A disposable laser print-cut-laminate polyester microchip for multiplexed PCR via infra-red-mediated thermal control |
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| Authors: | Yiwen Ouyang Gabriela R.M. Duarte Brian L. Poe Paul S. Riehl Fernando M. dos Santos Claudia C.G. Martin-Didonet Emanuel Carrilho James P. Landers |
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| Affiliation: | 1. Department of Chemistry, University of Virginia, Charlottesville, VA 22904, USA;2. Department of Mechanical Engineering, University of Virginia, Charlottesville, VA 22904, USA;3. Department of Pathology, University of Virginia Health Science Center, Charlottesville, VA, USA;4. Universidade Federal de Goiás, Goiânia, GO 74690-900, Brazil;5. Universidade Estadual de Goiás, Anápolis, GO 75132-400, Brazil;6. Instituto de Química de São Carlos, Universidade de São Paulo, São Carlos, SP 13566-590, Brazil;g Instituto Nacional de Ciência e Tecnologia de Bioanalítica, CP 6154, Campinas, SP 13083-970, Brazil |
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| Abstract: | Infrared (IR)-mediated thermal cycling system, a method proven to be a effective for sub-μL scale polymerase chain reaction (PCR) on microchips, has been integrated with DNA extraction and separation on a glass microchip in a fully integrated micro Total Analysis System by Easley et al., in 2006. IR-PCR has been demonstrated on both glass and PMMA microdevices where the fabrication (bonding) is not trivial. Polyester-toner (PeT) microfluidic devices have significant potential as cost-effective, disposable microdevices as a result of the ease of fabrication (∼$0.25 USD and <10 min per device) and availability of commercial substrates. For the first time, we demonstrate here the thermal cycling in PeT microchips on the IR-PCR system. Undesirable IR absorption by the black-toner bonding layer was eliminated with a spatial filter in the form of an aluminum foil mask. The solution heating rate for a black PeT microchip using a tungsten lamp was 10.1 ± 0.7 °C s−1 with a cooling rate of roughly −12 ± 0.9 °C s−1 assisted by forced air cooling. Dynamic surface passivation strategies allowed the successful amplification of a 520 bp fragment of the λ-phage genome (in 11 min) and a 1500 bp region of Azospirillum brasilense. Using a centrosymmetric chamber configuration in a multichamber PeT microchip, homogenous temperature distribution over all chambers was achieved with inter-chamber temperature differences at annealing, extension and denaturing steps of less than ±2 °C. The effectiveness of the multichamber system was demonstrated with the simultaneous amplification of a 390 bp amplicon of human β-globin gene in five PeT PCR microchambers. The relative PCR amplification efficiency with a human β-globin DNA fragment ranged from 70% to 90%, in comparison to conventional thermal cyclers, with an inter-chamber standard deviation of ∼10%. Development of PeT microchips for IR-PCR has the potential to provide rapid, low-volume amplification while also integrating PCR with extraction upstream and separation/detection downstream. |
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| Keywords: | Polyester-toner chip IR-PCR Multichamber chips Disposable chips Low-cost genetic analyzer |
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