Detection of Listeria innocua on roll-to-roll produced SERS substrates with gold nanoparticles

被引:23
|
作者
Uusitalo, S. [1 ]
Kogler, M. [2 ,7 ]
Valimaa, A. -L. [3 ]
Popov, A. [4 ]
Ryabchikov, Yu. [5 ,9 ]
Kontturi, V. [6 ]
Siitonen, S. [6 ]
Petaja, J. [1 ]
Virtanen, T. [8 ]
Laitinen, R. [3 ]
Kinnunen, M. [4 ]
Meglinski, I. [4 ]
Kabashin, A. [5 ]
Bunker, A. [2 ]
Viitala, T. [2 ]
Hiltunen, J. [1 ]
机构
[1] VTT Tech Res Ctr Finland, Kaitovayla 1, Oulu 90590, Finland
[2] Univ Helsinki, Fac Pharm, Div Pharmaceut Biosci, Ctr Drug Res, FIN-00014 Helsinki, Finland
[3] Univ Oulu, Natl Resources Inst Finland LUKE, Biobased Business & Ind, POB 413,Paavo Havaksen Tie 3, FI-90014 Oulu, Finland
[4] Univ Oulu, Fac Informat Technol & Elect Engn, Optoelect & Measurement Tech, Oulu, Finland
[5] Aix Marseille Univ, Lab Lasers, Plasmas Proc Photon, Case 917, 163 Ave Luminy, F-13288 Marseille 09, France
[6] Nanocomp Oy Ltd, Ensolantie 6, Lehmo 80710, Finland
[7] Tech Univ Berlin, Inst Biotechnol, Lab Bioproc Engn, Ackerstr 71-76, D-13355 Berlin, Germany
[8] Lappeenranta Univ Technol, Sch Engn Sci, Res Grp Membrane Technol, POB 20, FI-53851 Lappeenranta, Finland
[9] Russian Acad Sci, PN Lebedev Phys Inst, 53 Leninskii Prospekt, Moscow 119991, Russia
关键词
ENHANCED RAMAN-SPECTROSCOPY; RELEVANT MICROORGANISMS; FOODBORNE PATHOGEN; ESCHERICHIA-COLI; SCATTERING SERS; RAPID DETECTION; LARGE-AREA; IDENTIFICATION; MONOCYTOGENES; BACTERIA;
D O I
10.1039/c6ra08313g
中图分类号
O6 [化学];
学科分类号
0703 ;
摘要
The rapid and accurate detection of food pathogens plays a critical role in the early prevention of foodborne epidemics. Current bacteria identification practices, including colony counting, polymerase chain reaction (PCR) and immunological methods, are time consuming and labour intensive; they are not ideal for achieving the required immediate diagnosis. Different SERS substrates have been studied for the detection of foodborne microbes. The majority of the approaches are either based on costly patterning techniques on silicon or glass wafers or on methods which have not been tested in large scale fabrication. We demonstrate the feasibility of analyte specific sensing using mass-produced, polymer-based low-cost SERS substrate in analysing the chosen model microbe with biological recognition. The use of this novel roll-to-roll fabricated SERS substrate was combined with optimised gold nanoparticles to increase the detection sensitivity. Distinctive SERS spectral bands were recorded for Listeria innocua ATCC 33090 using an in-house build (785 nm) near infra red (NIR) Raman system. Results were compared to both those found in the literature and the results obtained from a commercial time-gated Raman system with a 532 nm wavelength laser excitation. The effect of the SERS enhancer metal and the excitation wavelength on the detected spectra was found to be negligible. The hypothesis that disagreements within the literature regarding bacterial spectra results from conditions present during the detection process has not been supported. The sensitivity of our SERS detection was improved through optimization of the concentration of the sample inside the hydrophobic polydimethylsiloxane (PDMS) wells. Immunomagnetic separation (IMS) beads were used to assist the accumulation of bacteria into the path of the beam of the excitation laser. With this combination we have detected Listeria with gold enhanced SERS in a label free manner from such low sample concentrations as 10(4) CFU ml(-1).
引用
收藏
页码:62981 / 62989
页数:9
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