Cellular Interactome Dynamics during Paclitaxel Treatment

Chavez, Juan D.; Keller, Andrew; Zhou, Bo; Tian, Rong; Bruce, James E.

doi:10.1016/j.celrep.2019.10.063

Cited by 55 publications

(71 citation statements)

References 84 publications

(102 reference statements)

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“…There have been several recent advances in enrichment and detection of crosslinked peptides by Crosslinking MS that suggest it will soon be able to map large portions of the cellular interactome in a single experiment 3 , 13 , 25 . This will open the door to detecting changes in these interactomes in different cellular states by quantification of the abundances of the detected crosslinks 2 , 26 . All of these advances require correctly controlled FDR to produce results that can be relied upon.…”

Section: Discussionmentioning

confidence: 99%

“…rosslinking mass spectrometry (Crosslinking MS) has become a key technology for understanding the architecture of multi-protein complexes by providing distance restraints between protein residues 1 . These studies are typically performed on purified complexes, but in recent years pioneering studies have used Crosslinking MS to study the topology of PPIs in more complex systems, such as cell lysates, organelles or whole cells [2][3][4][5][6][7][8][9][10][11][12][13] . Crosslinking MS is therefore emerging as a technique for mapping PPIs alongside existing tools, such as two-hybrid screens, affinity purification, proximity labelling techniques and co-fractionation studies.…”

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confidence: 99%

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Reliable identification of protein-protein interactions by crosslinking mass spectrometry

et al. 2021

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Protein-protein interactions govern most cellular pathways and processes, and multiple technologies have emerged to systematically map them. Assessing the error of interaction networks has been a challenge. Crosslinking mass spectrometry is currently widening its scope from structural analyses of purified multi-protein complexes towards systems-wide analyses of protein-protein interactions (PPIs). Using a carefully controlled large-scale analysis of Escherichia coli cell lysate, we demonstrate that false-discovery rates (FDR) for PPIs identified by crosslinking mass spectrometry can be reliably estimated. We present an interaction network comprising 590 PPIs at 1% decoy-based PPI-FDR. The structural information included in this network localises the binding site of the hitherto uncharacterised protein YacL to near the DNA exit tunnel on the RNA polymerase.

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Section: Discussionmentioning

confidence: 99%

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confidence: 99%

Reliable identification of protein-protein interactions by crosslinking mass spectrometry

et al. 2021

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“…Since XL‐MS can be performed with complex samples, such as, living cells, this technique offers the unique ability to visualize large‐scale conformational and protein interaction changes that can occur during perturbation 19,78 . For example, quantitative crosslinking with mass spectrometry (qXL‐MS) enables the assessment of interactome changes in control and drug treated cells 37,79,80 . As with traditional quantitative proteomics, qXL‐MS utilizes either stable isotope labeling or label‐free quantitation methods.…”

Section: Quantitative Xl‐msmentioning

confidence: 99%

“…Introduction of MS-cleavable bond(s) into a crosslinker spacer chain using collisions (PIR, 26 DSBU, 27 and DSSO 28 ), photons (IRCX 29 ), or electrons (DEST 30 ) allows release of linear peptides in gas phase for further fragmentation. Crosslinker with MS-cleavable bond(s) has been an enabling factor for advancing XL-MS for protein structural/interaction studies at proteome-wide scale, including whole cell lysate, [31][32][33][34] living cells, 28,[35][36][37] functional organelle, [38][39][40][41] tissues and organs. 18,42 Incorporation of two MS-cleavable bonds has introduced a novel class of crosslinker molecules named Protein Interaction Reporters (PIR), 26 in which the release of the middle spacer section upon cleavage of both labile bonds can produce reporter ions that serve to readily identify tandem spectra containing crosslinked peptides.…”

Section: Xl-ms General Workflowmentioning

confidence: 99%

Crosslinking mass spectrometry: A link between structural biology and systems biology

et al. 2021

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Protein structure underpins functional roles in all biological processes; therefore, improved understanding of protein structures is of fundamental importance in nearly all biological and biomedical research areas. Traditional techniques such as X‐ray crystallography and more recently, cryo‐EM, can reveal structural features on isolated proteins/protein complexes at atomic resolution level and have become indispensable tools for structural biology. Crosslinking mass spectrometry (XL‐MS), on the other hand, is an emerging technique capable of capturing transient and dynamic information on protein interactions and assemblies in their native environment. The combination of XL‐MS with traditional techniques holds potential for bridging the gap between structural biology and systems biology approaches. Such a combination will enable visualization of protein structures and interactions within the crowded macromolecular environment in living systems that can dramatically increase understanding of biological functions. In this review, we first discuss general strategies of XL‐MS and then survey recent examples to show how qualitative and quantitative XL‐MS studies can be integrated with available protein structural data to better understand biological function at systems level.

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“…[16][17][18][19] Regrettably, PTX has many toxic side effects such as myelosuppression, neurotoxicity, cardiotoxicity, joint or muscle pain, liver toxicity, and renal toxicity. [20][21][22] Moreover, it is sparingly water-soluble and therefore has limited application as an intravenous injection. 23 Luckily, AuNPs with good water solubility and targeting can reduce the side effects of such drugs and improve their efficacy.…”

Section: Introductionmentioning

confidence: 99%

Evaluation of the Biological Activity of Folic Acid-Modified Paclitaxel-Loaded Gold Nanoparticles

Ren¹,

Cai²,

Zhao³

et al. 2021

IJN

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Cellular Interactome Dynamics during Paclitaxel Treatment

Cited by 55 publications

References 84 publications

Reliable identification of protein-protein interactions by crosslinking mass spectrometry

Reliable identification of protein-protein interactions by crosslinking mass spectrometry

Crosslinking mass spectrometry: A link between structural biology and systems biology

Evaluation of the Biological Activity of Folic Acid-Modified Paclitaxel-Loaded Gold Nanoparticles

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