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The EuroBiotech Journal
Band 3 (2019): Heft 2 (April 2019)
Uneingeschränkter Zugang
Real time human micro-organisms biotyping based on Water-Assisted Laser Desorption/Ionization
Benoit Fatou
Benoit Fatou
,
Michel Salzet
Michel Salzet
und
Isabelle Fournier
Isabelle Fournier
| 24. Apr. 2019
The EuroBiotech Journal
Band 3 (2019): Heft 2 (April 2019)
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Article Category:
Research Article
Online veröffentlicht:
24. Apr. 2019
Seitenbereich:
97 - 104
DOI:
https://doi.org/10.2478/ebtj-2019-0011
Schlüsselwörter
Spidermass
,
real time analysis
,
mass spectrometry
,
bacteria typing
© 2019 Benoit Fatou, Michel Salzet, Isabelle Fournier, published by Sciendo
This work is licensed under the Creative Commons Attribution-NonCommercial-NoDerivatives 4.0 License.
Figure 1
Schematic representation of the tests proceed for pathogen identification using SpiderMass technology. 1) E. Coli were cultivated in poor broth medium. Microbial growth was assessed by the increase in A 620 nm after 8-hour incubation at 37°C . At different time of bacteria growth, 10 μl of the suspension are harvested and dropped either on agarose of a petri dish or smeared on glass slides. Direct analyses with SpiderMass were then conducted directly on the top of petri dish or smear. Direct m/z spectra profiles are then recorded.
Figure 2
Time course SpiderMass analyses from T0 to T24 hours of E. Coli growths in liquid suspension were performed on agarose of a petri dish. I 10 μl of the suspension collected at T0 and at T24h are harvested and dropped on agarose of a petri dish SpiderMass analyses were performed in negative and positive modes. (Duplicates are presented for each conditions).
Figure 3
Comparison of SpiderMass spectra A) collected either from culture medium directly , agarose (petri dish) and on smears on glass slides for bacteria collected at T24, B) represent the PCA analyses in negative mode of the spectra collected from petri dish a); Smear b) and Comparison between direct medium, agarose and smear by PCA in negative and positive modes c). C) Highlights of specific common ions detected in positive mode ranged from 549.432 to 564.453 from the 3 methods.
Figure 4
Reproducibility experiments were conducted on 3 different slides containing smears of bacteria collected at T24. Experiments were realized on the same slides analyzed 3 times during 3 consecutive days in negative A) and positive B) modes.
Figure 5
Biotyping studies in negative mode on smear of different species of pathogens i.e Gram negative (E. coli D31, Pseudomonas aeruginosa); Gram positive (Staphylococcus aureus, Enterococcus faecalis) and Yeast (Candida Albicans).
Figure 6
MS/MS analyses directly by SpiderMass in real time of selected ions from E. Coli corresponding to : m/z 688.35 to PE (16:0/cy17:0), m/z of m/z 719.35 to PG (16:0/16:1) and m/z 733.36 to PG (16:0/cys17:0), 773.38 to PG (18:1/18:1).
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