Site-selective photo-crosslinking for the characterisation of transient ubiquitin-like protein-protein interactions

Zac Sandy; Zijuan Wang; Deepak Behera; Benjamin M. Foster; Finlay A. Martin; Kira Brüninghoff; Kathleen M. Cain; Wolfgang Dörner; Maria Jose Cabello-Lobato; Josep V. Forment; Matthew J. Cliff; Igor Larrosa; Perdita Barran; Duncan L. Smith; Henning D. Mootz; Christine K. Schmidt

doi:10.1371/journal.pone.0316321

Site-selective photo-crosslinking for the characterisation of transient ubiquitin-like protein-protein interactions

Zac Sandy, Zijuan Wang, Deepak Behera, Benjamin M. Foster, Finlay A. Martin, Kira Brüninghoff, Kathleen M. Cain, Wolfgang Dörner, Maria Jose Cabello-Lobato, Josep V. Forment, Matthew J. Cliff, Igor Larrosa, Perdita Barran, Duncan L. Smith, Henning D. Mootz, Christine K. Schmidt

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

Abstract

Non-covalent protein-protein interactions are one of the most fundamental building blocks in cellular signalling pathways. Despite this, they have been historically hard to identify using conventional methods due to their often weak and transient nature. Using genetic code expansion and incorporation of commercially available unnatural amino acids, we have developed a highly accessible method whereby interactions between biotinylated ubiquitin-like protein (UBL) probes and their binding partners can be stabilised using ultraviolet (UV) light-induced crosslinks. The stabilised protein complexes can be purified using affinity purification and identified by mass spectrometry. The resultant covalent bonds can withstand even the harshest washing conditions, allowing for the removal of indirect binders whilst retaining and capturing weak and transient interactors that are commonly lost during wash steps. This technique is widely applicable and highly effective for identifying site-selective non-covalent interactors. Members of our team have previously demonstrated the benefit of this method using the small ubiquitin-like modifier (SUMO). Here, we provide further proof-of-principle validation of the method and highlight its generality by applying an optimised workflow to a lesser studied UBL, interferon stimulated gene 15 (ISG15). We show that this method is able to capture known ISG15 interactors from a complex protein mixture in a site-selective manner, only capturing proteins that specifically interact with the region of ISG15 where the unnatural amino acid was incorporated. This exquisite degree of sensitivity and specificity greatly improves upon previous screens aimed at identifying downstream non-covalent binders, or readers, of ISG15. Taken together, the approach opens the possibility of characterising previously undetected protein-protein interactions, with the potential of elucidating molecular mechanisms behind the most complex and poorly understood processes in the cell.

Original language	English
Article number	e0316321
Journal	PLoS ONE
Volume	20
Issue number	1
DOIs	https://doi.org/10.1371/journal.pone.0316321
Publication status	Published - 27 Jan 2025

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Sandy, Z., Wang, Z., Behera, D., Foster, B. M., Martin, F. A., Brüninghoff, K., Cain, K. M., Dörner, W., Cabello-Lobato, M. J., Forment, J. V., Cliff, M. J., Larrosa, I., Barran, P., Smith, D. L., Mootz, H. D., & Schmidt, C. K. (2025). Site-selective photo-crosslinking for the characterisation of transient ubiquitin-like protein-protein interactions. PLoS ONE, 20(1), Article e0316321. https://doi.org/10.1371/journal.pone.0316321

@article{5665722e55ad4a278c0d8e69e173fcba,

title = "Site-selective photo-crosslinking for the characterisation of transient ubiquitin-like protein-protein interactions",

abstract = "Non-covalent protein-protein interactions are one of the most fundamental building blocks in cellular signalling pathways. Despite this, they have been historically hard to identify using conventional methods due to their often weak and transient nature. Using genetic code expansion and incorporation of commercially available unnatural amino acids, we have developed a highly accessible method whereby interactions between biotinylated ubiquitin-like protein (UBL) probes and their binding partners can be stabilised using ultraviolet (UV) light-induced crosslinks. The stabilised protein complexes can be purified using affinity purification and identified by mass spectrometry. The resultant covalent bonds can withstand even the harshest washing conditions, allowing for the removal of indirect binders whilst retaining and capturing weak and transient interactors that are commonly lost during wash steps. This technique is widely applicable and highly effective for identifying site-selective non-covalent interactors. Members of our team have previously demonstrated the benefit of this method using the small ubiquitin-like modifier (SUMO). Here, we provide further proof-of-principle validation of the method and highlight its generality by applying an optimised workflow to a lesser studied UBL, interferon stimulated gene 15 (ISG15). We show that this method is able to capture known ISG15 interactors from a complex protein mixture in a site-selective manner, only capturing proteins that specifically interact with the region of ISG15 where the unnatural amino acid was incorporated. This exquisite degree of sensitivity and specificity greatly improves upon previous screens aimed at identifying downstream non-covalent binders, or readers, of ISG15. Taken together, the approach opens the possibility of characterising previously undetected protein-protein interactions, with the potential of elucidating molecular mechanisms behind the most complex and poorly understood processes in the cell.",

author = "Zac Sandy and Zijuan Wang and Deepak Behera and Foster, {Benjamin M.} and Martin, {Finlay A.} and Kira Br{\"u}ninghoff and Cain, {Kathleen M.} and Wolfgang D{\"o}rner and Cabello-Lobato, {Maria Jose} and Forment, {Josep V.} and Cliff, {Matthew J.} and Igor Larrosa and Perdita Barran and Smith, {Duncan L.} and Mootz, {Henning D.} and Schmidt, {Christine K.}",

year = "2025",

month = jan,

day = "27",

doi = "10.1371/journal.pone.0316321",

language = "English",

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Sandy, Z, Wang, Z, Behera, D , Foster, BM , Martin, FA, Brüninghoff, K, Cain, KM, Dörner, W, Cabello-Lobato, MJ, Forment, JV, Cliff, MJ , Larrosa, I , Barran, P, Smith, DL, Mootz, HD & Schmidt, CK 2025, 'Site-selective photo-crosslinking for the characterisation of transient ubiquitin-like protein-protein interactions', PLoS ONE, vol. 20, no. 1, e0316321. https://doi.org/10.1371/journal.pone.0316321

TY - JOUR

T1 - Site-selective photo-crosslinking for the characterisation of transient ubiquitin-like protein-protein interactions

AU - Sandy, Zac

AU - Wang, Zijuan

AU - Behera, Deepak

AU - Foster, Benjamin M.

AU - Martin, Finlay A.

AU - Brüninghoff, Kira

AU - Cain, Kathleen M.

AU - Dörner, Wolfgang

AU - Cabello-Lobato, Maria Jose

AU - Forment, Josep V.

AU - Cliff, Matthew J.

AU - Larrosa, Igor

AU - Barran, Perdita

AU - Smith, Duncan L.

AU - Mootz, Henning D.

AU - Schmidt, Christine K.

PY - 2025/1/27

Y1 - 2025/1/27

N2 - Non-covalent protein-protein interactions are one of the most fundamental building blocks in cellular signalling pathways. Despite this, they have been historically hard to identify using conventional methods due to their often weak and transient nature. Using genetic code expansion and incorporation of commercially available unnatural amino acids, we have developed a highly accessible method whereby interactions between biotinylated ubiquitin-like protein (UBL) probes and their binding partners can be stabilised using ultraviolet (UV) light-induced crosslinks. The stabilised protein complexes can be purified using affinity purification and identified by mass spectrometry. The resultant covalent bonds can withstand even the harshest washing conditions, allowing for the removal of indirect binders whilst retaining and capturing weak and transient interactors that are commonly lost during wash steps. This technique is widely applicable and highly effective for identifying site-selective non-covalent interactors. Members of our team have previously demonstrated the benefit of this method using the small ubiquitin-like modifier (SUMO). Here, we provide further proof-of-principle validation of the method and highlight its generality by applying an optimised workflow to a lesser studied UBL, interferon stimulated gene 15 (ISG15). We show that this method is able to capture known ISG15 interactors from a complex protein mixture in a site-selective manner, only capturing proteins that specifically interact with the region of ISG15 where the unnatural amino acid was incorporated. This exquisite degree of sensitivity and specificity greatly improves upon previous screens aimed at identifying downstream non-covalent binders, or readers, of ISG15. Taken together, the approach opens the possibility of characterising previously undetected protein-protein interactions, with the potential of elucidating molecular mechanisms behind the most complex and poorly understood processes in the cell.

AB - Non-covalent protein-protein interactions are one of the most fundamental building blocks in cellular signalling pathways. Despite this, they have been historically hard to identify using conventional methods due to their often weak and transient nature. Using genetic code expansion and incorporation of commercially available unnatural amino acids, we have developed a highly accessible method whereby interactions between biotinylated ubiquitin-like protein (UBL) probes and their binding partners can be stabilised using ultraviolet (UV) light-induced crosslinks. The stabilised protein complexes can be purified using affinity purification and identified by mass spectrometry. The resultant covalent bonds can withstand even the harshest washing conditions, allowing for the removal of indirect binders whilst retaining and capturing weak and transient interactors that are commonly lost during wash steps. This technique is widely applicable and highly effective for identifying site-selective non-covalent interactors. Members of our team have previously demonstrated the benefit of this method using the small ubiquitin-like modifier (SUMO). Here, we provide further proof-of-principle validation of the method and highlight its generality by applying an optimised workflow to a lesser studied UBL, interferon stimulated gene 15 (ISG15). We show that this method is able to capture known ISG15 interactors from a complex protein mixture in a site-selective manner, only capturing proteins that specifically interact with the region of ISG15 where the unnatural amino acid was incorporated. This exquisite degree of sensitivity and specificity greatly improves upon previous screens aimed at identifying downstream non-covalent binders, or readers, of ISG15. Taken together, the approach opens the possibility of characterising previously undetected protein-protein interactions, with the potential of elucidating molecular mechanisms behind the most complex and poorly understood processes in the cell.

U2 - 10.1371/journal.pone.0316321

DO - 10.1371/journal.pone.0316321

M3 - Article

SN - 1932-6203

VL - 20

JO - PLoS ONE

JF - PLoS ONE

IS - 1

M1 - e0316321

ER -

Site-selective photo-crosslinking for the characterisation of transient ubiquitin-like protein-protein interactions

Abstract

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