Species-specific quantification of circulating ebolavirus burden using VP40-derived peptide variants

Shu, Qingbo; Kenny, Tara; Fan, Jia; Lyon, Christopher J.; Cazares, Lisa H.; Hu, Tony

doi:10.1371/journal.ppat.1010039

Cited by 2 publications

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References 34 publications

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“…Inspired by our previous work on developing a rapid diagnostic test for Ebola infectious disease, [ 44 ] we tested the 4‐h sample preparation workflow in the multiplexed IP‐MS assay of EsxN and CFP‐10 peptide variants. We selected four representative MGIT samples infected with Mtb or M. kansasii or MAC, and shorten the time of trypsin digestion of MGIT samples from 16 to 1 h. It showed that the peptide variant targets were all identified correctly for their species origin (Figure S5–S10).…”

Section: Resultsmentioning

confidence: 99%

Peptidomic analysis of mycobacterial secreted proteins enables species identification

Shu

Rajagopal

Fan

et al. 2022

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Pulmonary disease arising from slow‐growing mycobacterial infections has emerged as an increasingly prevalent clinical concern over the past two to three decades. Proteins belonging to the family of ESAT‐6 secretion (Esx) systems play critical roles in the virulence of most pathogenic mycobacterial species and are associated with drug resistance. However, no clinical applications can detect and discriminate the expression of species‐specific variants of these proteins in clinical samples, such as early growth cultures, for rapid diagnosis of specific mycobacterial infections, which may require distinct interventions. Conventional immunoassay approaches are not suitable for this purpose due to the significant degree of conservation of Esx proteins among species. Herein we describe the development of a novel immunoprecipitation‐coupled mass spectrometry assay that can distinguish Esx proteins that are expressed by slow‐growing mycobacterial species commonly detected in clinical isolates. This approach uses custom antibodies raised against single semi‐conserved peptide regions in M. tuberculosis (Mtb) EsxB and EsxN to capture corresponding peptides from protein orthologs of mycobacteria associated with human respiratory infections, including Mtb, M. avium, M. intracellulare, M. kansasii, M. gordonae, and M. marinum, to detect these species in standard clinical cultures at the first sign mycobacterial growth to allow rapid disease diagnosis.

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Section: Resultsmentioning

confidence: 99%