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Automated microfluidic device reduces time to screen small organisms for genetic studies
June 24, 2008
Genetic studies on small organisms such as worms and flies can now be done more quickly using a new microfluidic device developed by engineers at the Georgia Institute of Technology. The new "lab-on-a-chip" can automatically position, image, determine the phenotype of and sort small animals, such as the worm Caenorhabditis elegans that is commonly used for biological studies.
"Classical genetic approaches require altering genetic information and monitoring changes in a large number of animals, which can be excruciatingly slow and often requires manual manipulations," said Hang Lu, an assistant professor in Georgia Tech School of Chemical and Biomolecular Engineering. "As researchers move from studying single genes to analyzing interactions and networks, studies that require large sample sizes will be critical and this device allows for consistent and reliable operation to rapidly screen many animals."
In the July print issue of the journal Nature Methods, available online June 22, Lu and graduate students Kwanghun Chung and Matthew Crane describe their automated microsystem and initial experimental results. The results show that they can sort small organisms without human intervention based on cellular and subcellular features, or traits, with a high degree of accuracy at a rate of several hundred animals per hour. This work was funded by the National Science Foundation and the National Institutes of Health.
Using the microfluidic system is simple. Each small animal is automatically loaded into the microchip. The setup automatically arranges each organism in an identical position in the chip to reduce the processing time and increase throughput.
Once the organism is loaded, it is briefly immobilized by an integrated local temperature control system that cools the animal to approximate four degrees Celsius. Cooling effectively stops the animal's motion and allows repeated imaging of the same organisms because unlike commonly-used anesthetic drugs, the cooling doesn't have long-term effects.
After cooling, the system uses a high-resolution microscope to acquire multi-dimensional images of the animal on-chip.
"The advantage of using our microchip is that it's completely compatible with any standard microscope you'd find in a biology laboratory - epifluorescence, stereo, multi-photon or confocal - with no modification required," explained Lu.
The researchers have shown that the intensity and patterns of fluorescent markers imaged inside cooled animals versus those in anesthetized animals exhibit no discernible differences. Based on each animal's phenotype, or how each animal looks under the microscope, the computer identifies whether it is wild-type or mutant and sorts it into the appropriate group.
Initial tests to assess the system were conducted on C. elegans, one of the tiniest multi-cellular organisms that share many fundamental cellular/molecular mechanisms with more advanced organisms. However, the automated system can also be adapted to study other small organisms such as fruit flies and fish embryos.
For one experiment, Lu and her team tested the ability of the system to analyze the gene expression pattern - the intensity, location and timing of appearance of a fluorescent protein - in a population of organisms. They were able to sort the free-moving animals into two categories, those fluorescing in a particle neuron and those that are not, at a speed of approximately 900 animals per hour. More than 90 percent of the animals were loaded into the observation chamber within 0.3 seconds after the previous animal exited.
In another experiment, the researchers were successful in separating a small number of mutant animals from a large population of wild-type animals based on the fluorescence in a single pair of neurons. With on-line processing and decision-making without human supervision, the system achieved a sorting speed of approximately 150 animals per hour and a false negative rate of less than 0.2 percent, indicating that almost all the mutants were captured by the system.
A third experiment was aimed at demonstrating the ability of the system to screen organisms based on micro-sized synaptic features of the animals. Results showed that the system was able to sort mixed populations at a rate of approximately 400 animals per hour for this application. In all three experiments, it would have taken researchers much longer to identify the worms manually with high-resolution microscopy a few worms at a time.
"This is the first automated device to combine high-resolution imaging with automated sorting of the worms." added Lu. "Now that we have the automated system, we are able to perform genetic screens a lot faster than what has traditionally been done and speed up the discovery of new genes, new functions and new pathways."
Georgia Institute of Technology Research News
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Optofluidics: Fundamentals, Devices, and Applications (Biophotonics)
by Yeshaiahu Fainman (Author), Luke Lee (Author), Demetri Psaltis (Author), Changhuei Yang (Author)
Cutting-Edge Optofluidics Theories, Techniques, and Practices Add novel functionalities to your optical design projects by incorporating state-of-the-art microfluidic technologies and tools. Co-written by industry experts, Optofluidics: Fundamentals, Devices, and Applications covers the latest functional integration of optical devices and microfluidics, as well as automation techniques. This authoritative guide explains how to fabricate optical lab-on-a-chip devices, synthesize photonic crystals, develop solid and liquid core waveguides, use fluidic self-assembly methods, and accomplish direct microfabrication in solutions. The book includes details on developing biological sensors and arrays, handling maskless lithography, designing high-Q cavities, and working with...
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Rapid discrimination of single-nucleotide mismatches using a microfluidic device with monolayered beads [An article from: Analytica Chimica Acta]
by J.K.K. Ng (Author), H. Feng (Author), W.T. Liu (Author)
This digital document is a journal article from Analytica Chimica Acta, published by Elsevier in 2007. The article is delivered in HTML format and is available in your Amazon.com Media Library immediately after purchase. You can view it with any web browser.
Description: A microfluidic device incorporating monolayered beads is developed for the discrimination of single-nucleotide mismatches, based on the differential dissociation kinetics between perfect match (PM) and mismatched (MM) duplexes. The monolayered beads are used as solid support for the immobilization of oligonucleotide probes containing a single-base variation. Target oligonucleotides hybridize to the probes, forming either PM duplexes or MM duplexes containing a single mismatch. Optimization studies show that PM...
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From the author: Real-time process monitoring of the fabrication process of microfluidic devices using a polymer injection molding machine was carried out using miniature ultrasonic probes. A thick piezoelectric lead-zirconate-titanate film as an ultrasonic transducer (UT) was fabricated onto one end of a 4-mm diameter and 12-mm long steel buffer rods using a sol gel spray technique....
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Continuous flow microfluidic device for cell separation, cell lysis and DNA purification [An article from: Analytica Chimica Acta]
by X. Chen (Author), D. Cui (Author), C. Liu (Author), H. Li (Author), J. Chen (Author)
This digital document is a journal article from Analytica Chimica Acta, published by Elsevier in 2007. The article is delivered in HTML format and is available in your Amazon.com Media Library immediately after purchase. You can view it with any web browser.
Description: A novel integrated microfluidic device that consisted of microfilter, micromixer, micropillar array, microweir, microchannel, microchamber, and porous matrix was developed to perform sample pre-treatment of whole blood. Cell separation, cell lysis and DNA purification were performed in this miniaturized device during a continuous flow process. Crossflow filtration was proposed to separate blood cells, which could successfully avoid clogging or jamming. After blood cells were lyzed in guanidine buffer, genomic...
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Microfluidic Devices in Nanotechnology: Current Status and a Future Perspective
by Challa S. S. R. Kumar (Author)
Nanotechnology, especially microfabrication, has been affecting every facet of traditional scientific disciplines. The first book on the application of microfluidic reactors in nanotechnology, Microfluidic Devices in Nanotechnology provides the fundamental aspects and potential applications of microfluidic devices, the physics of microfluids, specific methods of chemical synthesis of nanomaterials, and more. As the first book to discuss the unique properties and capabilities of these nanomaterials in the miniaturization of devices, this text serves as a one-stop resource for nanoscientists interested in microdevices.
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PNAS November 9, 2004: Reprogrammable Microfluidic Devices (Proceedings of the National Academy of Sciences, v. 101, # 45)
by National Academy of Sciences (Author)
pp. 15825-16082
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Microbial detection in microfluidic devices through dual staining of quantum dots-labeled immunoassay and RNA hybridization [An article from: Analytica Chimica Acta]
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This digital document is a journal article from Analytica Chimica Acta, published by Elsevier in 2006. The article is delivered in HTML format and is available in your Amazon.com Media Library immediately after purchase. You can view it with any web browser.
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The enhanced diffusional mixing for latex immunoagglutination assay in a microfluidic device [An article from: Analytica Chimica Acta]
by J.H. Han (Author), K.S. Kim (Author), J.Y. Yoon (Author)
This digital document is a journal article from Analytica Chimica Acta, published by Elsevier in 2007. The article is delivered in HTML format and is available in your Amazon.com Media Library immediately after purchase. You can view it with any web browser.
Description: Latex immunoagglutination assay in a microfluidic device is expected to be even easier than its large-sized, commercialized counterpart. However, such demonstration has had a limited success due to the difficulties in mixing in a microfluidic device, especially for the microparticles used in latex immunoagglutination assay. The primary goal of this work is to improve diffusional mixing towards the successful latex immunoagglutination in a microfluidic devices without any non-specific binding. To this end, SDS...
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Microfluidic Devices in Nanotechnology Part II
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This is the first book to discuss the developments in microfluidics coupled with nanotechnology. This approach is a revolutionary way for growing numbers of investigations to replace, in the future, conventional synthesis of nanomaterials and nanomaterials-based analytical methods by lab-on-a-chip systems combining micro fluidic devices with nanotechnology. Exciting applications range from chemistry, biology, molecular and cell biology, neuroscience, catalysis and nanomaterial’s synthesis.. With reviews by world-recognized microflluidic and nanotechnology experts, this authoritative work provides strong scaffolding for futuristic applications utilizing synergy from two powerful scientific elements.
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Integrated microfluidic devices [An article from: Analytica Chimica Acta]
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This digital document is a journal article from Analytica Chimica Acta, published by Elsevier in 2004. The article is delivered in HTML format and is available in your Amazon.com Media Library immediately after purchase. You can view it with any web browser.
Description: ''With the fundamentals of microscale flow and species transport well developed, the recent trend in microfluidics has been to work towards the development of integrated devices which incorporate multiple fluidic, electronic and mechanical components or chemical processes onto a single chip sized substrate. Along with this has been a major push towards portability and therefore a decreased reliance on external infrastructure (such as detection sensors, heaters or voltage sources).'' In this review we provide an...
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