Real-time library search increases cross-link identification depth across all levels of sample complexity

Author:

Ruwolt Max,He Yi,Lima Diogo Borges,Barshop William,Broichhagen JohannesORCID,Huguet Romain,Viner Rosa,Liu Fan

Abstract

AbstractCross-linking mass spectrometry (XL-MS) is a universal tool for probing structural dynamics and protein-protein interactionsin vitroandin vivo. Although cross-linked peptides are naturally less abundant than their unlinked counterparts, recent experimental advances improved cross-link identification by enriching the cross-linker modified peptides chemically with the use of enrichable cross-linkers. However, mono-links (i.e., peptides modified with a hydrolyzed cross-linker) still hinder efficient cross-link identification since a large proportion of measurement time is spent on their MS2 acquisition. Currently, cross-links and mono-links cannot be separated by sample preparation techniques or chromatography because they are chemically almost identical. Here, we found that based on the intensity ratios of four diagnostic peaks when using PhoX/tBu-PhoX cross-linkers, cross-links and mono-links can be partially distinguished. Harnessing their characteristic intensity ratios for real-time library search (RTLS)-based triggering of high-resolution MS2 scans increased the number of cross-link identifications from both single protein samples and intactE. colicells. Specifically, RTLS improves cross-link identification from unenriched samples and short gradients, emphasizing its advantages in high-throughput approaches and when instrument time or sample amount is limited.

Publisher

Cold Spring Harbor Laboratory

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