Further assessments of ligase LplA-mediated modifications of proteins in vitro and in cellulo

Alicia Schirer; Anne Rouch; Estelle Marcheteau; Johann Stojko; Sophie Landron; Elodie Jeantet; Benjamin Fould; Gilles Ferry; Jean A Boutin

doi:10.1007/s11033-021-06853-5

Further assessments of ligase LplA-mediated modifications of proteins in vitro and in cellulo

Mol Biol Rep. 2022 Jan;49(1):149-161. doi: 10.1007/s11033-021-06853-5. Epub 2021 Oct 31.

Authors

Alicia Schirer^{1

2}, Anne Rouch¹, Estelle Marcheteau¹, Johann Stojko¹, Sophie Landron¹, Elodie Jeantet¹, Benjamin Fould¹, Gilles Ferry¹, Jean A Boutin^{3

4

5}

Affiliations

¹ PEX Biotechnologie, Chimie, Biologie, Institut de Recherches Servier, 125 Chemin de Ronde, 78290, Croissy-sur-Seine, France.
² , Techno Parc de Thudinie 2, 6536, Thuin, Belgium.
³ PEX Biotechnologie, Chimie, Biologie, Institut de Recherches Servier, 125 Chemin de Ronde, 78290, Croissy-sur-Seine, France. ja.boutin.pro@gmail.com.
⁴ Institut de Recherches Internationales Servier, 50 rue Carnot, 92284, Suresnes, France. ja.boutin.pro@gmail.com.
⁵ Faculté de Pharmacie, PHARMADEV (Pharmacochimie et Biologie Pour le Développement), Université Toulouse 3 Paul Sabatier, 35 chemin des maraîchers, 31062, Toulouse Cedex 9, France. ja.boutin.pro@gmail.com.

PMID: 34718939
DOI: 10.1007/s11033-021-06853-5

Abstract

Background: Posttranslational modifications of proteins are catalyzed by a large family of enzymes catalyzing many chemical modifications. One can hijack the natural use of those enzymes to modify targeted proteins with synthetic chemical moieties. The lipoic acid ligase LplA mutants can be used to introduce onto the lysine sidechain lipoic acid moiety synthetic analogues. Substrate protein candidates of the ligase must obey a few a priori rules.

Methods and results: In the present report, we technically detailed the use of a cell line stably expressing both the ligase and a model protein (thioredoxin). Although the goal can be reach, and the protein visualized in situ, many experimental difficulties must be fixed. The sequence of events comprises (i) in cellulo labeling of the target protein with a N₃-lipoic acid derivative catalyzed by the mutant ligase, (ii) the further introduction by click chemistry onto this lysine sidechain of a fluorophore and (iii) the following of the labeled protein in living cells. One of the main difficulties was to assess the click chemistry step onto the living cells, because images from both control and experimental cells were similar. Alternatively, we describe at that stage, the preferred use of another technique: the Halo-Tag one that led to the obtention of clear images of the targeted protein in its cellular context. Although the ligase-mediated labeling of protein in situ is a rich domain for which many cellular tools must be developed, many difficulties must be considered before entering a systematic use of this approach.

Conclusions: In the present contribution, we added several steps of analytical characterization, both in vitro and in cellulo that were previously lacking. Furthermore, we show that the use of the click chemistry should be manipulated with care, as the claimed specificity might be not complete whenever living cells are used. Finally, we added another approach-the Halo Tag-to complete the previously suggested approaches for labelling proteins in cells, as we found difficult to strictly apply the previously reported methodology.

Keywords: Cellular; Fluorescence; In vitro; Ligase; Protein labelling.

MeSH terms

Click Chemistry
Escherichia coli / enzymology*
Escherichia coli Proteins / genetics*
Escherichia coli Proteins / metabolism
HEK293 Cells
Humans
Ligases / genetics*
Ligases / metabolism
Lysine / chemistry
Protein Engineering
Protein Processing, Post-Translational
Thioctic Acid / chemistry
Thioredoxins / chemistry
Thioredoxins / genetics
Thioredoxins / metabolism*

Substances

Escherichia coli Proteins
TXN protein, human
lplA protein, E coli
Thioredoxins
Thioctic Acid
Ligases
Lysine