<i>ortho</i>-Methoxyphenols as Convenient Oxidative Bioconjugation Reagents with Application to Site-Selective Heterobifunctional Cross-Linkers

ElSohly, Adel M.; MacDonald, John L.; Hentzen, Nina B.; Aanei, Ioana L.; Muslemany, Kareem M. El; Francis, Matthew B.

doi:10.1021/jacs.6b12966

Cited by 30 publications

(38 citation statements)

References 39 publications

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“…It is therefore likely that N‐terminal modification will not affect the inherent function of wild‐type proteins or enzymes in most cases . Since an N‐terminal α‐amino group has a lower p K a value than the ϵ‐amino group of the Lys side chain, a reagent targeting the N‐terminal amino acid is expected to be particularly effective for modification of this site . For example, Francis and co‐workers, and other researchers have reported a site‐specific and one‐step N‐terminal α‐amino group modification Scheme using 2‐pyridinecarbaldehyde derivatives …”

Section: Figurementioning

confidence: 99%

“…In biological systems, pyridoxal phosphate is an important cofactor which is involved in post‐translational modification of an amino group in peptides and proteins . Specific N‐terminal modification of a protein with 2‐pyridylcarbaldehyde, a nitrogen‐containing heteroaromatic compound with a formyl group which is similar to the pyridoxal phosphate cofactor, was reported to proceed via formation of a 4‐imidazolidinone ring involving two nitrogen atoms of the N terminus and adjacent residues . On the basis of this knowledge, we began our investigation by examining a series of five‐membered nitrogen‐containing heteroaromatic aldehydes as N‐terminal specific modification reagents.…”

Section: Figurementioning

confidence: 99%

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Triazolecarbaldehyde Reagents for One‐Step N‐Terminal Protein Modification

et al. 2020

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Site-specific modification of peptides and proteins is ak ey aspect of protein engineering.W ed eveloped am ethod for modification of the Nterminus of proteins using 1H-1,2,3-triazole-4-carbaldehyde( TA4C) derivatives, which can be prepared in one step. The N-terminal specific labelingo fb ioactive peptides and proteins with the TA4C derivatives proceeds under mild reactionc onditions in excellent conversion (angiotensinI: 92 %, ribonuclease A: 90 %). This method enables site-specific conjugation of various functional molecules such as fluorophores,b iotin, and polyethylene glycol attached to the triazole ring to the Nterminus. Furthermore, af unctional molecule modified with ap rimary amine moiety can be directly converted into aT A4C derivativethrough aDimroth rearrangement reaction with 1-(4-nitrophenyl)-1H-1,2,3-triazole-4-carbaldehyde. This methodc an be used to obtain N-terminal-modifiedp roteins via only two steps:1 )convenient preparation of aT A4C derivativew ith af unctional group and 2) modification of the Nterminus of the protein with the TA4C derivative.

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Section: Figurementioning

confidence: 99%

Section: Figurementioning

confidence: 99%

Triazolecarbaldehyde Reagents for One‐Step N‐Terminal Protein Modification

et al. 2020

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“…In a recent example, we introduced an aniline reactive handle to allow selective modification by oxidative coupling with an o ‐aminophenol modified label . The oxidative coupling was developed by Francis and co‐workers and uses oxidized o ‐aminophenols or o ‐methoxyphenols for coupling with anilines …”

Section: Label‐containing Moietymentioning

confidence: 99%

Considerations on Probe Design for Affinity‐Guided Protein Conjugation

2019

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The plethora of methods developed for the creation of protein conjugates often differs significantly with regard to the heterogeneity of the resulting products, in the degree of genetic manipulation of the protein required, and in the technical skills required to perform the conjugation procedure. Affinity‐guided protein conjugation is a protein labeling methodology based on noncovalent binding interactions between a labeling probe and the protein of interest. These interactions increase the local concentration of a reactive group in the probe on the protein surface thus facilitating the conjugation in proximity of the complexation site. The ability to produce high‐quality conjugates from nongenetically modified proteins both in vitro, but also in cells, demonstrates the power of affinity‐guided protein conjugation. Here, we present the progress of affinity‐guided protein conjugation in relation to selective protein labeling in living systems and the formation of high‐quality protein conjugates. Furthermore, the probe design will be discussed in relation to the utility of the probe for labeling in vitro or in living systems.

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“…[46] To explore different medicala nd biotechnological applications,b iomolecules( such as peptides, DNA,a nd antibodies) as well as small molecules (dyes, radioisotopes, MRI contrast agents, drugs)w ere coupled in ap recise mannert op roteins of interest. [47] Tilman Hackeng (CardiovascularR esearch Institute Maastricht/Maastricht University,T he Netherlands) discussed recent applicationso fo xime ligation reactions to probe functional heteromeric chemokinep rotein-protein interactions. [48] He furthermorer eporteda no xime ligationr eaction that can be accelerated under aqueous conditions, at low concentrationsa nd at neutral pH by freezing.…”

Section: Protein Synthesis Beyond the Ribosome: Advances In Chemical mentioning

confidence: 99%