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Rapid and robust cysteine bioconjugation with vinylheteroarenes

Hikaru Seki a, Stephen J. Walsh ab, Jonathan D. Bargh a, Jeremy S. Parker c, Jason Carroll b and David R. Spring *a
aDepartment of Chemistry, University of Cambridge, Lensfield Road, Cambridge, CB2 1EW, UK. E-mail: spring@ch.cam.ac.uk
bCancer Research UK Cambridge Institute, University of Cambridge, Robinson Way, Cambridge, CB2 0RE, UK
cEarly Chemical Development, Pharmaceutical Sciences, R&D, AstraZeneca, Macclesfield, UK

Received 18th May 2021 , Accepted 28th May 2021

First published on 7th June 2021


Abstract

Methods for residue-selective and stable modification of canonical amino acids enable the installation of distinct functionality which can aid in the interrogation of biological processes or the generation of new therapeutic modalities. Herein, we report an extensive investigation of reactivity and stability profiles for a series of vinylheteroarene motifs. Studies on small molecule and protein substrates identified an optimum vinylheteroarene scaffold for selective cysteine modification. Utilisation of this lead linker to modify a number of protein substrates with various functionalities, including the synthesis of a homogeneous, stable and biologically active antibody–drug conjugate (ADC) was then achieved. The reagent was also efficient in labelling proteome-wide cysteines in cell lysates. The efficiency and selectivity of these reagents as well as the stability of the products makes them suitable for the generation of biotherapeutics or studies in chemical biology.


Introduction

The chemical modification of proteins has a crucial role in enabling the interrogation of biology and providing improved medication. However, the controlled modification of these highly complex macromolecules remains challenging. To preserve the native structure and function of meta-stable proteins, mild reaction conditions are required.1,2 Furthermore, site-selective modification is often desirable, meaning that the transformation must be chemo- and regioselective for a target residue. Despite these challenges, a toolbox of reagents has been developed for the modification of proteinogenic amino acids: lysine,3 cysteine, tryptophan,4 methionine,5,6 tyrosine,7,8 histidine9 and the N-10,11 and C-terminus12 can now be functionalised with varying levels of success.

Cysteine modification is particularly attractive due to its high nucleophilicity under biocompatible conditions, solvent accessibility, and low natural abundance. In addition to the well-established α-halo acetamides,13–15 several cysteine-modification methodologies have been reported in recent years which selectively modify cysteine residues in a range of protein substrates. These reagents include bromomaleimides,16 bromopyridazinediones,17,18 unsaturated carbonyls,19–21 vinylsulfones,22–25 vinyl-pyridines26–28 and -pyridiniums,29 and unsaturated phosphonamidates;30,31 an excellent dedicated review has been published on cysteine modification reagents.32 Despite these new developments, in the field of biotherapeutic development, maleimide reagents remain most widely used due to their remarkable conjugation efficiency.33 For instance, antibody–drug conjugates (ADCs) are an emerging class of bioconjugate therapeutics, facilitating the targeted delivery of highly toxic payloads to target cells. ADCs comprise a tumour-specific monoclonal antibody attached to a potent cytotoxic drug via an appropriate linker. Indeed, six of the nine Food and Drug Administration (FDA)-approved ADCs are synthesised via maleimide modification of cysteine residues. Despite the utility of the maleimide linker, the product thiosuccinimide linkage has demonstrated poor stability caused by de-conjugation reactions. Instability of the protein–payload linkage can greatly affect the pharmacological properties of biotherapeutics such as ADCs, given that premature release of cytotoxic payloads can decrease its targeted delivery and cause off-target toxicity.34,35 To address this, modified maleimide reagents have been developed to increase the stability of the bioconjugate.36,37 One approach involves the use of self-hydrolysing maleimides which catalyse hydrolytic opening of the thiosuccinimide ring, thus reducing its susceptibility towards E1cB-type elimination.38,39

Despite these significant advances, new methods to predictively generate stable cysteine bioconjugates are still required. We have previously reported divinylpyrimidine and divinyltriazine reagents for cysteine cross-linking.40–47 While stable and functional modification of proteins or peptides could be achieved with these reagents, they are only useful when two proximal cysteine residues are present in the protein of interest. To expand the scope and generality of this scaffold, it was envisioned that monovinylheteroarene reagents would enable efficient and selective modification of single cysteine residues, regardless of spatial arrangement.28 Herein, a comprehensive comparison of a library of monovinylheteroarenes was conducted, culminating in the selective and stable modification of numerous protein substrates (Fig. 1).


image file: d1sc02722k-f1.tif
Fig. 1 Use of maleimides, divinylpyrimidines and vinylheteroarenes for post-translational protein modification.

Results and discussion

Reactivity of vinylheteroarenes towards biological nucleophiles

It was hypothesised that variable heteroarene ring electronics would greatly affect reactivity, with increasing electron deficiency increasing the rate of cysteine addition into the vinyl group. However, increased electrophilicity may also cause increased reactivity towards other proteinogenic nucleophiles (e.g. lysine, N-terminus). It was therefore deemed imperative to measure the rate of reaction of vinylheteroarenes with differing electronic characteristics with a range of proteinogenic nucleophiles. To begin investigations, vinyl-pyridine 1, -pyrimidine 2, -triazine 3 and -tetrazine 4[thin space (1/6-em)]48,49 were synthesised from commercially available starting materials (refer to ESI); these model linkers all contain an amino functionality for further functionalisation.

Vinylheteroarenes 1, 2, 3, and 4 (10 mM) were incubated with an equimolar quantity of Boc-Cys-OMe in a mixture of sodium phosphate (NaPi, pH 8, 50 mM in D2O) and CD3OD, and the reaction progress was monitored via1H NMR spectroscopy (ESI Section 2). Kinetic analysis revealed that vinylpyrimidine 2 and vinyltriazine 3 were the most reactive, displaying second order rate constants of 0.375 M−1 s−1 and 3.10 M−1 s−1, respectively (Fig. S2 and S3). Pleasingly, >95% conversion was observed in 20 minutes for 2 and 10 minutes for 3 when 10 mM vinylheteroarene solutions were incubated with stoichiometric Boc-Cys-OMe; this represents good kinetics for bioconjugation. For comparison, traceless Staudinger ligations and strain-promoted alkyne–azide cycloadditions have rate constants of only 10−3 M−1 s−1 and 10−2 M−1 s−1, respectively, and yet are widely used for protein modification.50 With this in mind, the reaction on vinylpyrimidine and vinyltriazine scaffolds was deemed sufficiently fast for cysteine modification. In contrast, the significantly lower measured rate constant for vinylpyridine 1 (4.91 × 10−3 M−1 s−1) was considered too low to be an effective bioconjugation method (Fig. S1). Surprisingly, no reaction with the vinyl group was observed upon treatment of vinyltetrazine 4 with Boc-Cys-OMe. Instead, a second set of vinyl peaks were observed in the 1H NMR spectra (Fig. S7), suggestive of direct nucleophilic attack on the tetrazine ring – a previously documented type of reactivity.51,52 As such, vinyltetrazines were also discounted from further studies.

Further investigations were conducted using 2 as a model substrate. Vinylpyrimidine 2 reacted with Boc-Cys-OMe over a range of biologically relevant pHs, with second order rate constants of 0.510, 0.636 and 0.851 M−1 s−1 at pH 7, 6 and 5, respectively (ESI Section 2.5). Furthermore, when more dilute NaPi (pH 8; 50 mM, 25 mM or 10 mM) was used as the reaction medium, a reduction of the second order rate constants was observed (ESI Section 2.6). These data suggest that vinylhetereoarenes react with cysteines via general base catalysis.

To ascertain the selectivity of these linkers for cysteines over other protein nucleophiles, vinylheteroarenes 1, 2 and 3 were incubated with either Boc-Lys-OMe or H-Ala-NH2 (representative of the protein N-terminus) under the same conditions used in the reactions with Boc-Cys-OMe (i.e. 10 mM vinylheteroarene, 10 mM amino acid, NaPi (pH 8, 50 mM), CD3OD; refer to ESI Sections 2.3 and 2.4). Pleasingly, no reactivity was observed between vinylpyridine 1 and vinylpyrimidine 2 with Boc-Lys-OMe or H-Ala-NH2 after monitoring overnight. Gratifyingly, the minimal reactivity that was observed between vinyltriazine 3 with the N-nucleophiles translates to >3200-fold selectivity for cysteine. This represents a significant improvement versus maleimides – the state-of-the-art linker for cysteine modification – which are known to react with both cysteine and lysine residues53–55 (Table 1).

Table 1 The second order rate constants for the reaction of vinylpyridine 1, vinylpyrimidine 2, vinyltriazine 3, and vinyltetrazine 4 with Boc-Cys-OMe, Boc-Lys-OMe or H-Ala-NH2. Average of two replicates; error bars represent standard deviation of the mean

image file: d1sc02722k-u1.tif

Linker Second order rate constants (k2), ×10−3 M−1 s−1
Boc-Cys-OMe Boc-Lys-OMe H-Ala-NH2
a No reaction observed. b Significant side reaction observed.
Vinylpyridine 1 4.91 ± 0.01 0a 0a
Vinylpyrimidine 2 375 ± 30 0a 0a
Vinyltriazine 3 3100 ± 30 0.323 ± 0.006 0.944 ± 0.090
Vinyltetrazine 4 n/ab
image file: d1sc02722k-u2.tif


Stability of vinylheteroarene–thiol conjugates

Given the favourable reaction rates and cysteine selectivity observed for both vinylpyrimidine and vinyltriazine scaffolds, our attention turned towards determining the stability of the corresponding linker–cysteine conjugates. It was proposed that using a fluorinated thiol would enable the use of 19F NMR to monitor the rate of decomposition, given the quantitative nature and high sensitivity of this technique. Thus, conjugates 5, 6 and 7 were synthesised by reacting difluorobenzyl mercaptan with vinylheteroarenes 2 and 3, and N-methylmaleimide, respectively.

To measure the stability of the linker–thiol conjugates under physiologically relevant conditions, thioethers 5, 6 and 7 (15 mM) in a pH 7.4 solution were incubated with an excess of 1-thioglycerol at 37 °C (ESI Section 3). 1-Thioglycerol was added to mimic biological thiols such as glutathione or human serum albumin and would trap any reactive species formed as a result of conjugate decomposition. Analysis by 19F NMR revealed that pyrimidinyl thioether 5 and triazinyl thioether 6 were exceptionally stable over the ten-day monitoring period with <5% decomposition observed (ESI Sections 3.2 and 3.3). In contrast, the maleimide-derived conjugate 7 was unstable under these conditions, with approximately 60% starting material remaining after ten days incubation (ESI Section 3.4). These results suggest that both vinyl-pyrimidine and -triazine scaffolds have the desired stability profile required for widespread biotherapeutic development (Fig. 2).


image file: d1sc02722k-f2.tif
Fig. 2 Stability comparison of pyrimidine 5, triazine 6, and succinimide 7 in NaPi (pH 7.4, 50 mM) and CD3CN, in the presence of 1-thioglycerol (150 mM). Average of two replicates; error bars represent standard deviation of the mean.

Vinylheteroarenes for residue-specific protein labelling

Having quantitatively evaluated the reactivity and stability of the vinylheteroarene scaffolds in small molecule assays, attention turned to investigating if these favourable results could be translated onto cysteine-containing proteins. Human serum albumin (HSA) is the most abundant protein found in plasma, which has also been utilised as a biomacromolecular delivery system in protein–drug conjugates.56 Among the 35 cysteines encoded in the HSA peptide sequence, 34 are present as disulfide bonds; one cysteine (Cys34) is found unpaired. Thus, HSA was deemed to be an ideal substrate to commence protein modification investigations. Since commercially available HSA was found to be partially capped with cysteine through a disulfide bond, they were first treated with dithiothreitol (DTT) to reveal the uncapped protein (ESI Section 4.1), which was subsequently used for bioconjugation studies.

To determine the reactivity of vinylpyrimidine 2 with HSA, extensive screening of reaction conditions was carried out. Pleasingly, >95% conversion to HSA-2 was observed by LCMS analysis upon treatment of HSA with 20 equivalents of 2 at 37 °C for 2 h in a trisaminomethane buffer (Tris·HCl, pH 8, 50 mM) containing 5% DMSO (v/v; see Table S5 for optimisation). Given these encouraging results, we were eager to evaluate the generality of this methodology by modifying HSA with a range of functional moieties. Using optimised bioconjugation conditions, HSA was reacted with vinylpyrimidine reagents bearing an alkyne biorthogonal handle 8, a nitrobenzoxadiazole (NBD) fluorophore 9, and a biotin tag 10, yielding the corresponding bioconjugates HSA-8, HSA-9, HSA-10, respectively, all in >95% conversion by LCMS analysis (Fig. S37–S39).

The reactivity of vinyltriazine 3 with HSA was also investigated. After extensive screening of reaction conditions (see Table S6 for optimisation), it was found that treatment of HSA with vinyltriazine 3 (20 molar equivalents) for 1 h at 37 °C, in phosphate-buffered saline (PBS, ×1, pH 7.3) containing 5% DMSO (v/v) produced the desired bioconjugate HSA-3 with >95% conversion by LCMS analysis (Fig. S40). However, subsequent attempts to modify HSA with alkyne-bearing vinyltriazine 11 generated a mixture of unmodified, singly modified and doubly modified protein, perhaps due to reaction with another nucleophilic site, e.g. the N-terminus. These data suggest that the vinylpyrimidine scaffolds have the best combination of reactivity, selectivity and stability for general widespread use in protein modification (Fig. 3).


image file: d1sc02722k-f3.tif
Fig. 3 Modification of human serum albumin (HSA) using vinylpyrimidine and vinyltriazine linkers. The modification of HSA with a variety of functional units including alkyne reactive handle, fluorophore and biotin was successfully achieved.

Modification of cysteine-engineered antibodies and biological evaluation of antibody–drug conjugates

Encouraged by the positive properties observed for vinylpyrimidine reagents, we turned our attention towards generating a homogeneous and functional ADC using these linkers. One approach for generating ADCs uses antibodies engineered with additional surface-exposed cysteines, which allows conjugation of cytotoxic payloads to produce highly homogeneous ADCs with a defined modification site and drug-to-antibody ratio.57 Antibodies targeting the extracellular domain of the HER2 receptor tyrosine kinase have demonstrated immense clinical benefit for many years, particularly for the treatment of HER2-positive breast cancer.58 Several ADCs targeting HER2 have also undergone development with Kadcyla®59 and Enhertu®60 obtaining FDA approval. The utility of our linkers was evaluated using an anti-HER2 IgG1 antibody mAb1 which has a cysteine insertion after position 239 in each heavy chain.61 The biological activity of ADCs generated using this antibody have been demonstrated previously in vitro and in in vivo mouse xenografts.61

To modify mAb1 with a variety of payloads, this antibody was first subjected to a reduction-partial reoxidation protocol to unmask the free thiols of the inserted cysteine residues,61 whilst maintaining the intra- and inter-chain disulfides (ESI Section 5.1). Next, the partially reduced antibody was treated with 20 equivalents of vinylpyrimidine 2 (i.e. 10 equivalents per cysteine) in Tris·HCl buffer (pH 8, 50 mM) for 4 hours at 37 °C. Analysis of the reaction via LCMS revealed >95% conversion to the desired conjugate mAb1-2 (Fig. S43). Pleasingly, modification was only observed on the heavy chains, where the engineered cysteines are located. Crucially, no modification was observed on the light chains, highlighting the excellent chemoselectivity of vinylpyrimidines for cysteines. Using analogous reaction conditions, the alkyne-modified bioconjugate mAb1-8 was generated with >95% conversion by reaction of partially reduced mAb1 with vinylpyrimidine 8 (Fig. 4 and S44).


image file: d1sc02722k-f4.tif
Fig. 4 The modification of mAb1 with linker 2 and 8. The samples were deglycosylated and reduced prior to LCMS analysis.

With a reactive alkyne handle installed on mAb1, its ability to be modified with functional payloads was investigated (ESI Sections 5.4 to 5.6). First, azido-biotin 12 was reacted in the presence of CuSO4·5H2O, tris(3-hydroxypropyltriazolylmethyl)amine (THPTA) and sodium ascorbate, with LCMS analysis revealing >95% conversion to the desired conjugate mAb1-8-12 (Fig. S45). Similarly, mAb1 was reacted with Alexa Fluor 488 azide 13, yielding a fluorophore-to-antibody ratio of 1.9 via UV-vis analysis, indicating a near-complete conversion to the desired mAb1-8-13. Furthermore, sodium dodecyl sulfate-polyacrylamide gel electrophoresis (SDS-PAGE) analysis of mAb1-8-13 displayed fluorescence for the heavy chains only, demonstrating modifications to be located on the heavy chains, consistent with mass spectrometry analysis (ESI Section 5.7). The successful synthesis of mAb1-8-12 and mAb1-8-13 demonstrate that the alkyne-bearing vinylpyrimidine linker is compatible with on-protein copper-catalysed azide–alkyne cycloaddition (CuAAC) reactions.

With these promising results in hand, we proceeded to synthesise an ADC using this linker system. Thus, an appropriate azide-modified cytotoxic warhead was required. Monomethyl auristatin E (MMAE) is an anti-mitotic drug with sub-nanomolar potency, commonly used in ADC research. It was thought that incorporation of a cleavable moiety to enable release of unmodified MMAE from the antibody would achieve optimal cytotoxicity.62 We recently reported the use of sulfatase-cleavable linkers for use in MMAE-containing ADCs.42 Accordingly, MMAE-arylsulfate-azide 14 was synthesised and subsequently reacted with alkynyl antibody mAb1-8 in the presence of CuSO4·5H2O, THPTA and sodium ascorbate, with LCMS analysis revealing >95% conversion to the desired ADC mAb1-8-14 (Fig. 5 and S46).


image file: d1sc02722k-f5.tif
Fig. 5 (a) On-protein copper catalysed azide–alkyne cycloaddition (CuAAC) reactions to functionalise alkynyl antibody mAb1-8. This antibody was successfully modified with biotin 12, Alexa Fluor 488 fluorophore 13 and arylsulfate-MMAE 14. (b) Deconvoluted mass spectrum of mAb1-8-12 heavy chain. (c) Deconvoluted mass spectrum of mAb1-8-14 heavy chain. Species with 46[thin space (1/6-em)]878 Da correspond to light chain dimer. (d) UV-vis spectrum of unmodified mAb1, mAb1-8, and mAb1-8-13. Bioconjugate mAb1-8-13 displayed a fluorophore-to-antibody ratio of 1.9.

The in vitro cytotoxicity of the anti-HER2 ADC was then evaluated by incubation in HER2-positive SKBR3 cells and HER2-negative MCF7 cells (ESI Section 7). Pleasingly, potent dose-dependent cytotoxicity was observed in SKBR3 cells. This demonstrates that the vinylpyrimidine linker does not negatively affect the antibody's biological processes in terms of receptor specificity, binding or internalisation. In contrast, the ADC had little effect on the viability of the HER2-negative MCF7 cells at the concentrations tested. These in vitro studies highlight the potential of the vinylpyrimidine platform to generate clinically relevant biotherapeutics (Fig. 6).


image file: d1sc02722k-f6.tif
Fig. 6 The in vitro evaluation of ADC mAb1-8-14 in HER2-positive cells (SKBR3) and HER2-negative cells (MCF7). Viability data shows the mean of three independent experiments and error bars represent standard error of the mean.

Labelling of cysteine-containing proteins in cell lysate

With the chemoselective modification of cysteine residues validated in isolated protein and antibody systems, we wanted to explore the linker's potential to probe the presence of proteome-wide cysteine residues. Accordingly, MCF7 cell lysates (at 1 mg mL−1) were treated with varying concentrations of vinylpyrimidine probe 8 (0 to 400 μM) at rt for 2 h. The alkyne-tagged lysates were then labelled with Alexa Fluor 488 azide 13 in the presence of CuSO4·5H2O, THPTA and sodium ascorbate (ESI Section 8.2). The Alexa Fluor 488-labelled proteins were separated via SDS-PAGE followed by visualisation by in-gel fluorescence scanning, which revealed concentration-dependent labelling of lysates (Fig. 7). Crucially, when MCF7 cell lysates were pre-treated with iodoacetamide before incubating with probe 8, no labelling was observed. This further supports that vinylpyrimidine 8 react with cysteine residues with exceptional chemoselectivity. These studies demonstrate that vinylpyrimidine linkers can successfully label lysates, and offers a complementary approach to methods found in literature.63,64
image file: d1sc02722k-f7.tif
Fig. 7 SDS-PAGE analysis of MCF7 cell lysate labelling studies. Cell lysates were first labelled with varying concentrations of probe 8, and further modified with Alexa Fluor 488 azide 13via a CuAAC reaction. For cysteine blocking studies, cell lysates were first pre-incubated with iodoacetamide. (a) In-gel fluorescence of cell lysates. (b) Coomassie staining of cell lysates. All lanes were prepared under reducing conditions. Molecular weight ladder in kDa. Refer to ESI Section 8 for further details.

Plasma stability

Finally, to determine the stability of bioconjugates in human plasma, the plasma stability of the vinylpyrimidine bioconjugates was determined, and compared to those synthesised using maleimide bioconjugation. It was anticipated that the synthesis of antibody–fluorophore conjugates would enable qualitative analysis of the stability profiles of the different scaffolds using SDS-PAGE. First, the interchain disulfides of the native anti-HER2 antibody trastuzumab mAb2 were reduced with tris(2-carboxyethyl)phosphine (TCEP) hydrochloride to reveal eight reactive thiols. Then, the reduced antibody was reacted with vinylpyrimidine 8 or maleimide 15 to generate the corresponding alkynyl antibodies. Finally, the resulting alkynes were subjected to CuAAC with Alexa Fluor 488 azide 13 in the presence of CuSO4·5H2O, THPTA and sodium ascorbate, yielding antibody–fluorophore conjugates mAb2-8-13 and mAb2-15-13, with a fluorophore-antibody ratio of 6.0 and 5.8, respectively (see ESI Sections 6.2 to 6.5 for full synthetic procedure). The trastuzumab–fluorophore conjugates mAb2-8-13 and mAb2-15-13 were then incubated in human plasma at 37 °C for eight days (ESI Section 6.6). Analysis by SDS-PAGE revealed that maleimide conjugate mAb2-15-13 over time formed a new fluorescence band at ∼67 kDa. This corresponds to the product formed from linker deconjugation followed by interception with serum albumin, in accordance with previous reports.65 In contrast, no transfer of fluorescence to any of the plasma proteins was observed for the vinylpyrimidine analogue mAb2-8-13 over the eight-day monitoring period. These plasma stability data confirm the exquisite stability of vinylpyrimidine conjugates. Further stability studies were conducted in human serum, which also demonstrated the superior stability of vinylpyrimidine conjugates over maleimide conjugates (Fig. S52 and 8).
image file: d1sc02722k-f8.tif
Fig. 8 Determination of plasma stability by SDS-PAGE for (a) mAb2-8-13 and (b) mAb2-15-13, which are bioconjugates synthesised by reduction of interchain disulfides of native trastuzumab mAb2, followed by bioconjugation with linker 8 or 15, respectively, and functionalisation with Alexa Fluor 488 13. In-gel fluorescence analysis displays no transfer of fluorescence for vinylpyrimidine-derived conjugate mAb2-8-13. In contrast, fluorescence transfer to serum proteins (indicated by the beige box) was observed for maleimide-derived mAb2-15-13. All lanes were prepared under reducing conditions. (c) UV-vis spectra for mAb2, mAb2-8-13, and mAb2-15-13.

Conclusion

In this work, a series of vinylheteroarene scaffolds were explored for cysteine modification. Through several small molecule reactivity, chemoselectivity and stability assays, vinylpyrimidine reagents emerged as the most promising candidates for selective modification of proteinogenic cysteine residues. Vinylpyrimidine reagents demonstrated rapid reactivity and chemoselectivity towards cysteines, and the resulting conjugates were exceptionally stable under physiologically relevant conditions. These reagents were then elaborated to modify cysteine residues in protein substrates, culminating in the synthesis of a homogeneous ADC. Biological assays revealed the modified proteins retain their biological function, demonstrated by cell-specific cytotoxicity. Utilising the linker's cysteine selective reactivity, the linkers were used as a probe for proteinogenic cysteine residues in cell lysates. Finally, the bioconjugates exhibited superior stability in human plasma compared to the widely used maleimide reagents. The advantageous properties and synthetic accessibility of the vinylheteroarene scaffold lends itself toward widespread usage, both in the development of biological probes and next generation biotherapeutics.

Author contributions

Research was conceived by all authors. Experiments were designed and performed by HS and SJW. Cell lysate preparation and in vitro cytotoxicity studies were conducted by SJW and JSC. Compound 14 was prepared by JDB. Antibodies used in this study were provided by JSP. The manuscript was written and proofread by all authors.

Conflicts of interest

There are no conflicts to declare.

Acknowledgements

We are grateful for assistance from Duncan J. Howe and Andrew Mason for analytical support; Andrew J. Counsell for assistance with chemical synthesis and for helpful discussions; and Danya Cheeseman for assistance with cell lysate preparation. H. S. thanks Trinity College Cambridge for a studentship. J. D. B. acknowledges an iCASE studentship from GlaxoSmithKline/EPSRC. D. R. S. acknowledges support from the EPSRC (EP/P020291/1) and Royal Society (Wolfson Research Merit Award). The Spring Laboratory acknowledges support from the EPSRC, BBSRC, MRC and Royal Society.

References

  1. E. A. Hoyt, P. M. S. D. Cal, B. L. Oliveira and G. J. L. Bernardes, Nat. Rev. Chem., 2019, 3, 147 Search PubMed.
  2. T. Tamura and I. Hamachi, J. Am. Chem. Soc., 2019, 141, 2782 Search PubMed.
  3. M. J. Matos, B. L. Oliveira, N. Martínez-Sáez, A. Guerreiro, P. M. S. D. Cal, J. Bertoldo, M. Maneiro, E. Perkins, J. Howard and M. J. Deery, et al. , J. Am. Chem. Soc., 2018, 140, 4004 Search PubMed.
  4. Y. Seki, T. Ishiyama, D. Sasaki, J. Abe, Y. Sohma, K. Oisaki and M. Kanai, J. Am. Chem. Soc., 2016, 138, 10798 Search PubMed.
  5. S. Lin, X. Yang, S. Jia, A. M. Weeks, M. Hornsby, P. S. Lee, R. V. Nichiporuk, A. T. Iavarone, J. A. Wells and F. D. Toste, et al. , Science, 2017, 355, 597 Search PubMed.
  6. M. T. Taylor, J. E. Nelson, M. G. Suero and M. J. Gaunt, Nature, 2018, 562, 563 Search PubMed.
  7. H. Ban, J. Gavrilyuk and C. F. Barbas, J. Am. Chem. Soc., 2010, 132, 1523 Search PubMed.
  8. S. Sato, K. Nakamura and H. Nakamura, ACS Chem. Biol., 2015, 10, 2633 Search PubMed.
  9. S. Jia, D. He and C. J. Chang, J. Am. Chem. Soc., 2019, 141, 7294 Search PubMed.
  10. J. I. Macdonald, H. K. Munch, T. Moore and M. B. Francis, Nat. Chem. Biol., 2015, 11, 326 Search PubMed.
  11. D. Chen, M. M. Disotuar, X. Xiong, Y. Wang and D. H. C. Chou, Chem. Sci., 2017, 8, 2717 Search PubMed.
  12. S. Bloom, C. Liu, D. K. Kölmel, J. X. Qiao, Y. Zhang, M. A. Poss, W. R. Ewing and D. W. C. Macmillan, Nat. Chem., 2018, 10, 205 Search PubMed.
  13. G. C. Kemp, A. C. Tiberghien, N. V. Patel, F. D'Hooge, S. M. Nilapwar, L. R. Adams, S. Corbett, D. G. Williams, J. A. Hartley and P. W. Howard, Bioorg. Med. Chem. Lett., 2017, 27, 1154 Search PubMed.
  14. S. C. Alley, D. R. Benjamin, S. C. Jeffrey, N. M. Okeley, D. L. Meyer, R. J. Sanderson and P. D. Senter, Bioconjugate Chem., 2008, 19, 759 Search PubMed.
  15. S. Puthenveetil, F. Loganzo, H. He, K. Dirico, M. Green, J. Teske, S. Musto, T. Clark, B. Rago and F. Koehn, et al. , Bioconjugate Chem., 2016, 27, 1880 Search PubMed.
  16. M. E. B. Smith, F. F. Schumacher, C. P. Ryan, L. M. Tedaldi, D. Papaioannou, G. Waksman, S. Caddick and J. R. Baker, J. Am. Chem. Soc., 2010, 132, 1960 Search PubMed.
  17. V. Chudasama, M. E. B. Smith, F. F. Schumacher, D. Papaioannou, G. Waksman, J. R. Baker and S. Caddick, Chem. Commun., 2011, 47, 8781 Search PubMed.
  18. A. Maruani, M. E. B. Smith, E. Miranda, K. A. Chester, V. Chudasama and S. Caddick, Nat. Commun., 2015, 6, 1 Search PubMed.
  19. B. Bernardim, P. M. S. D. Cal, M. J. Matos, B. L. Oliveira, N. Martínez-Saéz, I. S. Albuquerque, E. Perkins, F. Corzana, A. C. B. Burtoloso and G. Jiménez-Osés, et al. , Nat. Commun., 2016, 7, 13128 Search PubMed.
  20. Y. Zhang, X. Zhou, Y. Xie, M. M. Greenberg, Z. Xi and C. Zhou, J. Am. Chem. Soc., 2017, 139, 6146 Search PubMed.
  21. J. Yu, X. Yang, Y. Sun and Z. Yin, Angew. Chem., Int. Ed., 2018, 57, 11598 Search PubMed.
  22. J. Morales-Sanfrutos, J. Lopez-Jaramillo, M. Ortega-Muñoz, A. Megia-Fernandez, F. Perez-Balderas, F. Hernandez-Mateo and F. Santoyo-Gonzalez, Org. Biomol. Chem., 2010, 8, 667 Search PubMed.
  23. J. Morales-Sanfrutos, F. J. Lopez-Jaramillo, F. Hernandez-Mateo and F. Santoyo-Gonzalez, J. Org. Chem., 2010, 75, 4039 Search PubMed.
  24. E. Gil de Montes, E. Jiménez-Moreno, B. L. Oliveira, C. D. Navo, P. M. S. D. Cal, G. Jiménez-Osés, I. Robina, A. J. Moreno-Vargas and G. J. L. Bernardes, Chem. Sci., 2019, 10, 4515 Search PubMed.
  25. E. Gil de Montes, A. Istrate, C. D. Navo, E. Jiménez-Moreno, E. A. Hoyt, F. Corzana, I. Robina, G. Jiménez-Osés, A. J. Moreno-Vargas and G. J. L. Bernardes, Angew. Chem., Int. Ed., 2020, 132, 6255 Search PubMed.
  26. A. G. Watts, T. Kantner and A. B. Mackenzie, WO2010/070300, 2010.
  27. A. D. Baxter, C. M. Birchall, D. J. Mansell, J. H. Mysliwy and J. Thirlway, WO2016/067021, 2016.
  28. R. Sebastiano, A. Citterio, M. Lapadula and P. G. Righetti, Rapid Commun. Mass Spectrom., 2003, 17, 2380 Search PubMed.
  29. M. J. Matos, C. D. Navo, T. Hakala, X. Ferhati, A. Guerreiro, D. Hartmann, B. Bernardim, K. L. Saar, I. Compañón and F. Corzana, et al. , Angew. Chem., Int. Ed., 2019, 58, 6640 Search PubMed.
  30. M. Kasper, M. Glanz, A. Stengl, M. Penkert, S. Klenk, T. Sauer, D. Schumacher, J. Helma, E. Krause and M. C. Cardoso, et al. , Angew. Chem., Int. Ed., 2019, 58, 11625 Search PubMed.
  31. M. A. Kasper, A. Stengl, P. Ochtrop, M. Gerlach, T. Stoschek, D. Schumacher, J. Helma, M. Penkert, E. Krause and H. Leonhardt, et al. , Angew. Chem., Int. Ed., 2019, 58, 11631 Search PubMed.
  32. P. Ochtrop and C. P. R. Hackenberger, Curr. Opin. Chem. Biol., 2020, 58, 28 Search PubMed.
  33. S. J. Walsh, J. D. Bargh, F. M. Dannheim, A. R. Hanby, H. Seki, A. J. Counsell, X. Ou, E. Fowler, N. Ashman and Y. Takada, et al. , Chem. Soc. Rev., 2021, 50, 1305 Search PubMed.
  34. B. Q. Shen, K. Xu, L. Liu, H. Raab, S. Bhakta, M. Kenrick, K. L. Parsons-Reponte, J. Tien, S. F. Yu and E. Mai, et al. , Nat. Biotechnol., 2012, 30, 184 Search PubMed.
  35. L. N. Tumey, M. Charati, T. He, E. Sousa, D. Ma, X. Han, T. Clark, J. Casavant, F. Loganzo and F. Barletta, et al. , Bioconjugate Chem., 2014, 25, 1871 Search PubMed.
  36. P. A. Szijj, C. Bahou and V. Chudasama, Drug Discovery Today: Technol., 2018, 30, 27 Search PubMed.
  37. J. M. J. M. Ravasco, H. Faustino, A. Trindade and P. M. P. Gois, Chem.–Eur. J., 2019, 25, 43 Search PubMed.
  38. R. P. Lyon, J. R. Setter, T. D. Bovee, S. O. Doronina, J. H. Hunter, M. E. Anderson, C. L. Balasubramanian, S. M. Duniho, C. I. Leiske and F. Li, et al. , Nat. Biotechnol., 2014, 32, 1059 Search PubMed.
  39. R. J. Christie, R. Fleming, B. Bezabeh, R. Woods, S. Mao, J. Harper, A. Joseph, Q. Wang, Z. Q. Xu and H. Wu, et al. , J. Controlled Release, 2015, 220, 660 Search PubMed.
  40. S. J. Walsh, S. Omarjee, W. R. J. D. Galloway, T. T.-L. Kwan, H. F. Sore, J. S. Parker, M. Hyvönen, J. S. Carroll and D. R. Spring, Chem. Sci., 2019, 10, 694 Search PubMed.
  41. N. S. Robertson, S. J. Walsh, E. Fowler, M. Yoshida, S. Rowe, Y. Wu, H. Sore, J. Parker and D. R. Spring, Chem. Commun., 2019, 55, 9499 Search PubMed.
  42. J. D. Bargh, S. J. Walsh, A. Isidro-Llobet, S. Omarjee, J. S. Carroll and D. R. Spring, Chem. Sci., 2020, 11, 2375 Search PubMed.
  43. S. J. Walsh, J. Iegre, H. Seki, J. D. Bargh, H. F. Sore, J. S. Parker, J. S. Carroll and D. R. Spring, Org. Biomol. Chem., 2020, 18, 4224 Search PubMed.
  44. A. J. Counsell, S. J. Walsh, N. S. Robertson, H. F. Sore and D. R. Spring, Org. Biomol. Chem., 2020, 18, 4739 Search PubMed.
  45. J. Charoenpattarapreeda, S. J. Walsh, J. S. Carroll and D. R. Spring, Angew. Chem., Int. Ed., 2020, 59, 23045 Search PubMed.
  46. J. D. Bargh, S. J. Walsh, N. Ashman, A. Isidro-Llobet, J. S. Carroll and D. R. Spring, Chem. Commun., 2021, 57, 3457 Search PubMed.
  47. J. S. Parker, H. F. Sore, D. R. Spring and S. J. Walsh, WO 2020/025108, 2020.
  48. Z. Novák, B. Bostai, M. Csékei, K. Lőrincz and A. Kotschy, Heterocycles, 2003, 60, 2653 Search PubMed.
  49. A. M. Bender, T. C. Chopko, T. M. Bridges and C. W. Lindsley, Org. Lett., 2017, 19, 5693 Search PubMed.
  50. K. Lang and J. W. Chin, ACS Chem. Biol., 2014, 9, 16 Search PubMed.
  51. D. N. Kamber, Y. Liang, R. J. Blizzard, F. Liu, R. A. Mehl, K. N. Houk and J. A. Prescher, J. Am. Chem. Soc., 2015, 137, 8388 Search PubMed.
  52. B. J. Umlauf, K. A. Mix, V. A. Grosskopf, R. T. Raines and E. V. Shusta, Bioconjugate Chem., 2018, 29, 1605 Search PubMed.
  53. C. F. Brewer and J. P. Riehm, Anal. Biochem., 1967, 18, 248 Search PubMed.
  54. M. A. Kasper, M. Glanz, A. Stengl, M. Penkert, S. Klenk, T. Sauer, D. Schumacher, J. Helma, E. Krause and M. C. Cardoso, et al. , Angew. Chem., Int. Ed., 2019, 58, 11625 Search PubMed.
  55. J. Václavík, R. Zschoche, I. Klimánková, V. Matoušek, P. Beier, D. Hilvert and A. Togni, Chem.–Eur. J., 2017, 23, 6490 Search PubMed.
  56. A. Wall, K. Nicholls, M. B. Caspersen, S. Skrivergaard, K. A. Howard, K. Karu, V. Chudasama and J. R. Baker, Org. Biomol. Chem., 2019, 17, 7870 Search PubMed.
  57. J. R. Junutula, H. Raab, S. Clark, S. Bhakta, D. D. Leipold, S. Weir, Y. Chen, M. Simpson, S. P. Tsai and M. S. Dennis, et al. , Nat. Biotechnol., 2008, 26, 925 Search PubMed.
  58. K. McKeage and C. M. Perry, Drugs, 2002, 209–243 Search PubMed.
  59. A. Ballantyne and S. Dhillon, Drugs, 2013, 73, 755 Search PubMed.
  60. S. J. Keam, Drugs, 2020, 501–508 Search PubMed.
  61. N. Dimasi, R. Fleming, H. Zhong, B. Bezabeh, K. Kinneer, R. J. Christie, C. Fazenbaker, H. Wu and C. Gao, Mol. Pharm., 2017, 14, 1501 Search PubMed.
  62. J. D. Bargh, A. Isidro-Llobet, J. S. Parker and D. R. Spring, Chem. Soc. Rev., 2019, 48, 4361 Search PubMed.
  63. B. K. Hansen, C. J. Loveridge, S. Thyssen, G. J. Wørmer, A. D. Nielsen, J. Palmfeldt, M. Johannsen and T. B. Poulsen, Angew. Chem., Int. Ed., 2019, 58, 3533 Search PubMed.
  64. B. Bernardim, L. Dunsmore, H. Li, B. Hocking, R. Nuñez-Franco, C. D. Navo, G. Jiménez-Osés, A. C. B. Burtoloso, G. J. L. Bernardes and G. J. L. Bernardes, Bioconjugate Chem., 2020, 31, 1604 Search PubMed.
  65. S. Kolodych, O. Koniev, Z. Baatarkhuu, J. Y. Bonnefoy, F. Debaene, S. Cianférani, A. Van Dorsselaer and A. Wagner, Bioconjugate Chem., 2015, 26, 197 Search PubMed.

Footnote

Electronic supplementary information (ESI) available. See DOI: 10.1039/d1sc02722k

This journal is © The Royal Society of Chemistry 2021