4.7 Article

A new mass spectral library for high-coverage and reproducible analysis of the Plasmodium falciparum-infected red blood cell proteome

期刊

GIGASCIENCE
卷 11, 期 -, 页码 -

出版社

OXFORD UNIV PRESS
DOI: 10.1093/gigascience/giac008

关键词

Plasmodium falciparum; malaria; proteomics; data-dependent acquisition; data-independent acquisition; red blood cells; LC-MS; MS

资金

  1. Australian National Health and Medical Research Council (NHMRC) [APP1128003, APP1160705, APP1148700]

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A comprehensive spectral library for Plasmodium falciparum-infected RBCs has been created, measuring the abundance of peptides from both the parasite and RBC proteins. This library includes proteins from different RBC stages, the RBC compartment of trophozoite-iRBCs, and cytosolic fraction from uninfected RBCs. By using this library, semi-quantitative proteomics datasets have been generated to characterize different asexual parasite stages and compare drug-resistant and drug-sensitive parasites.
Background Plasmodium falciparum causes the majority of malaria mortality worldwide, and the disease occurs during the asexual red blood cell (RBC) stage of infection. In the absence of an effective and available vaccine, and with increasing drug resistance, asexual RBC stage parasites are an important research focus. In recent years, mass spectrometry-based proteomics using data-dependent acquisition has been extensively used to understand the biochemical processes within the parasite. However, data-dependent acquisition is problematic for the detection of low-abundance proteins and proteome coverage and has poor run-to-run reproducibility. Results Here, we present a comprehensive P. falciparum-infected RBC (iRBC) spectral library to measure the abundance of 44,449 peptides from 3,113 P. falciparum and 1,617 RBC proteins using a data-independent acquisition mass spectrometric approach. The spectral library includes proteins expressed in the 3 morphologically distinct RBC stages (ring, trophozoite, schizont), the RBC compartment of trophozoite-iRBCs, and the cytosolic fraction from uninfected RBCs. This spectral library contains 87% of all P. falciparum proteins that have previously been reported with protein-level evidence in blood stages, as well as 692 previously unidentified proteins. The P. falciparum spectral library was successfully applied to generate semi-quantitative proteomics datasets that characterize the 3 distinct asexual parasite stages in RBCs, and compared artemisinin-resistant (Cam3.IIR539T) and artemisinin-sensitive (Cam3.IIrev) parasites. Conclusion A reproducible, high-coverage proteomics spectral library and analysis method has been generated for investigating sets of proteins expressed in the iRBC stage of P. falciparum malaria. This will provide a foundation for an improved understanding of parasite biology, pathogenesis, drug mechanisms, and vaccine candidate discovery for malaria.

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