Design and fabrication of a microfluidic device for near-single cell mRNA isolation using a copper hot embossing master

Nugen, Sam R.; Asiello, Peter J.; Baeumner, Antje J.

doi:10.1007/s00542-008-0694-0

Cited by 30 publications

(25 citation statements)

References 19 publications

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“…25 The copper template was fabricated at the Cornell Nanoscale Facility (CNF) via photolithography using KMPR 1050 (Micro-Chem Corp., MA) and copper electroplating resulting in elevated channel structures. A 5×5cm piece of PMMA was sandwiched between the copper template and a blank copper plate, and using a hot press (CarverLaminating), the PMMA was patterned at 130°C and 8000 lbs.…”

Section: Experimental Methodsmentioning

confidence: 99%

Isolation and Amplification of mRNA within a Simple Microfluidic Lab on a Chip

et al. 2013

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The major modules for realizing molecular biological assays in a micro total analysis system (μTAS) were developed for the detection of pathogenic organisms. The specific focus was the isolation and amplification of eukaryotic messenger RNA (mRNA) within a simple, single-channel device for very low RNA concentrations that could then be integrated with detection modules. The hsp70 mRNA from Cryptosporidium parvum was used as a model analyte. Important points of study were surface chemistries within poly(methyl methacrylate) (PMMA) microfluidic channels that enabled specific and sensitive mRNA isolation and amplification reactions for very low mRNA concentrations. Optimal conditions were achieved when the channel surface was carboxylated via UV/ozone treatment followed by the immobilization of polyamidoamine (PAMAM) dendrimers on the surface, thus increasing the immobilization efficiency of the thymidine oligonucleotide, oligo(dT)25, and providing a reliable surface for the amplification reaction, importantly, without the need for blocking agents. Additional chemical modifications of the remaining active surface groups were studied to avoid non-specific capturing of nucleic acids and hindering of the mRNA amplification at low RNA concentrations. Amplification of the mRNA was accomplished using nucleic acid sequence-based amplification (NASBA), an isothermal, primer-dependent technique. Positive controls consisting of previously generated NASBA amplicons could be diluted 1015 fold and still result in successful on-chip re-amplification. Finally, the successful isolation and amplification of mRNA from as few as 30 C. parvum oocysts was demonstrated directly on-chip and compared to bench-top devices. This is the first proof of successful mRNA isolation and NASBA-based amplification of mRNA within a simple microfluidic device in relevant analytical volumes.

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Section: Experimental Methodsmentioning

confidence: 99%

Isolation and Amplification of mRNA within a Simple Microfluidic Lab on a Chip

et al. 2013

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“…The patterned substrate is then cooled to room temperature and developed for ten minutes in SU-8 developer under manual agitation. [2] Electroplating: Once the SU-8 micropatterned copper substrate (Fig. 1a) has been manufactured copper electroplating is performed to create raised microchannel structures on the copper substrate.…”

Section: A Microfluidic Device Fabricationmentioning

confidence: 99%

Quantum dot-linked immunoassay on a PMMA-based microfluidic device for biomarker detection

Hansberry

Clark

2012

2012 38th Annual Northeast Bioengineering Conference (NEBEC)

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Immunoassay and biosensor development are burgeoning research fields with high translational impact potential due to the high demand for reliable biomarker detection. While needs are diverse and based on application, it is generally desirable to have an immunoassay that is rapid, robust, and easy to use. In order to meet those needs, our group has developed a quantum dot-linked immunoassay with a PMMAbased microfluidic substrate that is capable of detecting a variety of biomarkers. We developed a PMMA microfluidic using photlithography, electroplating, and hot embossing techniques. This novel technology uses an ELISA-like sandwich to capture biomarkers in an antibody -antigen -anti-antigen antibody complex. Specifically, we use a diamino poly(ethylene glycol), glutaraldehyde crosslinking combination to covalently immobilize primary antibody in combination with a quantum dotstreptavidin-biotin conjugated secondary antibody, which is quantified through an ultraviolet light emitting diode and charged-couple device camera setup. Our ultimate goal is to detect physiologically relevant biomarkers to better help physicians diagnose and treat their patients.

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“…Microfluidic channels can be formed in substrates such as PMMA using laser ablation (Conlisk et al 2011;Hong et al 2010;Klank et al 2002), hot embossing (Nugen et al 2008) or injection molding (Zhou et al 2005). Laser ablation allows for rapid prototyping as opposed to other methods which require machining of a mold.…”

Section: Introductionmentioning

confidence: 99%

Development and characterization of a capillary-flow microfluidic device for nucleic acid detection

Jin

Dai

et al. 2012

Microsyst Technol

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We have developed a capillary flow-driven microfluidic biosensor to meet the needs of diagnostics for resource-limited areas. The device combined elements of lateral flow assays and microfluidic technology resulting in a hybrid with benefits of both formats. The biosensor was achieved by bonding two pieces of polymethyl methacrylate with channels ablated by a CO 2 laser, and enclosing an absorbent pad. The channels were UV/ozone treated to increase hydrophilicity which enabled capillary flow. The absorbent pad allowed for continuous flow in the channels once filled. The application of biosensor was demonstrated by detection of DNA with a sandwich assay. The target DNA was hybridized with nucleic acid modified magnetic beads as well as Ru(bpy) 3 2? doped silica nanoparticles. Fluorescent signals were quantified in a holder fabricated to fit in a fluorescent microtiter plate reader. The capillary flow microfluidic was capable to detect 1 pmol target. The assay format which features rapid analysis and does not require the use of pumps could allow for inexpensive point of care diagnostics in the future.

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Design and fabrication of a microfluidic device for near-single cell mRNA isolation using a copper hot embossing master

Cited by 30 publications

References 19 publications

Isolation and Amplification of mRNA within a Simple Microfluidic Lab on a Chip

Isolation and Amplification of mRNA within a Simple Microfluidic Lab on a Chip

Quantum dot-linked immunoassay on a PMMA-based microfluidic device for biomarker detection

Development and characterization of a capillary-flow microfluidic device for nucleic acid detection

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