Structure-guided approach to site-specific fluorophore labeling of the lac repressor LacI

The lactose operon repressor protein LacI has long served as a paradigm of the bacterial transcription factors. However, the mechanisms whereby LacI rapidly locates its cognate binding site on the bacterial chromosome are still elusive. Single-molecule fluorescence imaging approaches are well suited...

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Autores principales: Kipper, Kalle, Eremina, Nadja, Marklund, Emil, Tubasum, Sumera, Mao, Guanzhong, Lehmann, Laura Christina, Elf, Johan, Deindl, Sebastian
Formato: Online Artículo Texto
Lenguaje:English
Publicado: Public Library of Science 2018
Materias:
Research Article
Acceso en línea:https://www.ncbi.nlm.nih.gov/pmc/articles/PMC5983854/
https://www.ncbi.nlm.nih.gov/pubmed/29856839
http://dx.doi.org/10.1371/journal.pone.0198416
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author Kipper, Kalle
Eremina, Nadja
Marklund, Emil
Tubasum, Sumera
Mao, Guanzhong
Lehmann, Laura Christina
Elf, Johan
Deindl, Sebastian
author_facet Kipper, Kalle
Eremina, Nadja
Marklund, Emil
Tubasum, Sumera
Mao, Guanzhong
Lehmann, Laura Christina
Elf, Johan
Deindl, Sebastian
author_sort Kipper, Kalle
collection PubMed
description The lactose operon repressor protein LacI has long served as a paradigm of the bacterial transcription factors. However, the mechanisms whereby LacI rapidly locates its cognate binding site on the bacterial chromosome are still elusive. Single-molecule fluorescence imaging approaches are well suited for the study of these mechanisms but rely on a functionally compatible fluorescence labeling of LacI. Particularly attractive for protein fluorescence labeling are synthetic fluorophores due to their small size and favorable photophysical characteristics. Synthetic fluorophores are often conjugated to natively occurring cysteine residues using maleimide chemistry. For a site-specific and functionally compatible labeling with maleimide fluorophores, the target protein often needs to be redesigned to remove unwanted native cysteines and to introduce cysteines at locations better suited for fluorophore attachment. Biochemical screens can then be employed to probe for the functional activity of the redesigned protein both before and after dye labeling. Here, we report a mutagenesis-based redesign of LacI to enable a functionally compatible labeling with maleimide fluorophores. To provide an easily accessible labeling site in LacI, we introduced a single cysteine residue at position 28 in the DNA-binding headpiece of LacI and replaced two native cysteines with alanines where derivatization with bulky substituents is known to compromise the protein’s activity. We find that the redesigned LacI retains a robust activity in vitro and in vivo, provided that the third native cysteine at position 281 is retained in LacI. In a total internal reflection microscopy assay, we observed individual Cy3-labeled LacI molecules bound to immobilized DNA harboring the cognate O(1) operator sequence, indicating that the dye-labeled LacI is functionally active. We have thus been able to generate a functional fluorescently labeled LacI that can be used to unravel mechanistic details of LacI target search at the single molecule level.
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spelling pubmed-59838542018-06-16 Structure-guided approach to site-specific fluorophore labeling of the lac repressor LacI Kipper, Kalle Eremina, Nadja Marklund, Emil Tubasum, Sumera Mao, Guanzhong Lehmann, Laura Christina Elf, Johan Deindl, Sebastian PLoS One Research Article The lactose operon repressor protein LacI has long served as a paradigm of the bacterial transcription factors. However, the mechanisms whereby LacI rapidly locates its cognate binding site on the bacterial chromosome are still elusive. Single-molecule fluorescence imaging approaches are well suited for the study of these mechanisms but rely on a functionally compatible fluorescence labeling of LacI. Particularly attractive for protein fluorescence labeling are synthetic fluorophores due to their small size and favorable photophysical characteristics. Synthetic fluorophores are often conjugated to natively occurring cysteine residues using maleimide chemistry. For a site-specific and functionally compatible labeling with maleimide fluorophores, the target protein often needs to be redesigned to remove unwanted native cysteines and to introduce cysteines at locations better suited for fluorophore attachment. Biochemical screens can then be employed to probe for the functional activity of the redesigned protein both before and after dye labeling. Here, we report a mutagenesis-based redesign of LacI to enable a functionally compatible labeling with maleimide fluorophores. To provide an easily accessible labeling site in LacI, we introduced a single cysteine residue at position 28 in the DNA-binding headpiece of LacI and replaced two native cysteines with alanines where derivatization with bulky substituents is known to compromise the protein’s activity. We find that the redesigned LacI retains a robust activity in vitro and in vivo, provided that the third native cysteine at position 281 is retained in LacI. In a total internal reflection microscopy assay, we observed individual Cy3-labeled LacI molecules bound to immobilized DNA harboring the cognate O(1) operator sequence, indicating that the dye-labeled LacI is functionally active. We have thus been able to generate a functional fluorescently labeled LacI that can be used to unravel mechanistic details of LacI target search at the single molecule level. Public Library of Science 2018-06-01 /pmc/articles/PMC5983854/ /pubmed/29856839 http://dx.doi.org/10.1371/journal.pone.0198416 Text en © 2018 Kipper et al http://creativecommons.org/licenses/by/4.0/ This is an open access article distributed under the terms of the Creative Commons Attribution License (http://creativecommons.org/licenses/by/4.0/) , which permits unrestricted use, distribution, and reproduction in any medium, provided the original author and source are credited.
spellingShingle Research Article
Kipper, Kalle
Eremina, Nadja
Marklund, Emil
Tubasum, Sumera
Mao, Guanzhong
Lehmann, Laura Christina
Elf, Johan
Deindl, Sebastian
Structure-guided approach to site-specific fluorophore labeling of the lac repressor LacI
title Structure-guided approach to site-specific fluorophore labeling of the lac repressor LacI
title_full Structure-guided approach to site-specific fluorophore labeling of the lac repressor LacI
title_fullStr Structure-guided approach to site-specific fluorophore labeling of the lac repressor LacI
title_full_unstemmed Structure-guided approach to site-specific fluorophore labeling of the lac repressor LacI
title_short Structure-guided approach to site-specific fluorophore labeling of the lac repressor LacI
title_sort structure-guided approach to site-specific fluorophore labeling of the lac repressor laci
topic Research Article
url https://www.ncbi.nlm.nih.gov/pmc/articles/PMC5983854/
https://www.ncbi.nlm.nih.gov/pubmed/29856839
http://dx.doi.org/10.1371/journal.pone.0198416
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