Investigation of the effect of antifolates on Escherichia coli 1810

Eumkeb, Griangsak

January 1999

No description available.

579

Gel electrophoresis; Viable counts

Aspects of the biology of deep-sea anthozoa

Bronsdon, Sarah Kirstin

January 1997

No description available.

551.46

An evaluation of the chemosensitivity of superficial bladder cancer using the comet assay

Walsh, Ian Kinsella

January 1997

No description available.

610

Studies on the separation behaviour of nucleotides and oligonucleotides

McKeown, Alan Patrick

January 1999

No description available.

572

The effect of alien germplasm on 2M urea-soluble protein electrophoresis

Chavez, Elyzabeth

January 2011

Digitized by Kansas Correctional Industries

Grain--Analysis

Proteins--Analysis

Electrophoresis

Capillary electrophoresis of proteins with selective on-line affinity monoliths /

Armenta Blanco, Jenny Marcela,

January 2006

Thesis (Ph. D.)--Brigham Young University. Dept. of Chemistry and Biochemistry, 2006. / Includes bibliographical references.

Characterization of protein expression in breast cancer tissues by one and two-dimensional capillary electrophoresis /

Harwood, Melissa M.

January 2006

Thesis (Ph. D.)--University of Washington, 2006. / Vita. Includes bibliographical references (leaves 266-277).

A proteomic study of Pseudomonas putida by two-dimensional gel electrophoresis : establishing quantitative standards for intra-laboratory results /

Fowlkes, Kelly.

January 2007

Thesis (M.S.)--Rochester Institute of Technology, 2007. / Typescript. Includes bibliographical references (leaves 66-68).

A microfluidic device for continuous capture and concentration of pathogens from water

Balasubramanian, Ashwin Kumar

15 May 2009

A microfluidic device, based on electrophoretic transport and electrostatic trapping of charged particles, has been developed for continuous capture and concentration of microorganisms from water. A generic design, utilizing mobility and zeta potential measurements of various microorganisms exposed to different environmental conditions and physiological states, was employed. Water and buffer samples at pH values ranging from 5.2–7.0 were seeded with bacteria (E. coli, Salmonella, and Pseudomonas) and viruses (MS-2 and Echovirus). Negative control and capture experiments were performed simultaneously using two identical devices. Both culture based methods and real-time PCR analysis were utilized to characterize the capture efficiency as a function of time, flowrate, and applied electric field. Based on differences between the capture and negative control data, capture efficiencies of 90% to 99% are reported for E. coli, Salmonella, Pseudomonas, and MS-2, while the capture efficiency for Echovirus was around 75%. Overall, the device exhibits 16.67 fold sample volume reduction within an hour at 6 mL/hr. This results in a concentration factor of 15 at 90% capture efficiency. Direct quantification of capture on the anode of the prototype microfluidic device was also performed by particle tracking using fluorescent microscopy. Based on image processing, the capture data at different locations on the electrode surface is quantified as a function of the wall shear stress at these locations, which is calculated using CFD simulations. Finally, the Faradaic processes in the microchannel due to electrochemical reactions are studied to predict the amount of electrophoresis in the system. Scaling of the device to sample 5 L/hr can be achieved by stacking 835 identical microchannels. Power and wetted volume for the prototype and scaled devices are presented. The device can thus function either as a filtration unit or as a sample concentrator to enable the application of real-time detection sensor technologies. The ability to continuously sample water without chemical additives facilitates the use of this device in drinking water distribution systems. This work constitutes the first step in our development of a continuous, microbial capture and concentration system from large volumes of potable water.

Pathogens

Concentration

Microfluidic

Capture

Electrophoresis

Novel devices for analytical-scale isoelectric trapping separations

Lim, Peniel Jason

2006 December 1900

Isoelectric trapping (IET), has proven to be one of the most successful electrophoretic techniques used for separations of ampholytic compounds. IET is carried out in multicompartment electrolyzers (MCEs) in which adjacent compartments are joined through buffering membranes whose pH values bracket the pI of the ampholytic component to be trapped in the compartment. The present small-scale instruments use plastics as their structural materials, which causes poor Joule heat dissipation. The separation compartments have cylindrical or pear-shaped interiors with large internal diameters, which create long heat transfer paths. The long electrode distances yield low field strengths that lead to low electrophoretic velocities for the analytes. These factors interrelatedly limit the electric power that can be applied to the system, contributing to long separation times. Furthermore, these devices do not offer a realistic solution to the problems associated with the detection of low abundance proteins. To address these problems, two novel IET devices have been developed for small-scale IET separations. The first device, named MSWIFT, was constructed using thermally conductive, high-purity alumina as the structural material of the separation compartments. By creating narrow, 0.1- or 0.2-mL channels in thin alumina blocks, the heat transfer path from the center of the compartment to the wall was significantly decreased; and the distance between electrodes was greatly shortened. MSWIFT achieved 6 to 50 times faster IET separations compared to other MCEs. The second device, named ConFrac, was developed to simultaneously fractionate and concentrate ampholytic components from a complex sample into 0.1-mL collection compartments. By designing a system with a 2-dimensional pH gradient and allowing recirculation of the sample feed, the ConFrac demonstrated enrichment of analytes by a factor of 100 and greater.

Protein

Electrophoresis

Device

Isoelectric

Separation