LabDisk with complete reagent prestorage for sample-to-answer nucleic acid based detection of respiratory pathogens verified with influenza A H3N2 virusElectronic supplementary information (ESI) available: Details of respiratory qPCR panels and rotational frequency protocol. See DOI: 10.1039/c5lc00871a
Portable point-of-care devices for pathogen detection require easy, minimal and user-friendly handling steps and need to have the same diagnostic performance compared to centralized laboratories. In this work we present a fully automated sample-to-answer detection of influenza A H3N2 virus in a cent...
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| Main Authors | , , , , , , , , , , , |
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| Format | Journal Article |
| Published |
15.12.2015
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| Online Access | Get full text |
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| Abstract | Portable point-of-care devices for pathogen detection require easy, minimal and user-friendly handling steps and need to have the same diagnostic performance compared to centralized laboratories. In this work we present a fully automated sample-to-answer detection of influenza A H3N2 virus in a centrifugal LabDisk with complete prestorage of reagents. Thus, the initial supply of the sample remains the only manual handling step. The self-contained LabDisk automates by centrifugal microfluidics all necessary process chains for PCR-based pathogen detection: pathogen lysis, magnetic bead based nucleic acid extraction, aliquoting of the eluate into 8 reaction cavities, and real-time reverse transcription polymerase chain reaction (RT-PCR). Prestored reagents comprise air dried specific primers and fluorescence probes, lyophilized RT-PCR mastermix and stick-packaged liquid reagents for nucleic acid extraction. Employing two different release frequencies for the stick-packaged liquid reagents enables on-demand release of highly wetting extraction buffers, such as sequential release of lysis and binding buffer. Microfluidic process-flow was successful in 54 out of 55 tested LabDisks. We demonstrate successful detection of the respiratory pathogen influenza A H3N2 virus in a total of 18 LabDisks with sample concentrations down to 2.39 × 10
4
viral RNA copies per ml, which is in the range of clinical relevance. Furthermore, we detected RNA bacteriophage MS2 acting as internal control in 3 LabDisks with a sample concentration down to 75 plaque forming units (pfu) per ml. All experiments were applied in a 2 kg portable, laptop controlled point-of-care device. The turnaround time of the complete analysis from sample-to-answer was less than 3.5 hours.
Sample supply remains the only manual handling step for pathogen detection at the point-of-care. |
|---|---|
| AbstractList | Portable point-of-care devices for pathogen detection require easy, minimal and user-friendly handling steps and need to have the same diagnostic performance compared to centralized laboratories. In this work we present a fully automated sample-to-answer detection of influenza A H3N2 virus in a centrifugal LabDisk with complete prestorage of reagents. Thus, the initial supply of the sample remains the only manual handling step. The self-contained LabDisk automates by centrifugal microfluidics all necessary process chains for PCR-based pathogen detection: pathogen lysis, magnetic bead based nucleic acid extraction, aliquoting of the eluate into 8 reaction cavities, and real-time reverse transcription polymerase chain reaction (RT-PCR). Prestored reagents comprise air dried specific primers and fluorescence probes, lyophilized RT-PCR mastermix and stick-packaged liquid reagents for nucleic acid extraction. Employing two different release frequencies for the stick-packaged liquid reagents enables on-demand release of highly wetting extraction buffers, such as sequential release of lysis and binding buffer. Microfluidic process-flow was successful in 54 out of 55 tested LabDisks. We demonstrate successful detection of the respiratory pathogen influenza A H3N2 virus in a total of 18 LabDisks with sample concentrations down to 2.39 × 10
4
viral RNA copies per ml, which is in the range of clinical relevance. Furthermore, we detected RNA bacteriophage MS2 acting as internal control in 3 LabDisks with a sample concentration down to 75 plaque forming units (pfu) per ml. All experiments were applied in a 2 kg portable, laptop controlled point-of-care device. The turnaround time of the complete analysis from sample-to-answer was less than 3.5 hours.
Sample supply remains the only manual handling step for pathogen detection at the point-of-care. |
| Author | Baumann, D Hutzenlaub, T von Stetten, F Stumpf, F Simons, G Dingemanns, G Zengerle, R Strohmeier, O Plobner, L Sager, C Mark, D Schwemmer, F |
| AuthorAffiliation | Hahn-Schickard Agrobiogen GmbH Biotechnologie BIOSS - Centre for Biological Signalling Studies University of Freiburg Dr. Stein and colleagues Laboratory for MEMS Applications Medical Care Center PathoFinder B.V IMTEK - Department of Microsystems Engineering |
| AuthorAffiliation_xml | – name: Dr. Stein and colleagues – name: Hahn-Schickard – name: PathoFinder B.V – name: Laboratory for MEMS Applications – name: BIOSS - Centre for Biological Signalling Studies – name: Medical Care Center – name: University of Freiburg – name: Agrobiogen GmbH Biotechnologie – name: IMTEK - Department of Microsystems Engineering |
| Author_xml | – sequence: 1 givenname: F surname: Stumpf fullname: Stumpf, F – sequence: 2 givenname: F surname: Schwemmer fullname: Schwemmer, F – sequence: 3 givenname: T surname: Hutzenlaub fullname: Hutzenlaub, T – sequence: 4 givenname: D surname: Baumann fullname: Baumann, D – sequence: 5 givenname: O surname: Strohmeier fullname: Strohmeier, O – sequence: 6 givenname: G surname: Dingemanns fullname: Dingemanns, G – sequence: 7 givenname: G surname: Simons fullname: Simons, G – sequence: 8 givenname: C surname: Sager fullname: Sager, C – sequence: 9 givenname: L surname: Plobner fullname: Plobner, L – sequence: 10 givenname: F surname: von Stetten fullname: von Stetten, F – sequence: 11 givenname: R surname: Zengerle fullname: Zengerle, R – sequence: 12 givenname: D surname: Mark fullname: Mark, D |
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| Title | LabDisk with complete reagent prestorage for sample-to-answer nucleic acid based detection of respiratory pathogens verified with influenza A H3N2 virusElectronic supplementary information (ESI) available: Details of respiratory qPCR panels and rotational frequency protocol. See DOI: 10.1039/c5lc00871a |
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