A Thermally Responsive Phospholipid Pseudogel: Tunable DNA Sieving with Capillary Electrophoresis

Durney, Brandon C.; Lounsbury, Jenny A.; Poe, Brian L.; Landers, James P.; Holland, Lisa

doi:10.1021/ac303745g

Cited by 24 publications

(37 citation statements)

References 66 publications

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“…Aqueous solutions of the longchain phospholipid dimyristoyl-sn-glycero-3-phosphocholine (DMPC) and the short-chain phospholipid 1,2-dihexanoyl-snglycero-3-phosphocholine (DHPC) are known to form wormlike micelles [19,20]. A dynamic sieving matrix of 10% phospholipid with [DMPC]/[DHPC] = 2.5 was optimized for single-base pair resolution that was adequate for detection of short tandem repeats (STR) in selected loci utilized for human identification using a 100 cm long capillary within a 30 min run time [21]. This is comparable to separations on commercial capillary electrophoresis instruments for forensic STR analyses [22].…”

Section: Introductionmentioning

confidence: 99%

Reversible phospholipid nanogels for deoxyribonucleic acid fragment size determinations up to 1500 base pairs and integrated sample stacking

Durney

Bachert

Sloane

et al. 2015

Analytica Chimica Acta

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Phospholipid additives are a cost-effective medium to separate deoxyribonucleic acid (DNA) fragments and possess a thermally-responsive viscosity. This provides a mechanism to easily create and replace a highly viscous nanogel in a narrow bore capillary with only a 10°C change in temperature. Preparations composed of dimyristoyl-sn-glycero-3-phosphocholine (DMPC) and 1,2-dihexanoyl-sn-glycero-3-phosphocholine (DHPC) self-assemble, forming structures such as nanodisks and wormlike micelles. Factors that influence the morphology of a particular DMPC-DHPC preparation include the concentration of lipid in solution, the temperature, and the ratio of DMPC and DHPC. It has previously been established that an aqueous solution containing 10% phospholipid with a ratio of [DMPC]/[DHPC]=2.5 separates DNA fragments with nearly single base resolution for DNA fragments up to 500 base pairs in length, but beyond this size the resolution decreases dramatically. A new DMPC-DHPC medium is developed to effectively separate and size DNA fragments up to 1500 base pairs by decreasing the total lipid concentration to 2.5%. A 2.5% phospholipid nanogel generates a resolution of 1% of the DNA fragment size up to 1500 base pairs. This increase in the upper size limit is accomplished using commercially available phospholipids at an even lower material cost than is achieved with the 10% preparation. The separation additive is used to evaluate size markers ranging between 200 and 1500 base pairs in order to distinguish invasive strains of Streptococcus pyogenes and Aspergillus species by harnessing differences in gene sequences of collagen-like proteins in these organisms. For the first time, a reversible stacking gel is integrated in a capillary sieving separation by utilizing the thermally-responsive viscosity of these self-assembled phospholipid preparations. A discontinuous matrix is created that is composed of a cartridge of highly viscous phospholipid assimilated into a separation matrix of low viscosity. DNA sample stacking is facilitated with longer injection times without sacrificing separation efficiency.

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Section: Introductionmentioning

confidence: 99%

Reversible phospholipid nanogels for deoxyribonucleic acid fragment size determinations up to 1500 base pairs and integrated sample stacking

Durney

Bachert

Sloane

et al. 2015

Analytica Chimica Acta

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show abstract

“…Linear gels are viscous additives that provide good separation performance and do not need to be polymerized in the capillary. Issues associated with the introduction of highly viscous materials into narrow-bore capillaries have spawned the use of thermally reversible sieving materials (76)(77)(78), including phospholipid nanogels (36). These materials are introduced into the capillary at a temperature that generates low viscosity and then converted into a highly viscous separation additive in the capillary by changing the separation temperature.…”

Section: CLmentioning

confidence: 99%

“…Sieving is then accomplished at 30°C. Separations performed under conditions that do not denature DNA provided nearly single-base resolution of short tandem repeats relevant to human identification (36).…”

Section: CLmentioning

confidence: 99%

“…The accuracy of size standardization is a function of the size of the DNA separated, the available standard size, and the applied voltage. The size range of the measurement affects accuracy, as the DNA migration is linear (i.e., in Ogston sieving) up to ϳ450 bp (36). DNA fragments larger than this undergo reptation-based transport.…”

Section: CLmentioning

confidence: 99%

“…If the precision of the size determination is not critical, capillary nanogel separations can be obtained in shorter separation times (ϳ5 to 10 min) than those shown in Fig. 2C and 4B and yet still yield baseline resolution of the DNA fragments (36).…”

Section: CLmentioning

confidence: 99%

See 2 more Smart Citations

Aspergillus Collagen-Like Genes ( acl ): Identification, Sequence Polymorphism, and Assessment for PCR-Based Pathogen Detection

Tuntevski

Durney

Snyder

et al. 2013

Appl Environ Microbiol

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fThe genus Aspergillus is a burden to public health due to its ubiquitous presence in the environment, its production of allergens, and wide demographic susceptibility among cystic fibrosis, asthmatic, and immunosuppressed patients. Current methods of detection of Aspergillus colonization and infection rely on lengthy morphological characterization or nonstandardized serological assays that are restricted to identifying a fungal etiology. Collagen-like genes have been shown to exhibit species-specific conservation across the noncollagenous regions as well as strain-specific polymorphism in the collagen-like regions. Here we assess the conserved region of the Aspergillus collagen-like (acl) genes and explore the application of PCR amplicon size-based discrimination among the five most common etiologic species of the Aspergillus genus, including Aspergillus fumigatus, A. flavus, A. nidulans, A. niger, and A. terreus. Genetic polymorphism and phylogenetic analysis of the aclF1 gene were additionally examined among the available strains. Furthermore, the applicability of the PCR-based assay to identification of these five species in cultures derived from sputum and bronchoalveolar fluid from 19 clinical samples was explored. Application of capillary electrophoresis on nanogels was additionally demonstrated to improve the discrimination between Aspergillus species. Overall, this study demonstrated that Aspergillus acl genes could be used as PCR targets to discriminate between clinically relevant Aspergillus species. Future studies aim to utilize the detection of Aspergillus acl genes in PCR and microfluidic applications to determine the sensitivity and specificity for the identification of Aspergillus colonization and invasive aspergillosis in immunocompromised subjects.

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Harnessing Joule heating in microfluidic thermal gel electrophoresis to create reversible barriers for cell enrichment

Cornejo

Linz

2021

Electrophoresis

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Gel electrophoresis is a ubiquitous bioanalytical technique used to characterize the components of cell lysates. However, analyses of bulk lysates sacrifice detection sensitivity because intracellular biomolecules become diluted, and the liberation of proteases and nucleases can degrade target analytes. This report describes a method to enrich cells directly within a microfluidic gel as a first step toward online measurement of trace intracellular biomolecules with minimal dilution and degradation. Thermal gels were employed as the gel matrix because they can be reversibly converted between liquid and solid phases as a function of temperature. Rather than fabricate costly heating elements into devices to control temperature—and thus the phase of the gel—Joule heating was used instead. Adjoining regions of liquid‐phase and solid‐phase gel were formed within microfluidic channels by selectively inducing localized Joule heat. Cells migrated through the liquid gel but could not enter the solid gel—accumulating at the liquid–solid gel boundary—whereas small molecule contaminants passed through to waste. Barriers were then liquified on‐demand by removing Joule heat to collect the purified, non‐lysed cells for downstream analyses. Using voltage‐controlled Joule heating to regulate the phase of thermal gels is an innovative approach to facilitate in‐gel cell enrichment in low‐cost microfluidic devices.

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A Thermally Responsive Phospholipid Pseudogel: Tunable DNA Sieving with Capillary Electrophoresis

Cited by 24 publications

References 66 publications

Reversible phospholipid nanogels for deoxyribonucleic acid fragment size determinations up to 1500 base pairs and integrated sample stacking

Reversible phospholipid nanogels for deoxyribonucleic acid fragment size determinations up to 1500 base pairs and integrated sample stacking

Aspergillus Collagen-Like Genes ( acl ): Identification, Sequence Polymorphism, and Assessment for PCR-Based Pathogen Detection

Harnessing Joule heating in microfluidic thermal gel electrophoresis to create reversible barriers for cell enrichment

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