Your search keyword '"Teneile M. Alfaro"' showing total 7 results

1. Development of a Rapid Viability RT-PCR (RV-RT-PCR) Method to Detect Infectious SARS-CoV-2 from Swabs

Author

Maher Elsheikh, Teneile M. Alfaro, Sanjiv Shah, and Staci R. Kane

Subjects

viral detection, Coronavirus disease 2019 (COVID-19), Reverse Transcriptase PCR, Transmission (medicine), medicine.drug_class, Reverse Transcriptase Polymerase Chain Reaction, SARS-CoV-2, Severe acute respiratory syndrome coronavirus 2 (SARS-CoV-2), viruses, COVID-19, Biology, Virology, Virus, Article, Reverse transcription polymerase chain reaction, rapid viability, Real-time polymerase chain reaction, infectious SARS-CoV-2, medicine, Humans, RNA, Viral, Antiviral drug, Incubation, Pandemics

Abstract

Since the rapid onset of the COVID-19 pandemic, its causative virus, Severe Acute Respiratory Syndrome Coronavirus-2 (SARS-CoV-2), continues to spread and increase the number of fatalities. To expedite studies on understanding potential surface transmission of the virus and to aid environmental epidemiological investigations, we developed a rapid viability reverse transcriptase PCR (RV-RT-PCR) method that detects viable (infectious) SARS-CoV-2 from swab samples in

Published

2021

2. Development of a rapid viability polymerase chain reaction method for detection of Yersinia pestis

Author

Sanjiv Shah, Teneile M. Alfaro, and Staci R. Kane

Subjects

Microbiology (medical), DNA, Bacterial, Yersinia pestis, Pcr assay, Microbiology, Genome, Polymerase Chain Reaction, Article, law.invention, 03 medical and health sciences, Plasmid, law, Humans, Molecular Biology, Gene, Polymerase chain reaction, 030304 developmental biology, DNA Primers, Disease Reservoirs, 0303 health sciences, Plague, biology, 030306 microbiology, Chemistry, biology.organism_classification, Method development, Water sample, Water Microbiology, Plasmids

Abstract

Due to the occurrence of natural plague outbreaks and its historical usage as a biological weapon, Yersinia pestis is considered one of the high-priority biological threat agents. It can remain viable in certain environments including water for >100 days. Because of its slow-growth characteristic, it usually takes three or more days to detect and confirm the identity of viable Y. pestis cells by PCR, serological, or biochemical assays when using the traditional microbiological plate-culture-based analysis, and that too, assuming faster growing microbes present in a water sample do not mask the Y. pestis colonies and interfere with analysis. Therefore, a rapid-viability Polymerase Chain Reaction (RV-PCR) method was developed for detection of Y. pestis. The RV-PCR method combines 24 h-incubation broth culture in a 48-well plate, and pre- and post-incubation differential PCR analyses, thereby allowing for rapid and high-throughput sample analysis compared with the current plate culture method. One chromosomal and two plasmid gene target-based real-time PCR assays were down-selected, showing ca. 10 genome equivalent detection; the chromosomal assay was then used for RV-PCR method development. A 101-cell level (10–99 cells) sensitivity of detection was demonstrated even with complex sample backgrounds including known PCR inhibitors (ferrous sulfate and humic acid), as well as metal oxides and microbes present in Arizona Test Dust (ATD). The method sensitivity was maintained in the presence of dead Y. pestis cells up to 104 cells per sample. While affording high-throughput and rapid sample analysis, the 48-well plate format used in this method for sample enrichment significantly reduced labor requirements and generation of BioSafety Level-3 (BSL-3) laboratory waste as compared to the usual microbiological plate-culture-based methods. This method may serve as a model for other vegetative bacterial pathogens.

Published

2019

3. Rapid viability polymerase chain reaction method for detection of Francisella tularensis

Author

Staci R. Kane, Teneile M. Alfaro, and Sanjiv Shah

Subjects

DNA, Bacterial, Microbiology (medical), Polymerase Chain Reaction, Microbiology, Article, law.invention, Tularemia, 03 medical and health sciences, chemistry.chemical_compound, law, medicine, Humans, Francisella tularensis, Molecular Biology, Polymerase chain reaction, 030304 developmental biology, 0303 health sciences, Growth medium, biology, 030306 microbiology, Chemistry, Infectious dose, medicine.disease, biology.organism_classification, Bioterrorism, Slow growth, Brain heart infusion, Water Microbiology, Biological Monitoring

Abstract

Francisella tularensis, which causes potentially fatal tularemia, has been considered an attractive agent of bioterrorism and biological warfare due to its low infectious dose, reported environmental persistence, and ability to be transmitted to humans via multiple exposure routes. Due to slow growth on even selective culture media, detection of viable F. tularensis from environmental and drinking water samples, usually takes > 3 days. Therefore, a rapid viability polymerase chain reaction (RV-PCR) method was developed to detect and identify viable F. tularensis cells in environmental samples. The method uses a change in PCR response during high throughput (48-well) sample incubation in Brain Heart Infusion/Vitox/Fildes/Histidine growth medium to detect viable F. tularensis presence, which is at least two times faster than the current plate culture-based method. Using the method, 10(1) to 10(2) live F. tularensis cells were detected in simulated complex sample matrices containing chemical and biological interferences.

Published

2019

4. Rapid, high-throughput, culture-based PCR methods to analyze samples for viable spores of Bacillus anthracis and its surrogates

Author

P.W. Krauter, R. Mahnke, Sonia E. Létant, Staci R. Kane, Tina C. Legler, Gloria A. Murphy, Ellen Raber, and Teneile M. Alfaro

Subjects

Microbiology (medical), Sample processing, Field tests, Polymerase Chain Reaction, Sensitivity and Specificity, Microbiology, Endospore, Automation, chemistry.chemical_compound, Food science, Molecular Biology, Spores, Bacterial, Bacteriological Techniques, Chlorine dioxide, Microbial Viability, biology, fungi, Significant difference, Oxides, biology.organism_classification, Spore, Bacillus anthracis, chemistry, Bacillus atrophaeus, Chlorine Compounds, Environmental Monitoring

Abstract

To rapidly remediate facilities after a biothreat agent release, improved turnaround times are needed for sample analysis. Current methods to confirm the presence of a viable biothreat agent are limited by low sample throughput. We have developed a rapid-viability-polymerase chain reaction (RV-PCR) method to determine the presence of viable spores. The method combines high-throughput sample processing with 96-well PCR analysis, which measures a change in real-time, quantitative PCR response arising from increased target-cell populations during culturing. The method accurately detects 1 to 10 live spores in a high-dead spore background (10(6)). Field tests using approximately 1000 biological indicators, each containing 10(6) spores of the B. anthracis surrogate, Bacillus atrophaeus, exposed to seven lethal and sub-lethal chlorine dioxide levels showed no significant difference (p0.05) between RV-PCR and standard culturing methods for detecting the percent survival of spores. RV-PCR results were obtained in17 h compared to 7 days for the standard culturing method. High-throughput sample processing and RV-PCR protocols were also developed and tested for synthetic wipe samples containing reference dirt material. RV-PCR protocols allowed processing and accurate analysis of approximately100 dirty wipe samples (2''x2'' synthetic) containing approximately10 viable B. atrophaeus spores in24 h. Quantitative RV-PCR protocols based on a Most-Probable-Number (MPN) statistical approach developed for B. anthracis Sterne resulted in more rapid turnaround times than those for traditional culturing and no significant difference in log colony-forming units compared to traditional viability analysis. Integration of RV-PCR assays with high-throughput protocols will allow the processing of 200 wipe samples per day per robot using commercially available automation.

Published

2009

5. Operational Evaluation of the Rapid Viability PCR Method for Post-Decontamination Clearance Sampling

Author

Gloria A. Murphy, Sonia E. Létant, Staci R. Kane, Tonya L. Nichols, Marissa Mullins, Sanjiv Shah, Julie R. Avila, Edmund P. Salazar, and Teneile M. Alfaro

Subjects

Chromatography, Bacillus atrophaeus, fungi, Vaporized hydrogen peroxide, Human decontamination, Biology, biology.organism_classification, Endospore, Aerosolization, Microbiology, Spore, Bacillus anthracis, Air filter

Abstract

The Rapid Viability Polymerase Chain Reaction (RV-PCR) method was evaluated during the Bio-Response Operational Testing and Evaluation (BOTE), an interagency project to evaluate field-level facility biological remediation, using leading decontamination technologies. The tests were performed using an intentional release (aerosolization) of spores of Bacillus atrophaeus subspecies globigii (BG), as a surrogate for Bacillus anthracis, the etiologic agent for anthrax. Three decontamination methods were assessed including fumigation with vaporized hydrogen peroxide (VHP), fumigation with chlorine dioxide (CD), and a surface treatment process using pH-adjusted bleach.The RV-PCR method was developed to rapidly detect live B. anthracis spores during a bioterrorism event. The method uses a change in realtime PCR response before and after a nine hour incubation step, to determine the presence of viable bacterial spores in the sample; the method was recently verified for air filter, wipe and water samples at the 10-spore level for B. anthracis Ames spores, and was also developed for swab, sponge-stick, and vacuum sock/filter samples. In the method, high throughput sample processing is combined with PCR-based analysis before and after a rapid culture step to speed viability determination, especially for complex surface and environmental samples that present challenges to current culture-based methods. In the BOTE project, a total of 159 surface wipe samples from post-decontamination events were analyzed by splitting the suspension after spore recovery into two equal parts, with one part analyzed by RV-PCR and the other part by culture after concentrating to the same volume. In the BOTE project, the RV-PCR method provided rapid results for post-decontamination samples that were 98% (156/159 samples) consistent with results from culture analysis. The percentage agreement was noteworthy, given the large number of samples containing low spore levels. For the Post-VHP, Post-Bleach, and Post-CD event samples, the percentage agreement was 93% (41/44 samples), 100% (47/47 samples), and 100% (68/68 samples), respectively. The RV-PCR method performed well for the surrogate BG spores exposed to decontaminants at real-world application levels, and with wipe samples containing background debris and indigenous microbial populations.

Published

2013

6. Rapid-Viability PCR Method for Detection of Live, Virulent Bacillus anthracis in Environmental Samples ▿

Author

Ellen Raber, Teneile M. Alfaro, Sanjiv Shah, Staci R. Kane, Sonia E. Létant, Julie R. Avila, Gloria A. Murphy, and Thomas M. Bunt

Subjects

DNA, Bacterial, Time Factors, Virulence, Real-Time Polymerase Chain Reaction, Applied Microbiology and Biotechnology, Incubation period, Microbiology, Automation, High-Throughput Screening Assays, Methods, Environmental Microbiology, Incubation, Detection limit, Bacteriological Techniques, Microbial Viability, Ecology, biology, Bacteroidetes, biology.organism_classification, DNA extraction, Bacillus anthracis, Food Science, Biotechnology, Plasmids

Abstract

In the event of a biothreat agent release, hundreds of samples would need to be rapidly processed to characterize the extent of contamination and determine the efficacy of remediation activities. Current biological agent identification and viability determination methods are both labor- and time-intensive such that turnaround time for confirmed results is typically several days. In order to alleviate this issue, automated, high-throughput sample processing methods were developed in which real-time PCR analysis is conducted on samples before and after incubation. The method, referred to as rapid-viability (RV)-PCR, uses the change in cycle threshold after incubation to detect the presence of live organisms. In this article, we report a novel RV-PCR method for detection of live, virulent Bacillus anthracis , in which the incubation time was reduced from 14 h to 9 h, bringing the total turnaround time for results below 15 h. The method incorporates a magnetic bead-based DNA extraction and purification step prior to PCR analysis, as well as specific real-time PCR assays for the B. anthracis chromosome and pXO1 and pXO2 plasmids. A single laboratory verification of the optimized method applied to the detection of virulent B. anthracis in environmental samples was conducted and showed a detection level of 10 to 99 CFU/sample with both manual and automated RV-PCR methods in the presence of various challenges. Experiments exploring the relationship between the incubation time and the limit of detection suggest that the method could be further shortened by an additional 2 to 3 h for relatively clean samples.

Published

2011

7. Most-probable-number rapid viability PCR method to detect viable spores of Bacillus anthracis in swab samples

Author

Lisa Hodges, Sonia E. Létant, Ellen Raber, Teneile M. Alfaro, Laura J. Rose, Staci R. Kane, and Gloria A. Murphy

Subjects

Microbiology (medical), Spores, Bacterial, Validation study, Microbial Viability, fungi, Colony Count, Microbial, Contamination, Biology, biology.organism_classification, Microbiology, Endospore, Polymerase Chain Reaction, Spore, Bacillus anthracis, Most probable number, Environmental Microbiology, Pcr method, Molecular Biology

Abstract

A comparison of Most-Probable-Number Rapid Viability (MPN RV) PCR and traditional culture methods for the quantification of Bacillus anthracis Sterne spores in macrofoam swabs from a multi-center validation study was performed. The purpose of the study was to compare environmental swab processing methods for recovery, detection, and quantification of viable B. anthracis spores from surfaces. Results show that spore numbers provided by the MPN RV-PCR method were typically within 1-log of the values from a plate count method for all three levels of spores tested (3.1x10(4), 400, and 40 spores sampled from surfaces with swabs) even in the presence of debris. The MPN method tended to overestimate the expected result, especially at lower spore levels. Blind negative samples were correctly identified using both methods showing a lack of cross contamination. In addition to detecting low levels of spores in environmental conditions, the MPN RV-PCR method is specific, and compatible with automated high-throughput sample processing and analysis protocols, enhancing its utility for characterization and clearance following a biothreat agent release.

Published

2010