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Novel bacterial classification method by MALDI-TOF MS based on ribosomal protein coding in S10-spc-alpha Operon at Strain level

Posters | 2013 | Shimadzu | ASMSInstrumentation
MALDI, LC/MS, LC/TOF
Industries
Proteomics , Environmental
Manufacturer
Shimadzu

Summary

Importance of the Topic


Whole-cell MALDI-TOF MS (WC-MS) is a leading technique for bacterial identification based on protein mass fingerprints. While commercial systems excel at species-level classification, they often lack resolution for strain-level discrimination. Ribosomal proteins encoded in the conserved S10-spc-alpha operon represent robust biomarkers that can enable high-resolution typing even when full genome data are unavailable.

Objectives and Study Overview


This work introduces the S10-GERMS method, a proteome-based strategy to classify bacteria at strain and pathovar levels. The study focuses on Pseudomonas syringae, selecting multiple genome-sequenced and commercially available pathovars to evaluate the approach’s ability to distinguish closely related strains.

Methodology and Instrumentation


  • Whole-cell MALDI-TOF MS analysis of bacterial biomass to obtain observed protein mass spectra.
  • Sequencing of the S10-spc-alpha operon via Sanger methods and translation to amino acid sequences.
  • Calculation of theoretical masses for each ribosomal protein, incorporating N-terminal methionine loss.
  • Construction of an accurate database by matching theoretical and observed masses.
  • Phylogenetic typing of P. syringae strains based on selected ribosomal protein biomarkers.

Used Instrumentation


  • MALDI-TOF MS instrument: AXIMA Performance (Shimadzu Biotech/Kratos).
  • Acquisition mode: linear positive ion detection.
  • Matrix: sinapinic acid (10 mg/mL in 50% acetonitrile, 1% TFA).
  • Sample prep: washed whole cells mixed with matrix, air-dried on target.

Main Results and Discussion


  • From genome-sequenced P. syringae strains, 14 ribosomal proteins (< 15 kDa) were identified as reproducible mass peaks, with L24 and S17 (operon-encoded) and additional markers S12 and S16 distinguishing pathovars.
  • Seven sample strains (NBRC 3310, 3508, 12655, 12656, 14053, 14083, 14084) were profiled, revealing five distinct clusters correlating with known pathovars.
  • Profiling tables demonstrated consistent match between observed and theoretical masses, validating the database and classification scheme.

Benefits and Practical Applications of the Method


  • Enables rapid, strain-level discrimination without the need for complete genome sequencing.
  • Integrates easily with existing MALDI-TOF MS platforms widely used in microbial diagnostics, QA/QC, and environmental monitoring.
  • Supports outbreak investigations and contamination tracking by distinguishing closely related strains.

Future Trends and Potential Applications


  • Expansion of the biomarker database to additional operons and ribosomal proteins across diverse bacterial taxa.
  • Integration with high-throughput MALDI-TOF MS workflows and advanced bioinformatics for real-time surveillance.
  • Potential use in antimicrobial resistance monitoring and clinical microbiology for rapid pathogen typing.

Conclusion


The S10-GERMS approach leverages conserved ribosomal protein masses to achieve strain- and pathovar-level classification using routine WC-MS workflows. This method broadens the discriminative power of MALDI-TOF MS, offering a fast, reliable, and accessible tool for bacterial typing.

Reference


  1. Pineda F J, Chiva C, Sanz-Nebot V, Sánchez L, et al. Anal. Chem. 2003;75(16):3817–3822.
  2. Teramoto K, Ichihara K, Hosoda A, et al. Anal. Chem. 2007;79(23):8712–8719.
  3. Hotta Y, Tamura H, Sato H, et al. J. Proteome Res. 2011;9(12):6722–6728.
  4. Tamura H, Hotta Y, Yamamoto N, et al. J. Am. Soc. Mass Spectrom. 2013; DOI:10.1007/s13361-013-0627-8.

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