Covalent Protein Labeling by Enzymatic Phosphocholination

Katharina Heller; Philipp Ochtrop; Michael F. Albers; Florian B. Zauner; Aymelt Itzen; Christian Hedberg

doi:10.1002/anie.201502618

Covalent Protein Labeling by Enzymatic Phosphocholination

Katharina Heller, Philipp Ochtrop, Michael F. Albers, Florian B. Zauner, Aymelt Itzen, Christian Hedberg

Research output: Contribution to journal › Article › peer-review

36 Scopus citations

Abstract

We present a new protein labeling method based on the covalent enzymatic phosphocholination of a specific octapeptide amino acid sequence in intact proteins. The bacterial enzyme AnkX from Legionella pneumophila has been established to transfer functional phosphocholine moieties from synthetically produced CDP-choline derivatives to N-termini, C-termini, and internal loop regions in proteins of interest. Furthermore, the covalent modification can be hydrolytically removed by the action of the Legionella enzyme Lem3. Only a short peptide sequence (eight amino acids) is required for efficient protein labeling and a small linker group (PEG-phosphocholine) is introduced to attach the conjugated cargo.

Original language	English
Pages (from-to)	10327-10330
Number of pages	4
Journal	Angewandte Chemie International Edition in English
Volume	54
Issue number	35
DOIs	https://doi.org/10.1002/anie.201502618
State	Published - 1 Aug 2015
Externally published	Yes

Keywords

enzymes
nucleotides
phosphocholination
protein modifications

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10.1002/anie.201502618

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abstract = "We present a new protein labeling method based on the covalent enzymatic phosphocholination of a specific octapeptide amino acid sequence in intact proteins. The bacterial enzyme AnkX from Legionella pneumophila has been established to transfer functional phosphocholine moieties from synthetically produced CDP-choline derivatives to N-termini, C-termini, and internal loop regions in proteins of interest. Furthermore, the covalent modification can be hydrolytically removed by the action of the Legionella enzyme Lem3. Only a short peptide sequence (eight amino acids) is required for efficient protein labeling and a small linker group (PEG-phosphocholine) is introduced to attach the conjugated cargo.",

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AU - Ochtrop, Philipp

AU - Albers, Michael F.

AU - Zauner, Florian B.

AU - Itzen, Aymelt

AU - Hedberg, Christian

PY - 2015/8/1

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AB - We present a new protein labeling method based on the covalent enzymatic phosphocholination of a specific octapeptide amino acid sequence in intact proteins. The bacterial enzyme AnkX from Legionella pneumophila has been established to transfer functional phosphocholine moieties from synthetically produced CDP-choline derivatives to N-termini, C-termini, and internal loop regions in proteins of interest. Furthermore, the covalent modification can be hydrolytically removed by the action of the Legionella enzyme Lem3. Only a short peptide sequence (eight amino acids) is required for efficient protein labeling and a small linker group (PEG-phosphocholine) is introduced to attach the conjugated cargo.

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Covalent Protein Labeling by Enzymatic Phosphocholination

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