Introduction

Target-guided synthesis (TGS) is a subset of combinatorial chemistry in which the biological target (protein or nucleic acid) is directly involved in the choice of ligands assembled from a pool of reactive building blocks1. TGS can be divided into two major classes: dynamic combinatorial chemistry and kinetic TGS2,3. In kinetic TGS, the reaction that joins the building blocks is irreversible and selectivity for some products over others is a function of differential acceleration of that reaction by the target4. One approach of kinetic TGS, in situ click chemistry, employs the completely biorthogonal [1,3]-dipolar cycloaddition reaction between azides and alkynes and has received much attention5,6. This azide-alkyne cycloaddition (AAC) reaction is rather slow in a biologically relevant environment but is accelerated when the terminal azide and alkyne groups are held together in close proximity by a given biological target. Because a large kinetic barrier must be overcome in the AAC reaction, the positive hits from in situ click chemistry could represent compounds with substantial improvements in binding ability. In past decades, in situ click chemistry has become an effective approach to discover new drug candidates, thereby leading to the discovery of numbers of agents that bind nucleic acids and proteins with strong affinity7,8,9,10,11,12,13.

G-quadruplexes are unique four-stranded nucleic acid structures formed by guanine-rich sequences in many crucial genomic regions that can be divided into three main topologies: parallel, antiparallel and hybrid-type structures14,15. During the past two decades, G-quadruplexes have attracted extensive attention because of their biological significance and potential applications in supramolecular chemistry16,17, thereby promoting the development of fluorescent probes for the selective detection of these structures18,19,20. Among them, the development of fluorescent probes for a specific G-quadruplex topology is more attractive and challenging than probes only considering the selectivity for G-quadruplexes against single- and double-stranded nucleic acids. Until now, several probes that possess the ability to distinguish different G-quadruplex topologies were reported21,22,23,24,25,26,27. However, the rational discovery of such fluorescent probes is rarely reported. Interestingly, in 2012, the in situ click chemistry approach was proven to be suitable to enhance the binding affinity of small molecules with a given G-quadruplex12. Notably, fluorescence emission of molecules upon binding to G-quadruplexes and their binding affinities were always positively correlated24,28. Taken together, these results indicate that the in situ click chemistry approach might be feasible for the development of fluorescent probes for a specific G-quadruplex topology.

Recently, we have reported a series of triarylimidazole fluorescent probes for selectively detecting G-quadruplexes24,28. Among them, IZCM-1 exhibited considerable selectivity for parallel G-quadruplexes, but subsequently, some shortcomings were observed in our studies. First, discrimination between some sequences was not selective enough. For example, the fluorescence quantum yield value of IZCM-1 for the parallel G-quadruplex c-kit2 was only approximately 3.5-fold higher than that for the antiparallel G-quadruplex HRAS. Meanwhile, the detection limits for some parallel G-quadruplexes were not satisfactory enough. To improve the sensitivity of our probe, we further developed another triarylimidazole probe, IZCM-7, for the highly sensitive detection of G-quadruplexes. Nevertheless, discrepancy of fluorescence emission of IZCM-7 between parallel and non-parallel G-quadruplexes was further reduced. Therefore, the modification strategy of triarylimidazole fluorescent probes must be reconsidered and we began to examine the possibility of developing more selective fluorescent probes for parallel G-quadruplexes using an in situ click chemistry approach. We present a procedure using in situ click chemistry to identify selective fluorescent probes for parallel G-quadruplexes. To the best of our knowledge, this is the first example of the development of selective probes for a given nucleic acid topology using an in situ click chemistry approach.

Results and Discussion

Application of in situ click chemistry to identify fluorescent probe for specific G-quadruplex topology

Based on our previous results, c-kit2 G-quadruplex DNA representing a parallel structure and HRAS G-quadruplex DNA representing a non-parallel structure were chosen as templates. A G-quadruplex binding substrate 1 containing an alkyne substituent was used as the anchor molecule. Alkyne 1 was derived from IZCM-7, but it contained only one cationic side chain attached to the chromophore, thereby leaving room to modulate the binding properties of the substrate through a click reaction with a series of azides. The KD values of 1 to c-kit2 and HRAS were determined by SPR assays as 13.9 μM and 37.9 μM, respectively (see the Supplementary Information), demonstrating that 1 could actually bind to the G-quadruplexes and act as a starting anchor molecule. Azides 2 to 8, which contain neutral, positively and negatively charged groups that cover electrostatic and hydrogen bonding interaction modes, were employed as complementary reagents for in situ click chemistry screening (Fig. 1).

Figure 1
figure 1

Structures of all the compounds in this article.

(A) Structures of IZCM-1, IZCM-7, alkyne 1 and azide building blocks 28. (B) Adducts 915 generated by treating alkyne 1 with azides 28.

The in situ click chemistry experiments were conducted using 96-well microtiter plates. Each well contained a mixture of a G-quadruplex (c-kit2 or HRAS, 12.5 μM), alkyne 1 (12.5 μM) and a given azide reagent (50.0 μM) in Tris-HCl buffer (100 mM KCl, pH = 7.2). In parallel, control experiments without G-quadruplex were performed to test for product formation as a result of background reactivity. We aimed to find a compound that is an in situ hit when using parallel c-kit2 as a template but not a hit when using antiparallel HRAS. Next, the microtiter plate was stirred at room temperature for 72 h. Subsequently, the formation of the product was monitored by UPLC using mass spectrometric detection in the positive selected ion mode (UPLC/MS). Nevertheless, a very small amount of the corresponding product in each well was detected, indicating that the AAC reaction was extremely slow even in the presence of G-quadruplex templates. According to the previous research, a CuI catalyst could accelerate such an ACC reaction and compensate for poor kinetics while preserving high selectivity12. Based on this finding, we further modified our in situ click chemistry experiments by adding CuI catalyst to the reactions (CuI used in our experiments had a slight effect on the G-quadruplex topologies, see the Supplementary Information). Afterwards, we analyzed the reaction mixtures for the generated triazoles by UPLC/MS at three different time points: 1 h, 5 h and 24 h. The results are shown in Fig. 2 (upper). The ACC reactions were greatly accelerated by CuI catalyst. Compared with the control experiments (with CuI catalyst but without G-quadruplex templates), G-quadruplex template c-kit2 actually increased the formation of most 1,4-adducts (9, 10, 12, 13 and 15) to various extents at 1 h and 5 h, while HRAS promoted the generation of compounds 9, 10, 12 and 13. We also noticed that product formation of all azides with the exception of azide 8 reached almost 100% at 24 h, thereby making it difficult to evaluate the functions of DNA templates. Besides, the conversion rate of 15 was much lower than other 1,4-adducts. Such lower conversion could be ascribed to the weaker reactivity of 3-azidopropanoic acid because we had the same findings in our further synthesis of all the individual adduct (prepared on a preparative scale using the CuI process, see the Supplementary Information). In the present in situ click chemistry experiments, control experiments without G-quadruplex were performed. Thus, various reactivity of different azides would not affect the judgment on the hits. Taking our findings together, among all the 1,4-adducts, compound 15, which resulted from the cycloaddition of 1 and 8, was distinctive because c-kit2 accelerated the reaction, but HRAS hindered product formation at each of the three time points (Fig. 2, lower), suggesting that 15 prefers to bind c-kit2 with a much lower KD than HRAS and could possibly act as a favorable fluorescent probe for parallel G-quadruplexes.

Figure 2
figure 2

Outputs of in situ click chemistry.

Upper: conversion of all 1,4-adducts obtained from each pairwise reaction with and without G-quadruplexes at (A) 1 h, (B) 5 h and (C) 24 h. Lower: chromatogram tuned on the mass channel of adduct 15 obtained from the reaction performed with and without G-quadruplexes at (D) 1 h, (E) 5 h and (F) 24 h.

To provide a rationale regarding the template effect of G-quadruplexes, we analyzed the binding affinities of starting alkyne 1 and each individual adduct (prepared on a preparative scale using the CuI process, see the Supplementary Information) to c-kit2 and HRAS by SPR experiments. As shown in Table 1, without exception, the in situ hit compounds displayed higher binding affinities for G-quadruplexes than alkyne 1. Compound 15, which was a hit in the presence of c-kit2 but not HRAS, exhibited much stronger binding affinity to c-kit2 than to HRAS (see the Supplementary Information). The greatest difference in binding affinities between c-kit2 and HRAS distinguished 15 from other adducts, causing it to be a favorable fluorescent probe for parallel G-quadruplexes. Some other adducts such as 9, 10, 12 and 13, which were all in situ hits in the presence of HRAS and c-kit2, did not display remarkable differences in the binding affinities for c-kit2 and HRAS. However, the remaining two adducts, 11 and 14, which were not hits from the in situ click chemistry approach, displayed slight enhancements in the binding affinities to c-kit2 and HRAS. These results demonstrate that compounds formed in situ were very likely to be strong G-quadruplex-interacting molecules, whereas the reverse was not true, leading to “false negatives”9. Of the eight azides, positively charged (amines) azide-derived triazoles showed the weakest discrimination between c-kit2 and HRAS, the negatively charged (carboxylic acid) azide-derived products displayed excellent discrimination between the two G-quadruplexes. The neutral triazoles (hydroxyl) possessed a medium capability to discriminate between G-quadruplexes. In general, this trend agreed with results observed in the copper-catalyzed in situ click chemistry approach.

Table 1 Summary of in situ click chemistry experiments and dissociation constants.

Simultaneously, the fluorescence quantum yields of all 1,4-adducts and alkyne 1 in the presence of c-kit2 and HRAS were detected (Table 2). As expected, the general trend of fluorescence enhancements is compatible with the affinities of the 1,4-adducts binding to G-quadruplexes. Among all the 1,4-adducts, compound 15 presented the highest selectivity between c-kit2 and HRAS. Accordingly, these results reinforced our design idea to discover a fluorescent probe specific for parallel G-quadruplexes using an in situ click chemistry approach.

Table 2 Fluorescence quantum yields of all compounds with G-quadruplexesa.

Fluorescence studies of compound 15 interactions with nucleic acids

To further determine the selectivity of compound 15 for parallel G-quadruplexes, its fluorescence properties with various G-quadruplexes and other nucleic acids were explored using a fluorescence titration assay. As shown in Fig. 3A, 15 alone in buffer displayed extremely weak emission. Upon gradual addition of c-kit2, an emission peak at approximately 525 nm appeared and was significantly enhanced. This significant increase in fluorescence was also observed when 15 was treated with the G-quadruplexes KRAS, pu22 and bcl-2, which had all been determined to form parallel structures (Fig. 3B). In contrast, we observed much weaker fluorescence enhancement for the hybrid-type G-quadruplex structures HT-L2H and htg22 and for antiparallel G-quadruplexes including HRAS, TBA and c-kit3 under experimental conditions. In addition, negligible fluorescence enhancement was observed when 15 was titrated with single-stranded DNA (Py22, A21 and T21), double-stranded DNA (ds26 and ctDNA) and triplex DNA (TAA).

Figure 3
figure 3

Fluorescence properties of 15 with different nucleic acids.

(A) The fluorescence titration of 0.5 μM compound 15 with the stepwise addition of c-kit2 (arrow: 0–5 μM) in 10 mM Tris-HCl buffer, 100 mM KCl, pH 7.2. (B) The fluorescence intensity enhancement of 0.5 μM 15 at 525 nm against the sample concentrations, λex = 450 nm.

The fluorescence quantum yield values of 15 for different nucleic acids are summarized (see the Supplementary Information). Such data were in agreement with the results of a titration experiment showing that fluorescence enhancement was always more pronounced for parallel G-quadruplexes. The quantum yield of 15 for c-kit2 reached 0.44. This value is approximately 7.5 times higher than that for HRAS. Moreover, such discrepancy was more significant than that of IZCM-1, showing that the quantum yield for c-kit2 was only 3.5-fold higher than that for HRAS24. On average, the quantum yield of 15 for parallel G-quadruplexes was 10.4 times higher than that for other types of G-quadruplexes. In contrast, the values were 8.0 and 1.3 for IZCM-1 and IZCM-7, respectively24,28.

Furthermore, competition titrations were performed to confirm the selective fluorescence response of 15 binding to parallel G-quadruplexes. As shown in Fig. 4, when gradually adding c-kit2 into the solution containing 15 and 5 μM HRAS, the enhanced fluorescence trend was similar to that observed in the experiment without HRAS. These results suggested that 15 has promising utility in the selective detection of parallel G-quadruplexes.

Figure 4
figure 4

Competitive fluorescence titrations.

Fluorescence titrations of 0.5 μM 15 with the stepwise addition of c-kit2 with and without 5 μM HRAS in 10 mM Tris-HCl buffer, 100 mM KCl, pH 7.2.

Moreover, we evaluated the detection limits of 15 for parallel G-quadruplexes. The LOD values of 15 for parallel G-quadruplexes (KRAS, pu22 and c-kit2) in solution were approximately 10 nM, which were better than those of IZCM-1 and similar to those of IZCM-7 (see the Supplementary Information), indicating 15 was a more favourable sensitive fluorescent probe compared with lead IZCM-1.

As an example of application, we set to demonstrate the potential of compound 15 as a topology-specific staining reagent for parallel G-quadruplexes in electrophoresis gels. We employed KRAS, pu22, c-kit2, htg22, HRAS, c-kit3 and ds26 in the experiments. After electrophoresis, the polyacrylamide gels were immersed in 4 μg/mL compound 15 staining solution for 20 minutes and commercial SYBR® Green I was used as a benchmark. We were only able to detect bands corresponding to parallel G-quadruplexes KRAS, pu22 and c-kit2, whereas we found no staining for hybrid-type G-quadruplex htg22, antiparallel G-quadruplex HRAS and c-kit3 and double-stranded DNA ds26. In contrast, SYBR® Green I stained all the nucleic acid bands in the same gel (see the Supplementary Information). These results further highlighted the feasibility of using 15 as a selective fluorescent stain for parallel G-quadruplexes.

Binding model of compound 15 interactions with G-quadruplexes

Modification of 2-aminopurine (2-Ap) in different loops has been widely used to estimate the binding mode of small molecules with G-quadruplexes24,29. To gain more details on the interactions of 15 with parallel G-quadruplexes, we performed fluorescence experiments using the parallel G-quadruplex c-kit2 with 2-Ap substitutions at position 4, 12 and 16. The antiparallel G-quadruplex HRAS with 2-Ap substitutions at position 7, 16 and 21 was used as well. It was found that the fluorescence intensities of Ap4, Ap12 and Ap16 in c-kit2 were significantly affected upon the addition of 15 (Fig. 5A), indicating that 15 had close contacts with these bases and probably stretched over the whole G-quartet plane of c-kit2 accordingly. In contrast, the fluorescence intensities of Ap7, Ap16 and Ap21 in HRAS were slightly affected by 15 (see the Supplementary Informations), which proved that 15 might have very weak interaction with HRAS. Such results were consistent with the SPR studies showing 15 exhibited much stronger binding affinity to c-kit2 than to HRAS. Furthermore, we also carried out these 2-Ap experiments using compound 10 that had an N-methylpiperazine side chain instead of the carboxyl side chain. As compared to 15, we observed that the fluorescence of 2-Aps in both c-kit2 (at position 4, 12 and 16) and HRAS (at position 7 and 21) were remarkably affected upon addition of 10 (see the Supplementary Information), indicating that strong interactions occurred between 10 and the two G-quadruplexes, mainly because the positive N-methylpiperazine side chain would increase electrostatic interactions with HRAS. Notably, Ap7 and Ap21 in HRAS were positioned in two lateral loop region close to the same G-quartet. The distinct responses of 2-Aps in HRAS with the addition of 10 and 15 indicated that its lateral loop would hinder 15 from stacking onto the corresponding G-quartet, probably due to electrostatic repulsion between the negatively charged carboxyl side chain on 15 and phosphate groups in loop region and thus leading to their loose interaction and the subsequent weak fluorescence response of 15 in the presence of antiparallel G-quadruplex HRAS.

Figure 5
figure 5

Studies of binding model of 15 to parallel G-quadruplex c-kit2.

(A) Plot of normalized fluorescence intensity at 375 nm of 1 μM 2-Ap individually labeled c-kit2 versus binding ratio of [15]/c-kit2], λex = 305 nm. (B) Binding model of compound 15 to parallel G-quadruplex c-kit2 (PDB ID: 2KQR).

Based on the findings of 2-Ap experiments, molecular docking studies were performed to illustrate the binding of 15 to parallel G-quadruplex c-kit2. The parallel NMR G-quadruplex structure for c-kit2 was used as the template30. Molecular model of 15 with c-kit2 was generated by docking study. As shown in Fig. 5B, compound 15 perfectly stacked on the terminal G-quartet plane of c-kit2 by a π-π interaction. The three outstretched side arms on the triarylimidazole scaffold bound to the grooves of G-quadruplex c-kit2. Notably, the carboxyl side chain stretched into the groove of c-kit2 and then interacted with the guanine base via hydrogen bond, leading to the formation of a tight complex of 15 and c-kit2. Considering the binding of 15 to antiparallel G-quadruplex HRAS, these interactions could not occur because the negatively charged carboxyl side chain would hinder 15 from stacking onto the G-quartet. Collectively, these findings offered us understandable explanation about the selectivity of 15 to parallel G-quadruplexes.

Conclusions

In summary, we have successfully employed an in situ click chemistry approach to develop a more sensitive fluorescent probe for parallel G-quadruplexes based on the triarylimidazole scaffold. Based on our results, 15 was chosen as the most promising fluorescent probe, demonstrating excellent application in the selective and sensitive detection of parallel G-quadruplexes compared with the lead compounds IZCM-1 and IZCM-7. Such selective fluorescence response can be rationalized in terms of different binding affinities between 15 and G-quadruplexes. Taken together, our findings represent a new development towards the application of in situ click chemistry to develop selective fluorescent probes and may also shed light on the search for probes for a specific G-quadruplex topology. Furthermore, this study represents an important first step that can be used in the discovery of selective probes that target a given G-quadruplex structure with an independent sequence. It should also be noted that G-quadruplexes usually interact with proteins in vivo, accordingly their 3D structures will be different from those in vitro. It is more worthy to find probes targeting these in vivo structures. Undoubtedly, a lot of work should be done to ensure the feasibility of the in situ click chemistry approach in various situations. Further investigations are now underway.

Methods

Compound synthesis

All chemicals were purchased from commercial sources unless otherwise specified. Detailed description of the synthesis of each compound can be found in the Supplementary Information. Their structure and purity were confirmed by 1H and 13C NMR spectrometry, HRMS spectrometry and HPLC analysis.

Materials

All oligonucleotides used in this study (see the Supplementary Information) were purchased from Invitrogen (China) and Sangon (China). Calf thymus DNA (ctDNA) was purchased from Sigma-Aldrich (Singapore). All the oligonucleotides and ctDNA were dissolved in relevant buffer. Their concentrations were determined from the absorbance at 260 nm, respectively on the basis of respective molar extinction coefficients using NanoDrop 1000 Spectrophotometer (Thermo Scientific, USA). To obtain G-quadruplex formation, oligonucleotides were annealed in relevant buffer containing KCl by heating to 95 °C for 5 min, followed by gradual cooling to room temperature. The oligonucleotides were engaged in G-quadruplex formation, as determined by circular dichroism (CD) measurements. Stock solutions of compounds (10 mM) were dissolved in DMSO and stored at −80 °C. Further dilutions of samples to working concentrations were made with relevant buffer immediately prior to use.

CD Studies

CD studies were performed on a Chirascan circular dichroism spectrophotometer (Applied Photophysics, UK). A quartz cuvette with a 4 mm path length was used for the recording of spectra over a wavelength range of 230–330 nm with a 1 nm bandwidth, 1 nm step size and time of 0.5 s per point. The DNA samples were set at the concentration of 10 μM.

CuI-catalyzed in situ click chemistry

5 μL of G-quadruplex DNA solution at 100 μM (c-kit2 or HRAS), or 10 mM Tris-HCl buffer (PH 7.2, 100 mM KCl), was added to a 96-well microtiter plate. Then, 5 μL of 1 (100 μM) and 1 μL of azide 28 (1 mM) were added to the mixture (each azide had a different well in the microtiter plate), followed by the addition of 0.5 μl of CuSO4·5H2O (10 mM) and 0.5 μl of aq. sodium ascorbate (10 mM). 8 μL of Tris-HCl buffer was added to fix the final solution at 20 μL. The microtiter plate was stirred at room temperature for hours before being quenched by adding 180 μL of methanol. The mixtures were then transferred to 1.5 mL Eppendorf tubes and centrifuged at 16000 rpm for 10 min at 4 °C. 10 μL of each supernatant was injected into the UPLC-MS/MS system.

UPLC-MS/MS method

The chromatography was performed on an Acquity UPLC system (Waters Corp., Milford, MA, USA) with a binary solvent manager, an autosampler (set at 4 °C) and a column oven (set at 25 °C). A BEH C18 column (2.1 × 50 mm i.d., 1.7 μm; Waters, Wexford, Ireland) preceded by a BEH C18 VanGuard ™ pre-column (2.1 × 5 mm i.d., 1.7 μm, Waters, Wexford, Ireland) was employed for the sample separation. The mobile phase composed of 90% methanol and 10% water was used in isocratic mode at a flow rate of 0.35 mL/min. The run-time was 1.5 min. The injection volume was 10 μL.

For mass spectrometry, detection and quantification of analytes were carried out on a triple quadrupole tandem mass spectrometer (Waters Quattro Premier XE, Micromass MS Technologies, Manchester, UK). The electrospray ionization (ESI) source was set in positive ionization mode. Multiple reaction monitoring mode was performed. The optimal MS parameters were as follows: capillary voltage, 3.0 kV; cone voltage, 40 V; source temperature, 120 °C. Ultrahigh-purity nitrogen and argon were used as desolvation gas (700 L/h) and collision gas (0.21 mL/min), respectively. Masslynx™ 4.1 software was used to collect and process data. The conversion of each adduct formation was determined with area normalization method.

SPR Studies

SPR measurements were performed on a ProteOn XPR36 Protein Interaction Array system (Bio-Rad Laboratories, CA) using a Streptavidin-coated GLH sensor chip. Biotinylated oligonucleotides (SPR-HRAS and SPR-c-kit2) were attached to the chip. In a typical experiment, biotinylated DNA was folded in filtered and degassed running buffer (50 mM Tris-HCl, 100 mM KCl, pH 7.2). The DNA samples were then captured (about 1000 RU) in five flow cell, leaving one flow cell as a blank. Solutions of the compounds were prepared with running buffer through serial dilutions of stock solution. Five concentrations were injected simultaneously at a flow rate of 50 μL/min for 400 s of association phase, followed with 500 s of dissociation phase at 25 °C. The GLH sensor chip was regenerated with short injection of 1 M KCl between consecutive measurements. The final graphs were obtained by subtracting blank sensorgrams from different DNA sensorgrams. Data were analyzed with ProteOn manager software, using the Langmuir model for fitting kinetic data.

UV-Vis Spectroscopic Studies

UV-Vis spectroscopic studies were performed on a UV-2450 spectrophotometer (Shimadzu, Japan) using 1 cm path length quartz cuvette. All the oligonucleotides were firstly prepared through heating at 95 °C for 5 min followed with slow cooling to room temperature. Small aliquots of a stock solution of oligonucleotide were added into the solution containing compounds at fixed concentration (1 μM) in Tris-HCl buffer (10 mM, pH 7.2) with 100 mM KCl. The final concentration of oligonucleotide was 10 μM. The intensities of absorbance at 450 nm were recorded, preparing for further determination of fluorescence quantum yields.

Fluorescence Studies

Fluorescence studies were performed on a LS-55 luminescence spectrophotometer (Perkin-Elmer, USA). A quartz cuvette with 2 mm × 10 mm path length was used for the spectra recorded at 5 nm excitation and emission slit widths unless otherwise specified.

For titration experiment, all oligonucleotides were firstly prepared through heating at 95 °C for 5 min followed with slow cooling to room temperature. Small aliquots of a stock solution of sample (oligonucleotides, ctDNA) were added into the solution containing the compounds at fixed concentration (1 μM) in Tris-HCl buffer (10 mM, pH 7.2) with 100 mM KCl. The final concentration of sample was varied from 0 to 5 μM. After each addition of sample, the reaction was stirred and allowed to equilibrate for at least 1 min and fluorescence measurement was taken at Ex 450 nm.

The fluorescence quantum yield (ΦF) of all the compounds was calculated relative to a standard solution of rhodamine 123 in ethanol (ΦF = 0.90) and was determined using the following formula: Φu = Φs (Au/As) × (Iu/Is), where Φ is the fluorescence quantum yield, I is the measured integrated emission intensity and A is the optical density (absorbance). The u refers to the compound of unknown quantum yield and s refers to the reference compound (Rohdamine 123) of known quantum yield. The fluorescence spectra were recorded at 5 nm excitation and emission slit widths for the determination of Φ.

The LOD values of 15, IZCM-1 and IZCM-7 for different nucleic acids in solution were calculated on the basis of the equation LOD = K × Sb/m. The K value is generally taken to be 3 according to the IUPAC recommendation. The Sb value represents the standard deviation for multiple measurements (n = 20) of blank solution. The m value is the slope of the calibration curve, which was derived from the linear range of a fluorescence titration curve with different nucleic acids and standards for the sensitivity of this method.

Gel Electrophoresis Studies

Different oligonucleotides were loaded onto a 20% bisacrylamide gel in 1 × TBE buffer containing 100 mM KCl and electrophoresed at 4 °C. The oligonucleotides were stained with compound 15 (4 μg/mL, 20 minutes) and then by the commercial staining agent SYBR® Green I (1×, 20 minutes). DNA fragments were visualized under UV light and photographed by using AlphaImager EC (ProteinSimple).

2-Ap Titration Experiments

Compound 15 were added into the solution containing 2-Ap-labeled oligonucleotides at fixed concentration (1 μM) in Tris-HCl buffer (10 mM, pH 7.2) with 100 mM KCl. The final concentration of 15 was varied from 0 to 10 μM. After each addition of 15, the reaction was stirred and allowed to equilibrate for at least 1 min and fluorescence measurement was taken at Ex 305 nm.

Molecular Docking Process

The structures of compound 15 were constructed and optimized with Gaussian 03 using the HF/6-31G* basis set. The parallel c-kit2-derived NMR G-quadruplex structure was used as the templates (PDB ID: 2KQR) for the docking studies. The docking simulations were performed using Schrodinger software for the binding site based on the reference compounds.

Additional Information

How to cite this article: Hu, M.-H. et al. A new application of click chemistry in situ: development of fluorescent probe for specific G-quadruplex topology. Sci. Rep. 5, 17202; doi: 10.1038/srep17202 (2015).