Rapid pathogen detection using a microchip PCR array instrument

Belgrader, Phillip; Benett, William J.; Hadley, Dean R.; Long, Gary W.; Mariella, Raymond P.; Milanovich, Fred P.; Nasarabadi, Shanavaz; Nelson, W. John; Richards, James B.; Stratton, Paul

doi:10.1093/clinchem/44.10.2191

Cited by 150 publications

(58 citation statements)

References 15 publications

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“…In addition, MS2 bacteriophages have previously been used a surrogate for poliovirus and many other enteric viruses due to similarity of their characteristics. Several investigators utilized MS2 as a simulant of pathogenic viral strains (Belgrader et al, 1998;Alvarez et al, 2000;Shin and Sobsey, 2003;Thomas et al, 2004;Tseng and Li, 2005b). The MS2 bacteriophage stock solution was prepared from a freeze-dried phage stock vial (ATCC 15597-B1) by adding 9 ml of Luria-Bertani broth, which had been made using ultra-filtered deionized water.…”

Section: Test Particlesmentioning

confidence: 99%

Physical Collection Efficiency of Filter Materials for Bacteria and Viruses

Burton

Grinshpun

Reponen

2006

The Annals of Occupational Hygiene

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The purpose of this study was to determine the physical collection efficiency of commercially available filters for collecting airborne bacteria, viruses, and other particles in the 10-900 nm (nanometer) size range. Laboratory experiments with various polytetrafluoroethylene (PTFE), polycarbonate (PC) and gelatin filters in conjunction with Button Inhalable samplers and three-piece cassettes were undertaken. Both biological and non-biological test aerosols were used: Bacillus atrophaeus, MS2, polystyrene latex (PSL), and sodium chloride (NaCl). The B.atrophaeus endospores had an aerodynamic diameter of 900 nm, whereas MS2 virion particles ranged from 10 to 80 nm. Monodisperse 350 nm PSL particles were used as this size was believed to have the lowest filtration efficiency. NaCl solution (1% weight by volume) was used to create a polydisperse aerosol in the 10-600 nm range. The physical collection efficiency was determined by measuring particle concentrations size-selectively upstream and downstream of the filters. The PTFE and gelatin filters showed excellent collection efficiency (>93%) for all of the test particles. The PC filters showed lower collection efficiency for small particles especially <100 nm. Among the tested filters, the lowest collection efficiencies, 49 and 22%, were observed for 1 and 3-microm pore size PC filters at the particle sizes of 47 and 63 nm, respectively. The results indicate that the effect of filter material is more significant for the size range of single virions than for bacteria. The effect of filter loading was examined by exposing filters to mixtures of PSL particles, which aimed at mimicking typical indoor dust levels and size distributions. A 4-h loading did not cause significant change in the physical collection efficiency of the tested filters.

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Section: Test Particlesmentioning

confidence: 99%

Physical Collection Efficiency of Filter Materials for Bacteria and Viruses

Burton

Grinshpun

Reponen

2006

The Annals of Occupational Hygiene

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“…4 As a result of the poor purication of template DNA, primer-template mismatches, spontaneous formation of primer dimers, and non-optimized PCRmixture ratio and thermocycling conditions, the formation of the target amplicon may be accompanied by non-specic side products called PCR artifacts. To x this problem, several enhancers have been introduced: (1) various additives in PCR mixture, such as betaine, 5 dithiothreitol, 6 dimethyl sulfoxide, 7 single-stranded DNA-binding protein (SSB); 8 (2) instrumental design, including development of thermocyclers with precise heating/cooling rates; 9,10 (3) optimization of PCR system through optimal Mg 2+ concentration, cycle numbers and proper primer design; [11][12][13] (4) enzyme modication; 14,15 and (5) new touchdown 16 and nested 17 PCR strategies. Although these tools improve the PCR outcome, yet they are not all-purpose and the optimization protocol can be case dependent.…”

Section: Introductionmentioning

confidence: 99%

Gold nanoparticle-assisted polymerase chain reaction: effects of surface ligands, nanoparticle shape and material

et al. 2016

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“…The time required to complete the assay was only 3 hours. Recent development of thermocyclers and spectrofluorometers that use silicon chips has reduced the size of the instrumentation needed and permitted assays to be completed even faster—in only a few minutes 31,32 . Thus, the assay provides both the speed and extreme sensitivity that might be suitable for detecting the small numbers of bacteria thought to contaminate blood during the initial days of storage.…”

Section: Discussionmentioning

confidence: 99%