Engineered botulinum neurotoxin B with improved efficacy for targeting human receptors

Tao, Liang; Peng, Lisheng; Berntsson, R.P.-A.; Liu, Sai Man; Park, Sunhyun; Yu, Feifan; Boone, Christopher D.; Palan, Shilpa; Beard, Matthew; Chabrier, Pierre‐Etienne; Stenmark, Pål; Krupp, Johannes; Dong, Min

doi:10.1038/s41467-017-00064-y

Cited by 58 publications

(67 citation statements)

References 53 publications

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“…31,32 BoNT serotype B, the only alternative to A used currently in the clinic, displays lower efficacy in humans due to a mutation in the synaptotagmin 2 receptor which results in its poor affinity at this receptor. 33 Here, B1 was highly potent in mice both in the PNHD and in vivo models, consistent with previously reported data for this species in in vitro and ex vivo assays. 34 In rats, B1 was the least potent serotype in vivo as well as in the SCN assay when evaluating VAMP1 cleavage, in agreement with reports of VAMP1 being relatively resistant to cleavage by serotype B 35 BoNT serotypes C, E, and F have been used in humans in a small number of case studies.…”

Section: Discussionsupporting

confidence: 91%

“…BoNT serotype B, the only alternative to A used currently in the clinic, displays lower efficacy in humans due to a mutation in the synaptotagmin 2 receptor which results in its poor affinity at this receptor . Here, B1 was highly potent in mice both in the PNHD and in vivo models, consistent with previously reported data for this species in in vitro and ex vivo assays .…”

Section: Discussionsupporting

confidence: 89%

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A comparison of biological activity of commercially available purified native botulinum neurotoxin serotypes A1 to F1 in vitro, ex vivo, and in vivo

Donald

Elliott

Gray

et al. 2018

Pharmacology Res & Perspec

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Botulinum neurotoxin (BoNT) is a major therapeutic agent. Of seven native BoNT serotypes (A to G), only A and B are currently used in the clinic. Here we compared the potency of commercially available purified native serotypes A1 to F1 across in vitro, ex vivo, and in vivo assays. BoNT potency in vitro was assessed in rat primary cells (target protein cleavage and neurotransmitter release assays) in supraspinal, spinal, and sensory systems. BoNT potency ex vivo was measured in the mouse phrenic nerve hemidiaphragm (PNHD) assay, measuring muscle contractility. In vivo, BoNT‐induced muscle relaxation in mice and rats was assessed in the Digit Abduction Score (DAS) test, while effects on body weight (BW) gain were used to assess tolerability. In all assays, all BoNT serotypes were potent toxins, except serotype D1 in vivo which failed to produce significant muscle flaccidity in mice and rats. In rats, all serotypes were well‐tolerated, whereas in mice, reductions in BW were detected at high doses. Serotype A1 was the most potent serotype across in vitro, ex vivo, and in vivo assays. The rank order of potency of the serotypes revealed differences among assays. For example, species‐specificity was seen for serotype B1, and to a lesser extent for serotype C1. Serotypes F1 and C1, not currently in the clinic, showed preference for sensory over motor models and therefore could be considered for development in conditions involving the somatosensory system.

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Section: Discussionsupporting

confidence: 91%

Section: Discussionsupporting

confidence: 89%

A comparison of biological activity of commercially available purified native botulinum neurotoxin serotypes A1 to F1 in vitro, ex vivo, and in vivo

Donald

Elliott

Gray

et al. 2018

Pharmacology Res & Perspec

Self Cite

View full text Add to dashboard Cite

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“…This is usually achieved in two ways: 1) discretizing phonon spectrum by utilizing nanodiamond with a size smaller than half of phonon wavelength, similar to the idea of suppressing spontaneous emission from atoms by employing a nanocavity; [145] 2) creating a phononic bandgap by fabricating a periodic nanostructure on diamond, [80,140,141,146] which becomes possible thanks to the recent advance in diamond nanofabrications. [147,148] Up till now, these techniques have not been applied to split-vacancy centers yet, but the second approach of strain engineering has made some progress on both SiV − [72,143] and GeV − [144] systems.…”

Section: Spin Control Of Single XV − Color Centermentioning

confidence: 99%

Building Blocks for Quantum Network Based on Group‐IV Split‐Vacancy Centers in Diamond

2019

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One ultimate goal of quantum information processing is to construct a quantum network for direct sharing of quantum information between distant parties based on stationary qubits for information storage and flying qubits for information transmission. This requires long‐lived quantum memories, efficient light–matter interface, and deterministic quantum gate operations. Among matter qubits, the electron spin of nitrogen vacancy center in diamond is an appealing option for its long coherence time at room temperature, deterministic microwave control, and optical preparation and readout of the qubit. However, its poor optical properties, including weak zero‐phonon‐line emission and large spectral diffusion, limit its potential for large‐scale deployment in quantum nodes. This has motivated the investigation for alternative quantum emitters that combine long‐time memory and coherent optical properties together. The emerging group‐IV split‐vacancy color centers in diamond, such as silicon‐vacancy, germanium‐vacancy, tin‐vacancy, and lead‐vacancy centers, are promising candidates of this ongoing exploration. These quantum emitters simultaneously possess microsecond spin coherence time and optically bright transitions with narrow linewidths. This review reports recent efforts on extending the spin coherence time of these color centers via temperature, strain, and charge control, which paves the road towards constructing solid‐based matter–photon interface for quantum network applications.

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“…For the LFN-LC/A C699S construct, the N terminal domain of LF (residues 1 -262 of native LF) and the catalytic domain of Botulinum neurotoxin type A1 (BoNT/A1) (residues 1 -448 of native BoNT/A1) separated by a (GGS)2 linker was codon-optimized and cloned into the pK8 expression vector with a cleavable C-terminal His-tag. This was expressed in E .coli strain NiCo21 (DE3) using conditions previously described (96) and purified by IMAC using NiHP (GE Healthcare Life Sciences) and AEC using QHP (GE Healthcare Life Sciences) columns. The Histag was removed by O/N incubation with TEV protease (Millipore Sigma) at 4 °C followed by negative INAC, and the final product was desalted into PBS pH 7.2 and stored at -80 °C.…”

Section: Recombinant Protein Expression and Purificationmentioning

confidence: 99%

Anthrax Toxin as a Molecular Platform to Target Nociceptive Neurons and Modulate Pain

Yang

Isensee

Neel

et al. 2020

Preprint

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ANTXR2 expression on nociceptive neurons allows selective targeting and modulation of pain by native and engineered anthrax toxins. ABSTRACTBacterial toxins are able to act on neurons to modulate signaling and function. Here, we find that nociceptive sensory neurons that mediate pain are enriched in the receptor for anthrax toxins, ANTXR2. Anthrax Edema Toxin (ET) induced cAMP and PKA signaling in Nav1.8 + nociceptive neurons and modulated pain in vivo. Peripherally administered ET mediated mechanical allodynia in naïve mice and during B. anthracis infection. Intrathecally administered ET produced analgesic effects, potently blocking pain-like behaviors in multiple mouse models of inflammatory and chronic neuropathic pain. Nociceptor-specific ablation of ANTXR2 attenuated ET-induced signaling and analgesia. Modified anthrax toxin successfully delivered exogenous protein cargo into nociceptive neurons, illustrating utility of the anthrax toxin system as a molecular platform to target pain. ET further induced signaling in human iPSC-derived sensory neurons. Our findings highlight novel interactions between a bacterial toxin and nociceptors that may be utilized for developing new pain therapeutics.

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Engineered botulinum neurotoxin B with improved efficacy for targeting human receptors

Cited by 58 publications

References 53 publications

A comparison of biological activity of commercially available purified native botulinum neurotoxin serotypes A1 to F1 in vitro, ex vivo, and in vivo

A comparison of biological activity of commercially available purified native botulinum neurotoxin serotypes A1 to F1 in vitro, ex vivo, and in vivo

Building Blocks for Quantum Network Based on Group‐IV Split‐Vacancy Centers in Diamond

Anthrax Toxin as a Molecular Platform to Target Nociceptive Neurons and Modulate Pain

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