High-Sensitivity Proteome-Scale Searches for Crosslinked Peptides Using CRIMP 2.0

Crowder, David A.; Sarpe, Vladimir; Amaral, B.C. do; Brodie, Nicholas I.; Schriemer, David C.

doi:10.1021/acs.analchem.3c00329

Cited by 10 publications

(3 citation statements)

References 30 publications

(76 reference statements)

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“…All raw files were analyzed using Mass Spec Studio 32 (v2.4) CRIMP 2.0, 33 including those from Rey et al. 2021 23 for consistency.…”

Section: Methodsmentioning

confidence: 99%

Do Not Waste Time─Ensure Success in Your Cross-Linking Mass Spectrometry Experiments before You Begin

Nouchikian,

Fernandez-Martinez,

Renard

et al. 2024

Anal. Chem.

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Cross-linking mass spectrometry (XL-MS) has become a very useful tool for studying protein complexes and interactions in living systems. It enables the investigation of many large and dynamic assemblies in their native state, providing an unbiased view of their protein interactions and restraints for integrative modeling. More researchers are turning toward trying XL-MS to probe their complexes of interest, especially in their native environments. However, due to the presence of other potentially higher abundant proteins, sufficient cross-links on a system of interest may not be reached to achieve satisfactory structural and interaction information. There are currently no rules for predicting whether XL-MS experiments are likely to work or not; in other words, if a protein complex of interest will lead to useful XL-MS data. Here, we show that a simple iBAQ (intensity-based absolute quantification) analysis performed from trypsin digest data can provide a good understanding of whether proteins of interest are abundant enough to achieve successful cross-linking data. Comparing our findings to large-scale data on diverse systems from several other groups, we show that proteins of interest should be at least in the top 20% abundance range to expect more than one cross-link found per protein. We foresee that this guideline is a good starting point for researchers who would like to use XL-MS to study their protein of interest and help ensure a successful cross-linking experiment from the beginning. Data are available via ProteomeXchange with identifier PXD045792.

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“…All raw files were analyzed using Mass Spec Studio 32 (v2.4) CRIMP 2.0, 33 including those from Rey et al. 2021 23 for consistency.…”

Section: Methodsmentioning

confidence: 99%

Do Not Waste Time─Ensure Success in Your Cross-Linking Mass Spectrometry Experiments before You Begin

Nouchikian,

Fernandez-Martinez,

Renard

et al. 2024

Anal. Chem.

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“…20 An obvious advantage of Mass spec studio is that it supports multiple custom additions in its user interface, allowing visualization of MS1 and MS2 data in the results interface and allowing users to map cross-linking results directly to protein structures with PyMol (Figure 3D). Besides, the recently updated CRIMP 2.0 integrates an improved two-pass library reduction engine and a new scoring algorithm, 43 allows for a search of both noncleavable and MS-cleavable cross-linkers. However, the overall performance of the engine and its capabilities to identify various cross-linkers remain to be tested.…”

Section: Xl-ms Search Enginesmentioning

confidence: 99%

Innovation in Cross-Linking Mass Spectrometry Workflows: Toward a Comprehensive, Flexible, and Customizable Data Analysis Platform

Nie

2023

J. Am. Soc. Mass Spectrom.

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Cross-linking mass spectrometry (XL-MS) is widely used in the analysis of protein structure and protein−protein interactions (PPIs). Throughout the entire workflow, the utilization of cross-linkers and the interpretation of cross-linking data are the core steps. In recent years, the development of crosslinkers and analytical software mostly follow up on the classical models of non-cleavable cross-linkers such as BS3/DSS and MScleavable cross-linkers such as DSSO. Although such a paradigm promotes the maturity and robustness of the XL-MS field, it confines the innovation and flexibility of new cross-linkers and analytical software. This critical insight will discuss the classification, advantages, and disadvantages of existing data analysis search engines. Take the new platinum-based metal cross-linker as an example, potential pitfalls in characterization of cross-linked peptides using existing software are discussed. Finally, ideas on developing more flexible, comprehensive, and userfriendly cross-linkers and software tools are proposed.

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“…After crosslink installation, cells are lysed and digested in a standard “bottom-up” workflow common to conventional proteomics routines, generating linked peptides for detection by MS. Crosslinked peptides are minor reaction products and cannot be identified with the conventional database searching strategies used in the proteomics community. New software makes the detection of crosslinks more efficient than ever before 14–18 , but very little progress has been made in improving the crosslinking reaction itself. To faithfully sample both the spatial and temporal properties of the proteome, crosslinkers must cross the cell membrane, perfuse freely throughout the cell, and react quickly.…”

Section: Introductionmentioning

confidence: 99%

Cell fixation improves performance ofin situcrosslinking mass spectrometry while preserving cellular ultrastructure

Michael,

Amaral,

Ball

et al. 2024

Preprint

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Crosslinking mass spectrometry (XL-MS) has the potential to map the interactome of the cell with high resolution and depth of coverage. However, current in vivo XL-MS methods are hampered by crosslinkers that demonstrate low cell permeability and require long reaction times. Consequently, interactome sampling is not high and long incubation times can distort the cell, bringing into question the validity any protein interactions identified by the method. We address these issues with a fast formaldehyde-based fixation method applied prior to the introduction of secondary crosslinkers. Using human A549 cells and a range of reagents, we show that 4% formaldehyde fixation with membrane permeabilization preserves cellular ultrastructure and simultaneously improves reaction conditions for in situ XL-MS. Protein labeling yields can be increased even for nominally membrane-permeable reagents, and surprisingly, formaldehyde does not compete with conventional amine-reactive crosslinking reagents. Prefixation with permeabilization uncouples cellular dynamics from crosslinker dynamics, enhancing control over crosslinking yield and permitting the use of any chemical crosslinker.

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High-Sensitivity Proteome-Scale Searches for Crosslinked Peptides Using CRIMP 2.0

Cited by 10 publications

References 30 publications

Do Not Waste Time─Ensure Success in Your Cross-Linking Mass Spectrometry Experiments before You Begin

Do Not Waste Time─Ensure Success in Your Cross-Linking Mass Spectrometry Experiments before You Begin

Innovation in Cross-Linking Mass Spectrometry Workflows: Toward a Comprehensive, Flexible, and Customizable Data Analysis Platform

Cell fixation improves performance ofin situcrosslinking mass spectrometry while preserving cellular ultrastructure

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