Publications by authors named "Timothy D Minogue"

Background: Point of need diagnostics provide efficient testing capability for remote or austere locations, decreasing the time to answer by minimizing travel or sample transport requirements. Loop-mediated isothermal amplification (LAMP) is an appealing technology for point-of-need diagnostics due to its rapid analysis time and minimal instrumentation requirements.

Methods: Here, we designed and optimized nine LAMP assays that are sensitive and specific to targeted bacterial select agents including Bacillus anthracis, Francisella tularensis, Yersinia pestis, and Brucella spp.

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Antimicrobial resistance (AR) is one of the greatest threats to global health and is associated with higher treatment costs, longer hospital stays, and increased mortality. Current gold standard antimicrobial susceptibility tests (AST) rely on organism growth rates that result in prolonged time-to-answer for slow growing organisms. Changes in the cellular transcriptome can be rapid in the presence of stressors such as antibiotic pressure, providing the opportunity to develop AST towards transcriptomic signatures.

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Diagnostic limitations challenge management of clinically indistinguishable acute infectious illness globally. Gene expression classification models show great promise distinguishing causes of fever. We generated transcriptional data for a 294-participant (USA, Sri Lanka) discovery cohort with adjudicated viral or bacterial infections of diverse etiology or non-infectious disease mimics.

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Rapid pathogen identification is a critical first step in patient isolation, treatment, and controlling an outbreak. Real-time PCR is a highly sensitive and specific approach commonly used for infectious disease diagnostics. However, mismatches in the primer or probe sequence and the target organism can cause decreased sensitivity, assay failure, and false negative results.

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The emergence of SARS-CoV-2 and the subsequent pandemic has highlighted the need for animal models that faithfully replicate the salient features of COVID-19 disease in humans. These models are necessary for the rapid selection, testing, and evaluation of potential medical countermeasures. Here, we performed a direct comparison of two distinct routes of SARS-CoV-2 exposure-combined intratracheal/intranasal and small particle aerosol-in two nonhuman primate species, rhesus and cynomolgus macaques.

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Next-generation sequencing is rapidly finding footholds in numerous microbiological fields, including infectious disease diagnostics. Here, we describe a molecular inversion probe panel for the identification of bacterial, viral, and parasitic pathogens. We describe the ability of Illumina and Oxford Nanopore Technologies (ONT) to sequence small amplicons originating from this panel for the identification of pathogens in complex matrices.

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Crimean-Congo hemorrhagic fever virus (CCHFV) is a highly pathogenic tick-borne RNA virus prevalent in Asia, Europe, and Africa, and can cause a hemorrhagic disease (CCHF) in humans with mortality rates as high as 60%. A general lack of both effective medical countermeasures and a comprehensive understanding of disease pathogenesis is partly driven by an historical lack of viable CCHF animal models. Recently, a cynomolgous macaque model of CCHF disease was developed.

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Article Synopsis
  • Syrian hamsters can develop a deadly illness similar to human hantavirus pulmonary syndrome (HPS) when infected with Andes virus (ANDV), while Hantaan virus (HTNV) leads to an asymptomatic infection.
  • Researchers used NanoString technology to study 770 genes in the blood of these hamsters, revealing significant differences in immune response genes related to type I interferon, complement activation, and apoptosis pathways between the two virus infections.
  • The study found that ANDV delays the immune response, which may help the virus evade the host's defenses and worsen the disease; this research is the first of its kind and could lead to new treatment options for hantavirus infections.
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Ebola virus is a continuing threat to human populations, causing a virulent hemorrhagic fever disease characterized by dysregulation of both the innate and adaptive host immune responses. Severe cases are distinguished by an early, elevated pro-inflammatory response followed by a pronounced lymphopenia with B and T cells unable to mount an effective anti-viral response. The precise mechanisms underlying the dysregulation of the host immune system are poorly understood.

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Airborne transmission is predicted to be a prevalent route of human exposure with SARS-CoV-2. Aside from African green monkeys, nonhuman primate models that replicate airborne transmission of SARS-CoV-2 have not been investigated. A comparative evaluation of COVID-19 in African green monkeys, rhesus macaques, and cynomolgus macaques following airborne exposure to SARS-CoV-2 was performed to determine critical disease parameters associated with disease progression, and establish correlations between primate and human COVID-19.

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Development and implementation of rapid antimicrobial susceptibility testing is critical for guiding patient care and improving clinical outcomes, especially in cases of sepsis. One approach to reduce the time-to-answer for antimicrobial susceptibility is monitoring the inhibition of DNA production, as differences in DNA concentrations are more quickly impacted compared to optical density changes in traditional antimicrobial susceptibility testing. Here, we use real-time PCR to rapidly determine antimicrobial susceptibility after short incubations with antibiotic.

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During 2013-2014, we collected 1,926 serum samples from humans and 4,583 ticks (Hyalomma asiaticum or Dermacentor nuttalli) in select regions of Mongolia to determine the risk for Crimean-Congo hemorrhagic fever virus (CCHFV) infection among humans in this country. Testing of human serum samples by ELISA demonstrated an overall CCHFV antibody prevalence of 1.4%; Bayankhongor Province had the highest prevalence, 2.

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Rapid pathogen identification during an acute febrile illness is a critical first step for providing appropriate clinical care and patient isolation. Primary screening using sensitive and specific assays, such as real-time PCR and ELISAs, can rapidly test for known circulating infectious diseases. If the initial testing is negative, potentially due to a lack of developed diagnostic assays or an incomplete understanding of the pathogens circulating within a geographic region, additional testing would be required including highly multiplexed assays and metagenomic next generation sequencing.

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Background: Next-generation sequencing (NGS) is revolutionizing a variety of molecular biology fields including bioforensics, biosurveillance, and infectious disease diagnostics. For pathogen detection, the ability to sequence all nucleic acids in a sample allows near limitless multiplexability, free from a priori knowledge regarding an etiologic agent as is typically required for targeted molecular assays such as real-time PCR. Furthermore, sequencing capabilities can generate in depth genomic information, allowing detailed molecular epidemiological studies and bioforensics analysis, which is critical for source agent identification in a biothreat outbreak.

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Article Synopsis
  • Next-generation sequencing (NGS) is an emerging technology for diagnosing infectious diseases but requires standardized methods to be clinically reliable.
  • The DETEQT software was developed to improve the accuracy of NGS diagnostics by using a novel bioinformatics pipeline that assesses sequence data for better diagnostic outcomes.
  • DETEQT has shown over 95% accuracy in clinical evaluations and is integrated into a user-friendly platform, making it accessible for non-experts in clinical labs.
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  • Ebola virus (EBOV) causes a severe hemorrhagic fever and can produce its own microRNAs (miRNAs) to evade the host's immune response.
  • Researchers studied EBOV variants in mice, rhesus macaques, cynomolgus macaques, and humans, identifying ten viral miRNAs that were present across all species during infection, with some showing increased levels before symptoms appeared.
  • The consistent presence of specific miRNAs in various hosts suggests they could serve as important diagnostic tools and play a role in how EBOV causes disease.
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Targeted sequencing promises to bring next-generation sequencing (NGS) into routine clinical use for infectious disease diagnostics. In this context, upfront processing techniques, including pathogen signature enrichment, must amplify multiple targets of interest for NGS to be relevant when applied to patient samples with limited volumes. Here, we demonstrate an optimized molecular inversion probe (MIP) assay targeting multiple variable regions within the 16S ribosomal gene for the identification of biothreat and ESKAPE pathogens in a process that significantly reduces complexity, labor, and processing time.

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Zika virus (ZIKV) is a mosquito-borne member of the genus that has emerged since 2007 to cause outbreaks in Africa, Asia, Oceania, and most recently, in the Americas. Here, we used an isolate history as well as genetic and phylogenetic analyses to characterize three low-passage isolates representing African (ArD 41525) and Asian (CPC-0740, SV0127-14) lineages to investigate the potential phenotypic differences in vitro and in vivo. The African isolate displayed a large plaque phenotype (∼3-4 mm) on Vero and HEK-293 cells, whereas the Asian isolates either exhibited a small plaque phenotype (∼1-2 mm) or did not produce any plaques.

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  • CCHFV is a tick-borne virus that can cause symptoms like fever and myalgia, sometimes leading to hemorrhagic fever with a mortality rate between 5% and 30%.
  • The virus is widespread across continents, and its genetic diversity poses challenges for accurate diagnostic assays, which can result in false negatives.
  • An updated RT-PCR assay was developed to enhance detection of CCHFV strains, showing significant improvements in sensitivity and inclusivity, underpinning the need for ongoing viral sequencing to strengthen diagnostic methods.
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  • Ebola virus disease (EVD) has high mortality rates (20-90%) and is characterized by intense virus replication and host immune response, leading researchers to explore immune responses through transcriptomics.
  • In a study with cynomolgus macaques, different exposure routes to the Ebola virus Makona were analyzed using RNA-Seq and a NanoString nCounter targeting 769 genes, finding similar overall transcriptional responses and correlated gene expression patterns.
  • Both methods effectively predicted immune cell populations and demonstrated that developing a NanoString codeset specific to non-human primates can enhance research on filoviruses while circumventing the logistical challenges of RNA-Seq.
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  • Antibiotic-resistant infections pose a serious challenge in healthcare, necessitating quick and effective antibiotic treatments.
  • Diagnostic tools that swiftly identify bacterial resistance profiles are essential for timely patient care.
  • A new method using MALDI-TOF mass spectrometry showed 95% accuracy in determining the resistance of Staphylococcus aureus to antibiotics within 3 hours of detecting bacteria in blood cultures.
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Research involving biosafety level 3 pathogens such as West Nile virus (WNV) is often limited by the limited space and technical constraints of these environments. To conduct complex analytical studies outside of high containment, robust and reliable inactivation methods are needed that maintain compatibility with downstream assays. Here we report the inactivation of WNV in spiked serum samples using a commercially available SDS-PAGE sample buffer for proteomic studies.

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Antibiotic resistance (AR) is an epidemic of increasing magnitude requiring rapid identification and profiling for appropriate and timely therapeutic measures and containment strategies. In this context, ciprofloxacin is part of the first-line of countermeasures against numerous high consequence bacteria. Significant resistance can occur via single nucleotide polymorphisms (SNP) and deletions within ciprofloxacin targeted genes.

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