play upon reduction of linear oligoviologen chains in which the dicationic BIPY2+ units are separated periodically by xylene linkers, rendering them to fold both in solution and in the solid-state. [40] It should be emphasized, however, that the nature of the folded (super)structures of these oligoviologens are either susceptible to changes in concentration or (ii) lack imposed linear geometries, i.e., they can form loops, which limits their potential applications at least as far as serving as a prototype for artificial molecular muscles is concerned. As a consequence, it is of paramount importance to introduce ring components on to the oligoviologens in order to arrest the chains self-entangling and further regulate the folded secondary superstructures so that they are (i) less influenced by changes in concentration since they are MIMs, and obliged to adopt linear geometries. On the basis of these considerations, we have chosen oligoviologens with four and five BIPY2+ units—namely 4V8+ and 5V10+—to serve as the linear components of the oligorotaxanes (FIG. 2), since (iii) their self-folding tendencies[40] under reducing conditions are less pronounced, when compared with their longer analogues, making it possible for them to interact with the rings to form the desired oligorotaxanes, while (iv) compared with their shorter analogues, they can potentially bind more CBPQT2(.+) rings under reducing conditions, a situation which is expected to provide additional (co)-conformational control during the folding and unfolding processes by (v) generating more BIPY.+ recognition sites to stabilize their radical-state superstructures, and (vi) providing stronger Coulombic repulsion so as to force the secondary structures to become extended upon oxidation.
As the key intermediates in the construction of these oligorotaxanes, the formation (FIG. 2) of the oligopseudorotaxanes between the reduced oligoviologens—namely 4V4(.+) and 5V5(.+)—and the CBPQT2(.+) ring, was first of all investigated (FIGS. 3A and 3B) by performing UV/Vis/NIR titrations. Following the reduction of the oligoviologen 4V8+ to its radical cationic state by Zn dust, the absorption spectrum of a MeCN solution of 4V4(.+) (10 μM) was recorded at room temperature. Next, an increasing amount of CBPQT2(.+) from 1 to 10 equiv was titrated into this MeCN solution and the UV/Vis/NIR spectra were recorded. The results reveal (FIGS. 3A and 3B) that, when only 4V4(.+) is present in the solution, an absorption band around 900 nm is observed, indicating the formation of BIPY.+ dimers induced by intramolecular radical-pairing interactions.[40] Upon the addition of CBPQT2(.+), however, a new absorption band emerges (FIGS. 3A and 3B) centered on 1110 nm, which clearly indicates the formation of trisradical complexes. [41] As the concentration of CBPQT2(.+) in the solution increases, the intensity of the trisradical band grows with a gradual decrease in its intensity increment until finally a saturation point is reached, a situation which suggests the maximum number of BIPY.+ units on the 4V4(.+) have been encircled by the CBPQT2(.+) rings. It is also noteworthy that this absorption band is significantly red-shifted, compared (1066 nm) with the example of the inclusion complex MV.+⊂CBPQT2(.+) between reduced methyl viologen (MV.+) and [32] This observation possibly comes about because of the fact that 4V4(.+) binds multiple CBPQT2(.+) rings in solution, such that the resulting radical pairs interact with each other intermolecularly through space to form (FIG. 2) a continuous π-stack, giving rise to a narrower electron-migrating energy gap—in other words, a red-shifted absorption.
A similar phenomenon was observed in the case of 5V5(.+), where an absorption band, centered on 1140 nm, emerges (FIG. 4A) immediately after the addition of CBPQT2(.+), indicating rapid formation of trisradical inclusion complexes. It is worth noting that the absorption band in the case of 5V5(.+) is further red-shifted with respect to that observed in the case of 4V4(.+), presumably because of the participation of an additional BIPY.+ subunit in the n-stack results (FIG. 2) in a stacked superstructure of even greater length. All these observations suggest that the CBPQT2(.+) rings interact strongly with both 4V4(.+) and 5V5(.+), in spite of the existence of competitive intramolecular radical-pairing interactions within 4V4(.+) and 5V5(.+) themselves. This situation possibly pertains because BIPY.+ units prefer to stack in a face-to-face manner in solution, and the CBPQT2(.+) rings, whose rigid geometry already dictates that two BIPY.+ units be parallel, facilitates this type of stacking fashion.
In order to determine the binding stoichiometry between both the reduced oligoviologens 4V4(.+) and 5V5(.+), and CBPQT2(.+), Job plots were performed. The titrations reveal that CBPQT2(.+) forms 2:1 complexes with both 4V4(.+) and 5V5(.+) in MeCN solutions, confirming the formation of the oligopseudorotaxanes. According to this binding stoichiometry, we found that the stronger interactions between CBPQT2(.+) and 4V4(.+), as well as between CBPQT2(.+) and 5V5(.+), compared to the self-dimerization of 4V4(.+) and 5V5(.+), are also supported by the results of DFT calculations. The formation enthalpies (ΔH) of the inclusion complex 4V4(.+)⊂2CBPQT2(.+) and 5V5(.+)⊂2CBPQT2(.+) are 66.1 and 73.6 kcal mol-1, whereas the ΔH values for the 4V4(.+) and 5V5(.+) dimers are only 42.7 and 48.4 kcal mol-1, respectively, indicating that the organized geometry provided by the CBPQT2(.+) rings amount to approximately 24 kcal mol-1 stabilizing energy. More importantly, these 2:1 binding stoichiometries support the formation of favorable radical-pairing interactions between all of the BIPY.+ units in both the oligoviologens and the CBPQT2(.+) rings—a co-conformation which is in a good agreement with the red-shifted band observed in the UV/Vis/NIR spectra—as a consequence of the assembly (FIG. 2) of well-defined secondary structures. Furthermore, the binding constants between reduced oligoviologens and CBPQT2(.+) were calculated, demonstrating both 4V4(.+) and 5V5(.+) bind strongly (Ka˜109M−2) with two CBPQT2(.+) rings in solution.
In order to elucidate the binding mechanism between the reduced oligoviologens and CBPQT2(.+), cyclic voltammetry (CV) was also performed. The CV (FIG. 5A) of an equimolar mixture of 4V8+ and CBPQT4+ reveals the presence of a single reduction peak (−300 mV, peak potential) leading to the radical species. Indeed, six electrons are involved in this reduction process: two electrons go into the CBPQT4+ ring, forming the diradical dication CBPQT2(.+), and four electrons go to 4V8+, forming the tetraradical tetracation 4V4(.+). As a consequence of this simultaneous six-electron process, formation of the 4V4(.+)⊂CBPQT2(.+) inclusion complex occurs spontaneously. It is noteworthy that the reduction potential at −300 mV is cathodically shifted significantly, compared with those for the individual 4V8+ oligomer (at −330 mV) and the CBPQT4+ rings (at −360 mV)29, i.e., the mixture is easier to reduce, indicating that the formation of the inclusion complex stabilizes the radical species. On re-oxidation, the result is that one of the BIPY.+ radical cations of the complexed CBPQT2(.+) associates more weakly with the 4V4(.+) than the other BIPY.+, leading to the conclusion that the oxidation of this inclusion complex occurs in a stepwise manner, with the weaker interacting BIPY.+ in the CBPQT2(.+) ring and the unpaired BIPY.+ in 4V4(.+) being oxidized first of all at a potential at −209 mV, leaving the strongly interacting BIPY.+ subunits to become oxidized at more positive potentials, i.e., +32 mV.
In the case of 5V10+ and CBPQT4+, an equimolar mixture also gives (FIG. 5B) a more positive reduction potential at −264 mV, compared with those of their individual components, indicating the formation of the inclusion complex. More significantly, when the inclusion complex is undergoing oxidation, it registers the first potential at −205 mV, a value which is close to that of the inclusion complex between 4V8+ and CBPQT4+, indicating that the unpaired BIPY.+ radical cations have a similar tendency to become oxidized. By contrast, the second potential is shifted slightly to +45 mV, presumably because the presence of an additional BIPY.+ radical cation makes the dissociation between 5V5(.+) and CBPQT2(.+) even more difficult.
Computational studies were carried out in order to demonstrate how the superstructures of the oligopseudorotaxanes are regulated by radical-pairing interactions. In the case of 4V4(.+)⊂2CBPQT2(.+), we examined four possible co-conformations, and discovered that the one (FIG. 6A) incorporating two CBPQT2(.+) rings which are centered on the first and the third BIPY.+ subunits, that allows all the BIPY.+ radical cations, in both 4V4(.+) and in the CBPQT2(.+) rings to stack employing a total of seven (BIPY.+)2 radical pairs, has the highest stability. The open superstructures with the middle BIPY.+ subunit in 4V4(.+) twisted away (FIGS. 6B-C), which releases some strain at the angle of BIPY.+-paraxylene-BIPY.+ in 4V4(.+), is not sufficient to compensate for the loss of one radical pair—leaving six (BIPY.+)2 radical pairs in total—between the BIPY.+ radical cations, rendering them much higher energy (2˜7 kcal mol−1) co-conformations.
Four co-conformations of 5V5(.+)⊂2CBPQT2(.+), where the one with the largest number of (BIPY.+)2 pairs is (FIG. 7A) the most stable co-conformation, constitutes a result which is in a good agreement with 4V4(.+)⊂2CBPQT2(.+). It is also noteworthy that, compared with the 4V4(.+)⊂2CBPQT2(.+) superstructure, once the continuous BIPY.+ stacking is interrupted in the case of 5V5(.+)⊂2CBPQT2(.+), the resulting co-conformations (FIGS. 7B-C) are significantly more destabilized (10.0, 14.1 and 20.2 kcal mol−1), indicating that the π-π stacking contributes to the stabilization energy. These observations can be rationalized by the presence of a continuous π-π stack, in which all the orbitals can interact with each other, leading to a lower orbital binding energy. In the case of the longer π-π stack, 5V5(.+)⊂2CBPQT2(.+), this effect is even more pronounced. The computational investigations also reveal how the number of BIPY.+ subunits affects the secondary structures of the possible co-conformations, providing a unique example where longer oligoviologens have a higher tendency of folding.
Having shown that both of oligopseudorotaxanes prefer a highly ordered secondary structures in solution, we decided to investigate whether this behavior can be promoted in the case of the oligorotaxanes and so facilitate potential applications. Therefore, we carried out the syntheses of the oligorotaxanes, which rely on the templation present in their oligopseudorotaxane progenitors. In the beginning, an azide group is attached, by means of hexamethylene chain linkers to each end of the oligoviologens. These linkers are expected to be long enough to act as collecting zones for the CBPQT4+ rings in their fully oxidized states. The azide-functionalized oligoviologens are then mixed with a gross excess (10 equiv) of CBPQT4+ in MeCN under an Ar atmosphere. Upon reduction to their radical cationic states, the solutions turn, first of all, to dark blue and then, after a few minutes, to an intense purple color, indicating the formation of the inclusion complexes. After stirring the solutions overnight to allow the formation of the inclusion complexes to reach thermodynamic equilibrium, a bulky alkyne 4, which acts as the stopper precursor, is added and the solutions are stirred for a further 20 days. The highly charged oligorotaxanes, 3R|4BP.16PF6 and 3R|5BP.18PF6, were isolated (FIG. 8) from the corresponding reaction mixtures by preparative-HPLC in yields43 of 10 and 6%, respectively. 1H NMR and 1H-1H COSY spectra show (See SI, Section 3) that the CBPQT4+ rings become located, after oxidation, on the hexamethylene chains as a result of Coulombic repulsions, as evidenced by the significantly lower resonating frequencies (<0 ppm) of protons on the hexamethylene chains. Therefore, it is apparent that 3R|4BP16+ and 3R|5BP18+ are fully stretched in their oxidized states. It is also noteworthy that both the oligorotaxanes 3R|4BP16+ and 3R|5BP18+ are composed of one oligoviologen dumbbell and two CBPQT4+ rings, as confirmed by the 1H NMR integration and high resolution mass spectrometry (HR-MS). The outcome is also consistent with the solution-state experiments performed on the oligopseudorotaxanes, demonstrating that the binding stoichiometries are retained during the production of the oligorotaxanes, in spite of the fact that the constitutions of oligoviologens are slightly different.
With the two oligorotaxanes 3R|4BP16+ and 3R|5BP18+ in hand, we then set out to investigate the behavior of their radical cationic states—namely 3R|4BP8(.+) and 3R|5BP9(.+)—in MeCN solutions. The comparison of their UV/Vis/NIR spectra (FIGS. 9A-9D) with those of the oligopseudorotaxanes shows that, while the peaks around 600 nm still remain (FIGS. 9A and 9C) a feature characteristic of the free CBPQT2(.+) rings in the case of oligopseudorotaxane, they are replaced by blue-shifted absorption bands centered on 550 nm, in the case of 3R|4BP8(.+) and 3R|5BP9(.+), an observation which is typical of strong BIPY.+ radical pimerization.44 This absorption peak assignment is further confirmed by a variable-temperature UV/Vis/NIR experiment. Moreover, the absorption intensities of the trisradical bands of 3R|4BP8(.+) and 3R|5BP9(.+) are significantly higher (FIGS. 9B and 9D) than those of the 1:2 molar mixtures of (i) 4V4(.+) and (ii) 5V5(.+) with CBPQT2(.+), despite their almost identical chemical compositions. Indeed, we found that the absorption intensities are close to those of the saturated situations in the cases of oligopseudorotaxanes. These observations suggest that the molecular recognition between 4V4(.+), 5V5(.+) and CBPQT2(.+), along with the strengths of the radical-pairing interactions are enhanced on account of the interlaced superstructures, which restrict the motions of the CBPQT2(.+) rings so that they rest exclusively along the oligoviologen chains, facilitating the folding process.
In order to gain a deeper insight into the mechanically interlocked structures and understand the properties of the radical-radical pairing recognition between the interlocked dumbbells and ring components, we performed (FIGS. 10A-10B) CV experiments on the oligorotaxanes 3R|4BP16+ and 3R|5BP18+ and compared the results with those obtained (FIGS. 10C-10F) using the oligopseudorotaxanes. It turns out (FIGS. 10A-10B) that the CV profiles of the oligorotaxanes display three reduction peaks with potentials at −60, −190 and −271 mV for 3R|4BP16+ and at 0, −174 and −273 mV for 3R|5BP18+. The two additional reduction peaks in both cases, whose potentials are shifted toward positive values compared with those of their oligopseudorotaxane progenitors, can be interpreted in terms of a stepwise formation of the (BIPY.+)n pairs in 3R|4BP16+ and 3R|5BP18+ upon reduction. In the case of 3R|4BP16+, all the BIPY2+ units experience repulsion in its fully oxidized state. Upon reduction, a two-electron process is observed at a potential of 60 mV. Considering that the 4V8+ dumbbell has a higher reduction potential than the CBPQT4+ rings, we believe that both these electrons go preferentially into the dumbbell components in order to relief the repulsion between the BIPY2+ units. Subsequently the oligorotaxane accepts another two electrons at a potential of 190 mV, whereupon both rings become reduced to CBPQT2+(.+), leading to the translation from the hexamethylene chains to the BIPY.+ radical cations of the dumbbell so as to form (BIPY.+)2 dimeric units. The reduction of the remaining four BIPY2+ dication in both the dumbbell and the rings gives rise to the formation of trisradicals. Differential pulse voltammetry (DPV) experiments confirm the numbers of electrons involved in each step of the reduction process. Upon re-oxidation, these reduction processes are fully reversible, allowing the partially oxidized intermediates to be observed at −115 mV for 3R|4BP16+ and at −135 mV for 3R|5BP18+. These reduction processes are not observed in the corresponding oligopseudorotaxanes. These results suggest that the radical cationic forms of the oligorotaxanes are more difficult to oxidize than their oligopseudorotaxane progenitors, demonstrating their increased stabilities as a consequence of their mechanically interlocked structures, enforcing the BIPY.+ radical cations to come into close proximity.
In summary, we have reported a new class of oligorotaxanes, 3R|4BP.16PF6 and 3R|5BP.18PF6, which combine the advantages of both foldamers and mechanically interlocked molecules under reducing conditions. Composed of only positively charged components, it is only possible to access them by a template-directed approach that takes advantage of radical-pairing interactions, followed by a stoppering protocol employing Cu-free alkyne-azide cycloadditions. The formation of the key intermediates, oligopseudorotaxanes 4V4(.+)⊂2CBPQT2(.+) and 5V5(.+)⊂2CBPQT2(.+), are confirmed by both spectroscopic and electrochemical studies in solution. Computational studies reveal that these oligopseudorotaxanes preferentially form highly ordered secondary structures, wherein the CBPQT2(.+) ring components play an important role in promoting all the BIPY.+ radical cations to stack in extended arrays, in order to maximize the stabilizing effect resulting from radical-pairing interactions. Comparison of the properties of the oligopseudorotaxanes with those of the oligorotaxanes shows that the secondary structures are further regulated in the oligorotaxanes since the components are obliged to remain in close proximity. More importantly, the redox-controlled actuation processes present (FIG. 11B) in these oligorotaxanes, which allow their secondary structures to be switched between folded and unfolded states, differentiate them from donor-acceptor,[20, 28] interactions-based systems (FIG. 11A). Moreover, these actuation processes lead to contractions and extensions of the oligorotaxanes, rendering them ideal prototypes of artificial molecular muscles. This research sheds light on the behavior of foldameric oligorotaxanes so that their structural and mechanical properties can be harnessed in devices.
Computational Studies of Oligopseudorotaxanes 4V4(.+)⊂2CBPQT2(.+) and 5V5(.+)⊂2CBPQT2(.+).
The folded co-conformations of the two oligopseudorotaxanes, 4V4(.+)⊂2CBPQT2(.+) and 5V5(.+)⊂2CBPQT2(.+), were investigated using the M06 of density functional theory. In addition to the general gradient approximation and kinetic energy functionals, M06 includes hybrid exact exchange to account for the localization needed to give good energies and has been optimized to account for van der Waals interactions important in supramolecular complexes. The superstructures were optimized at the M06L using the 6-31G* basis set while more accurate energies were obtained with single-point calculations at the M06 level using the 6-311++G** basis set. All calculations included solvation based on the Poisson-Boltzmann solvation model for MeCN (∈=37.5 and R0=2.18 Å) implemented in Jaguar 7.7.
Miscellaneous
All methods described herein can be performed in any suitable order unless otherwise indicated herein or otherwise clearly contradicted by context. The use of any and all examples, or exemplary language (e.g., “such as”) provided herein, is intended merely to better illuminate the invention and does not pose a limitation on the scope of the invention unless otherwise claimed. No language in the specification should be construed as indicating any non-claimed element as essential to the practice of the invention.
Preferred aspects of this invention are described herein, including the best mode known to the inventors for carrying out the invention. Variations of those preferred aspects may become apparent to those of ordinary skill in the art upon reading the foregoing description. The inventors expect a person having ordinary skill in the art to employ such variations as appropriate, and the inventors intend for the invention to be practiced otherwise than as specifically described herein. Accordingly, this invention includes all modifications and equivalents of the subject matter recited in the claims appended hereto as permitted by applicable law. Moreover, any combination of the above-described elements in all possible variations thereof is encompassed by the invention unless otherwise indicated herein or otherwise clearly contradicted by context.
Examples
Materials and General Methods
Chemicals were purchased as reagent grade and used without further purification. Commercial grades of anhydrous MeCN and N,N-dimethylformamide (DMF) were used as solvents in all reactions. Benzyl viologen BnV.2PF6 and compounds 1.6PF6 and 3.8PF6 were prepared[40, 42] according to literature procedures. Thin layer chromatography (TLC) was performed on silica gel 60F254 (E Merck). Column chromatography was carried out on silica gel 60F (Merck 9385, 0.040-0.063 mm). High performance liquid chromatography (HPLC) was performed on a preparative RP-HPLC instrument, using a C18 column (Agilent, 10 μm packing, 30 mm×250 mm). The eluents employed were MeCN and H2O, both mixed with 0.1% (v/v) trifluoroacetic acid (TFA). The detector was set to λ=254 nm. HPLC Analyses were performed on an analytical RP-HPLC instrument, using a C18 column. For UV/Vis/Near Infrared (NIR) studies, all sample preparations were completed in an Argon-filled atmosphere. Samples were loaded into quartz 1 cm tubes and sealed with a clear ridged UV doming epoxy (IllumaBond 60-7160RCL) and used immediately after preparation. Nuclear magnetic resonance (NMR) spectra were recorded at 298 K on Bruker Avance 500 and 600 spectrometers, with working frequencies of 500 and 600 MHz for 1H, and 125 and 150 MHz for 13C nuclei, respectively. Chemical shifts are reported in ppm relative to the signals corresponding to the residual non-deuterated solvents.3 EPR Spectra were recorded using a Bruker Elexsys E580-X EPR spectrometer, equipped with a variable Q dielectric resonator (ER-4118X-MD5-W1). Samples were prepared by reduction with cobaltocene and the solution was loaded into quartz 1.4 mm tubes and sealed with a clear ridged UV doming epoxy (IllumaBond 60-7160RCL). Samples were used immediately after preparation. Solution CW-EPR spectra were collected with a 0.4 G modulation amplitude 5.12 ms time constant and 20.48 ms conversion time. High-resolution mass spectra were measured on an Agilent 6210 Time-of-Flight (TOF) LC-MS, using an ESI source, coupled with Agilent 1100 HPLC stack, using direct infusion (0.6 mL min−1). Measurements at X-band (9.5 GHz) were performed with a Bruker Elexsys E580, equipped with a variable Q dielectric resonator (ER-4118X-MD5-W1). Cyclic voltammetry experiments were performed on a Princeton Applied Research 263 A Multipurpose instrument interfaced to a PC, using a glassy carbon working electrode (0.071 cm2, Cypress system). The electrode surface was polished routinely with an alumina/water slurry on a felt surface immediately before use. The counter electrode was a Pt coil and the reference electrode was an AgCl coated Ag wire. The concentrations of the samples were 1 mM in 100 mM electrolyte solutions of tetrabutylammonium hexafluorophosphate (TBAPF6) in MeCN.
Scheme S1. One-Step Synthesis of 4BP.8PF6 from 1.6PF6
4BP.8PF6: 1.6PF6 (90 mg, 0.05 mmol) and 2 (148 mg, 0.5 mmol) were dissolved in DMF (10 mL) at room temperature. The reaction mixture was heated to 90° C. for 5 days and cooled down to room temperature, then Me2CO was added to the solution. The resulting precipitate was filtered off, washed with Me2CO, re-dissolved in H2O, and re-precipitated by adding an excess of NH4PF6 (FIG. 12). The solid was filtered off and washed with H2O, MeOH and finally Et2O to afford 4BP.8PF6 as a yellow solid (85 mg, 75%). 1H NMR (500 MHz, CD3CN): δ=8.98 (d, J=6.9 Hz, 12H), 8.92 (d, J=6.9 Hz, 4H), 8.42 (d, J=5.1 Hz, 12H), 8.39 (d, J=5.1 Hz, 4H), 7.62 (s, 12H), 5.87 (s, 12H), 4.64 (t, J=7.6 Hz, 4H), 3.33 (t, J=6.8 Hz, 4H), 2.05 (p, J=7.4 Hz, 4H), 1.69-1.60 (m, 4H), 1.51-1.38 (m, 8H). 13C NMR (126 MHz, CD3CN): δ=150.1, 145.3, 134.0, 130.0, 127.2, 127.2, 126.8, 63.5, 50.5, 30.4, 27.8, 25.3, 24.7. HRMS (ESI): m/z calcd for C76H80F36N14P6 [M-2PF6]2+ 1029.7279. found 1029.7287.
Scheme S2. One-Step Synthesis of 5BP.10PF6 from 3.8PF6
5BP.10PF6: 3.8PF6 (70 mg, 0.03 mmol) and 2 (89 mg, 0.3 mmol) were dissolved in DMF (10 mL) at room temperature. The reaction mixture was heated to 90° C. for 5 days and cooled down to room temperature, then Me2CO was added to the solution. The resulting precipitate was filtered off, washed with Me2CO, re-dissolved in H2O, and re-precipitated by adding an excess of NH4PF6. (FIG. 13) The solid was filtered off and washed with H2O, MeOH and finally Et2O to afford 5BP.10PF6 as a yellow solid (61 mg, 70%). 1H NMR (500 MHz, CD3CN): δ=8.98 (d, J=6.9 Hz, 16H), 8.92 (d, J=6.9 Hz, 4H), 8.42 (d, J=5.1 Hz, 16H), 8.39 (d, J=5.1 Hz, 4H), 7.62 (s, 12H), 7.61 (s, 4H), 5.87 (s, 16H), 4.64 (t, J=7.6 Hz, 4H), 3.33 (t, J=6.8 Hz, 4H), 2.05 (p, J=7.4 Hz, 4H), 1.69-1.60 (m, 4H), 1.51-1.38 (m, 8H). 13C NMR (126 MHz, CD3CN): δ=150.1, 145.3, 134.0, 130.0, 127.2, 127.2, 126.9, 63.5, 50.5, 30.4, 27.8, 25.3, 24.7. HRMS (ESI): m/z calcd for C94H96F48N16P8 [M-2PF6]2+ 1304.7578. found 1304.7573.
Scheme S3. Synthesis of 3R|4BP.16PF6 Templated by Radical-Pairing Interactions
3R|4BP.16PF6: S3.8PF6 (46 mg, 0.02 mmol) and CBPQT.4PF6 (220 mg, 0.2 mmol) were dissolved in degassed MeCN (20 mL) in an Ar-filled glove box. An excess of Zn dust was added to this solution. After stirring for 30 mins, the colorless solution turned dark purple and the solid was filtered off. The purple filtrate was stirred overnight before compound 4 (51 mg, 0.2 mmol) was added. The reaction mixture was then heated to 40° C. and stirred under an Ar atmosphere for 20 days, during which time the reaction was monitored by RP-HPLC. (FIG. 14) The solvent was evaporated off, and the residue was purified by prep-HPLC (H2O-MeCN, 0.1% TFA, 0-75% MeCN in 35 min). The fraction was combined and the solvent was evaporated off, and the solid was re-dissolved in H2O, and precipitated by addition of an excess of NH4PF6. The solid was filtered off and washed with H2O, MeOH and finally Et2O to afford 3R|4BP.16PF6 as a white solid (9 mg, 10%). 1H NMR (500 MHz, d6-Me2CO): δ=9.57 (d, J=7.2 Hz, 12H), 9.51 (d, J=6.2 Hz, 8H), 9.48 (d, J=6.2 Hz, 8H), 9.28 (d, J=6.2 Hz, 4H), 8.90 (d, J=6.4 Hz, 16H), 8.84 (d, J=6.4 Hz, 4H), 8.82-8.78 (m, 12H), 7.90-7.80 (m, 12H), 7.77 (s, 16H), 6.36-5.99 (m, 28H), 4.78 (t, J=8.4 Hz, 3H), 4.38 (s, 4H), 4.25 (s, 4H), 2.63 (t, J=8.4 Hz, 4H), 1.60 (br, 4H), 1.14 (s, 18H), 1.12 (s, 18H), 0.09 (br, 4H), 0.58 (br, 4H), 1.46 (br, 4H). 13C NMR (126 MHz, CD3CN): δ=158.6, 150.7, 148.5, 146.2, 146.1, 145.6, 145.4, 136.3, 135.0, 130.6, 130.5, 130.4, 127.7, 127.6, 127.5, 76.7, 75.1, 64.9, 64.2, 48.9, 31.4, 31.3, 28.5, 28.3, 28.2, 25.9, 25.8, 25.7, 25.4. HRMS (ESI): m/z calcd for C176H188F78N22O8P13 [M-3PF6]3+ 1540.6775. found 1540.6770.
Scheme S4. Synthesis of 3R|5BP.18PF6 Templated by Radical-Pairing Interactions
3R|5BP.18PF6: 5BP.10PF6 (58 mg, 0.02 mmol) and CBPQT.4PF6 (220 mg, 0.2 mmol) were dissolved in degassed MeCN (20 mL) in an Ar-filled glove box. An excess of Zn dust was added to this solution. After stirring for 30 mins, the colorless solution turned dark purple and the solid was filtered off. The purple filtrate was stirred overnight before compound 4 (51 mg, 0.2 mmol) was added. The reaction mixture was then heated to 40° C. and stirred under an Ar atmosphere for 20 days, during which time the reaction was monitored by RP-HPLC (H2O-MeCN, 0.1% TFA, 0-75% MeCN in 35 min). (FIG. 15) The solvent was evaporated off, and the residue was purified by prep-HPLC. The fraction was combined and the solvent was evaporated off, and the solid was re-dissolved in H2O, and precipitated by addition of an excess of NH4PF6. The solid was filtered off and washed with H2O, MeOH and finally Et2O to afford 3R|5BP.18PF6 as a yellow solid (6 mg, 6%). 1H NMR (500 MHz, d6-Me2CO): δ=9.57 (d, J=7.2 Hz, 12H), 9.51 (d, J=6.2 Hz, 8H), 9.48 (d, J=6.2 Hz, 8H), 9.28 (d, J=6.2 Hz, 4H), 8.90 (d, J=6.4 Hz, 16H), 8.84 (d, J=6.4 Hz, 4H), 8.82-8.78 (m, 12H), 7.90-7.80 (m, 12H), 7.77 (s, 16H), 6.36-5.99 (m, 28H), 4.78 (t, J=8.4 Hz, 3H), 4.38 (s, 4H), 4.25 (s, 4H), 2.63 (t, J=8.4 Hz, 4H), 1.60 (br, 4H), 1.14 (s, 18H), 1.12 (s, 18H), 0.05 (br, 4H), 0.61 (br, 4H), 1.51 (br, 4H). 13C NMR (126 MHz, CD3CN): δ=158.6, 150.7, 148.5, 146.2, 146.1, 145.6, 145.4, 136.3, 135.0, 130.6, 130.5, 130.4, 127.7, 127.6, 127.5, 76.7, 75.1, 64.9, 64.2, 48.9, 31.4, 31.3, 28.5, 28.3, 28.2, 25.9, 25.8, 25.7, 25.4. HRMS (ESI): m/z calcd for C194H204F90N24O8P15 [M-3PF6]3+ 1724.7741. found 1724.7800.
1H NMR Spectroscopic Analysis of Oligorotaxane 3R|4BP.16PF6 and 3R|5BP.18PF6.
Compound 3R|4BP.16PF6 has a simple 1H NMR spectrum (FIG. 16) on account of its high symmetry and only four BIPY2+ subunits. In its oxidized state, the positive-charged CBPQT4+ rings are positioned on the hexamethylene chains as a result of the Coulombic repulsions with the BIPY2+ subunits of the thread, giving rise to the substantially lower resonating frequency (<0 ppm) of protons on the hexamethylene chains. In addition, the methyl groups of the stopper separate into two set of peaks, as a result of heterotopic nature of the triazole rings.
In the aromatic region of the spectrum, the signals for protons Hα and Hα′ are well resolved. In particular, the resonances for Hα′ on the CBPQT4+ units appear as two set of peaks, presumably as a result of the free rotation of the BIPY2+ units along the C—N bond being hindered by the hexamethylene chain. In contrast, the signals for protons Hβ and Hβ′ on the dumbbell and the cyclophane CBPQT4+, respectively, resonate at a similar frequencies, exhibiting overlapped peak signals. Protons on the hexamethylene chains were assigned unambiguously to resonances by identifying important through-bond couplings in the 1H-1H gCOSY (FIGS. 17A-17B) such as HaHb, HbHc, HcHd, HdHe and HeHf.
For compound 3R|5BP.18PF6, the 1H NMR spectrum (FIG. 18) is more complicated because the dumbbell has one more BIPY2+ subunit. Likewise, the protons of the hexamethylene chains can be assigned unambiguously to resonances by identifying important through-bond couplings in the 1H-1H gCOSY (FIGS. 19A-19B) including HaHb, HbHc, HcHd, HdHe and HeHf.
It is noteworthy that protons Hc, Hd and He of 3R|5BP.18PF6 resonate slightly upfield compared with those in 3R|4BP.16PF6, indicating that the CBPQT4+ rings are pushed farther from the BIPY2+ subunits on the dumbbell, presumably on account of the higher Coulombic repulsions as one more BIPY2+ subunit is introduced into the rod portion of the dumbbell.
The protons of the aromatic region can be assigned by recording (FIG. 20) the 1H NMR spectrum at 233 K. The integral value and the splitting pattern indicate that the α and β protons of the BIPY2+ in the CBPQT4+ rings separate into four sets of peaks, presumably as a result of the rotation of the BIPY2+ units of the CBPQT4+ rings around the hexamethylene chain is ‘frozen’ under lower temperatures. The crossed peaks correspond to proton resonances of NH4+ from NH4PF6.
HPLC and HRMS Characterizations of Oligorotaxanes 3R|4BP.16PF6 and 3R|5BP.18PF6
The HPLC traces and the HRMS spectra of 3R|4BP.16PF6 and 3R|5BP.18PF6 are shown in FIGS. 21A-21B and FIGS. 22A-22D.
Job plots of 4V4(.+)⊂2CBPQT2(.+) and 5V5(.+)⊂2CBPQT2(.+)
In order to verify the binding stoichiometry between CBPQT2(.+) and oligoviologen threads, we constructed a Job plot for 4V4(.+) and CBPQT2(.+) (FIGS. 23A-23B), as well as 5V5(.+) and CBPQT2(.+) (FIGS. 24A-24B) in MeCN.
The intensity of the trisradical complex absorption band at 1090 nm for 4V4(.+) and 1100 nm for 5V5(.+) was used for detecting the extent of binding as the molar ratio was varied. The Job plot is referenced to the concentration of CBPQT2(.+). The maximum intensity of the trisradical complex band occurred at χ=0.66, where x is the concentration of CBPQT2(.+) divided by the sum of concentration of CBPQT2(.+) and corresponding oligoviologen radical cationic species, indicating that both 4V4(.+) and 5V5(.+) bind two CBPQT2(.+) units in solution.
UV/Vis/NIR Absorption Spectrophotometric Titration of 4V4(.+) and 5V5(.+) by CBPQT2(.+)
FIGS. 25A-25B show a spectrophotometric titration of CBPQT2(.+) into a MeCN solution of 4V4(.+). This data was used to calculate a binding constant (Ka) of 3.3±0.8×109 M−2 based on the 1:2 binding model.
FIGS. 26A-26B show a spectrophotometric titration of CBPQT2(.+) into a MeCN solution of 5V5(.+). This data was used to calculate a binding constant (Ka) of 3.0±0.5×109 M−2 based on the 1:2 binding model as well. It is noteworthy that this Ka value is comparable with that of 4V4(.+), indicating their similar abilities to bind CBPQT2(.+) in MeCN. As 5V5(.+) is one viologen unit longer than 4V4(.+), the binding process is less entropically favored. Therefore, the binding enthalpy between CBPQT2(.+) and 5V5(.+) is more negative to offset the additional entropy penalty. Moreover, this Ka value is also close to the square of the binding constant4 between CBPQT2(.+) and MV.+ (7.9±5.5×104M−1), demonstrating that the strength of binding between viologen units and the CBPQT2(.+) units is retained in the case of oligoviologens.
Variable-Temperature UV/Vis/NIR Spectroscopy of 3R|4BP.16PF6
It is known that the radical-pairing interactions become weaker at higher temperature in solution. The structural information for the oligorotaxanes under reducing conditions, therefore, can be obtained by monitoring the change of the UV/Vis/NIR absorption intensities at different temperatures. Based on this knowledge, we selected 3R|4BP.16PF6 as an example on which to perform a variable-temperature UV/Vis/NIR experiment.
The spectra (FIG. 27) demonstrate that as the temperature of the solution increases, the absorption peaks centered at 550 and 1110 nm, which correspond to the formation of trisradical complex, decrease in their intensities. This observation suggests that the interactions between the CBPQT2(.+) ring and the BIPY.+ units on the dumbbell are less favored at higher temperatures. As a result, the characteristic absorption band of unpaired BIPY.+ units, i.e., the one at 604 nm, becomes more dominant at higher temperatures.
Cyclic voltammetry titration of 4V4(.+)⊂2CBPQT2(.+) and 5V5(.+)⊂2CBPQT2(.+)
In order to shed further light on the interacting mechanism between 4V4(.+) and CBPQT2(.+), a CV titration was performed.
The result (FIG. 28) shows that upon increasing the amount of CBPQT4+ from 1 equiv to 10 equiv, a reduction peak at −340 mV gradually emerges. It shifts toward the reduction potential of free CBPQT4+, indicating the saturation of binding between 4V4(.+) and CBPQT2(.+) when an excess of CBPQT4+ is added to the solution. In addition, as the equiv of CBPQT4+ increases in the solution, a peak shoulder with a potential of +37 mV can be observed, which is shifted significantly in the positive direction, indicating the existence of the radical dimer—namely, BIPY.+ pimerization—a structure generated from the one-electron oxidation of the trisradical complex between 4V4(.+) and CBPQT2(.+).
A CV titration experiment investigating (FIG. 29) the binding between 5V5(.+)⊂2CBPQT2(.+) has also been carried out. Similarly, the saturation of binding was also confirmed by the observation of the reduction peak at −320 mV. In addition, the formation of the BIPY.+ radical dimer can also be confirmed as a redox peak at +43 mV emerges upon oxidation. It is also noteworthy that this peak potential is shifted dramatically compared with that of the inclusion complex of MV.+⊂CBPQT2(.+), presumably because the BIPY.+ dimers between 4V4(.+) and 5V5(.+) with CBPQT2(.+) are more stable.
Differential Pulse Voltammetric Characterization of 3R|4BP.16PF6
In order to gain a better understanding of the electron transfer processes during the formation of the radical states of these oligorotaxanes, as well as to find out how the mechanically interlocked structure affects the recognition between BIPY.+ radicals, we selected 3R|4BP.16PF6 as an example on which to perform a differential pulse voltammetry (DPV) experiment.
The DPV profile shows (FIG. 30) three bands during the reduction process, an observation which agrees with the results from CV experiments where the reduction of 3R|4BP16+ to its radical state is complete after three steps. Comparison of the relative integrations associated with each band reveals a 1:1:2 ratio in relation to the numbers of electrons. Since a total number of eight electrons are involved during this reduction process, it can be concluded that the oligorotaxane 3R|4BP16+ receives two, followed by two, followed by four, electrons during the course of the three steps.
Redox Stimuli-Induced Contraction and Expansion of 3R|4BP.16PF6
In order to gain an understanding of the changes in the lengths of the molecules during the redox-controlled switching processes of the oligorotaxanes, we selected 3R|4BP.16PF6 as an example and performed diffusion ordered spectroscopy (DOSY) on its oxidized state (FIG. 31) and electron paramagnetic resonance (EPR) spectroscopy (FIGS. 32A-32B) on its reduced state.
The DOSY spectrum shows that the diffusion coefficient value (D) of 3R|4BP.16PF6 in CD3CN is 4.6×10−6 cm2 s−1. Given the Einstein-Stokes equation D=kT/6πηr, the radius (r) of 3R|4BP.16PF6 can be estimated as 1.4 nm. It should be noted, however, that this equation relates to spherical particles and so the DOSY can only give a rough estimation of molecular dimensions.
On the other hand, the dimension of the reduced state of 3R|4BP16+, namely 3R|4BP8(.+), was investigated (FIGS. 32A-32B) by EPR spectroscopy. 3R|4BP8(.+) in MeCN (0.2 mM) can be generated by heterogeneous 8-electron reduction of 3R|4BP16+ using freshly activated Zn dust in a N2-filled glovebox. The radical cation benzyl viologen (BnV.+) in MeCN (0.2 mM) was prepared in a similar fashion and used as a reference compound. A low sample concentration was employed in order to avoid any intermolecular interactions, and the samples were subjected to EPR measurements immediately after their preparation. The BnV.+ solution at room temperature is blue-colored and shows (FIG. 32A) the typical cw X-Band EPR spectrum of a viologen radical cation, for which the g factor is 2.0031. The hyperfine structure can be rationalized on the basis of the electron spin coupling to two equivalent N atoms and 12H atoms, which can be divided further into two pairs of two methylene protons on the benzylic groups and two equivalent sets, each of four protons, on the bipyridinium core. In contrast, the EPR signal for the purple-colored 3R|4BP8(.+) under identical experimental conditions is four-fold weaker despite the fact that it contains eight viologen units per molecule. The weak intensity is indicative of a pronounced spin-pairing effect and is in line with the intramolecular diamagnetic π-dimerization. The detected weak EPR signal can be attributed to a small thermal population of paramagnetic co-conformations.
The cw-EPR spectrum of the octaradical 3R|4BP8(.+) even in frozen MeCN at 4.1 K shows (FIG. 32B) only one unresolved resonance. No clear evidence for high multiplicity (S>½) states can be observed, thus preventing the measurement of the zero-field splitting parameter D needed for estimation of the molecular diameter.
The change in the length of the oligorotaxane 3R|4BP16+ on reduction to 3R|4BP8(.+) is supported by computational analysis. Since 3R|4BP16+ is too large to be simulated by DFT calculations, we sought an approximation by comparing the “central regions” of 3R|4BP16+ and 3R|4BP8(.+). We measured the centroid-centroid distance between the two terminal BIPY2+ units in the simulated conformation (FIG. 33A) of 4V8+ and the centroid-centroid distance between the two terminal BIPY.+ units—one on the 4V4(.+) component and the other on the distant CBPQT2(.+) ring—in the co-conformation (FIG. 33B) of the oligopseudorotaxane 4V4(.+)⊂2CBPQT2(.+). It turns out that, upon reduction, the molecular length contracts by 6 Å from 29.8 to 23.8 Å. This result confirms our conclusion that the oligorotaxanes experience expansion-contraction movements during the redox-stimulated processes.
Computational Details of Oligoviologens Folding with CBPQT2(.+)
The geometries were optimized at M06L/6-31G* level in the presence of the Poisson-Boltzmann solvation model for acetonitrile (∈=37.5 and R0=2.18 Å). Different C—C bond torsions are chosen as the initial structures to give different number of BIPY2(.+) pairs. The single point energies were refined at M06/6-311++G** level. The optimized structures reported in the FIGS. 6A-6D of the main text are provided below, with the calculated energies at each level. Units are in Hartree.
|
M06L/6-31G*
M06/6-311++G**
|
M06L/6-31G* in
in gas
in gas
Total energy
|
acetonitrile (A)
phase (B)
phase (C)
(C + A − B)
|
|
|
Co-conformation 3a
|
−6208.69096
−6206.86399
−6204.35455
−6206.18151
|
Co-conformation 3b
|
−6208.69356
−6206.99997
−6204.48428
−6206.17787
|
Co-conformation 3c
|
−6208.68304
−6206.95888
−6204.446
−6206.17016
|
Co-conformation 3d
|
−6208.68477
−6206.90408
−6204.38941
−6206.17010
|
Co-conformation 3e
|
−7013.50973
−7011.31315
−7008.47273
−7010.66930
|
Co-conformation 3f
|
−7013.48893
−7011.40759
−7008.57209
−7010.65344
|
Co-conformation 3g
|
−7013.48517
−7011.39524
−7008.55690
−7010.64683
|
Co-conformation 3h
|
−7013.47898
−7011.56174
−7008.7199
−7010.63714
|
|
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