Melanie K. Brown scite author profile

Melanie K. Brown

5Publications

19Citation Statements Received

96Citation Statements Given

How they've been cited

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114

Affiliations

Teesside University, Virginia Commonwealth University Medical Center, Sentara Norfolk General Hospital

Publications

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Defining the Clinical Significance of Alloscardovia omnincolens in the Urinary Tract

et al. 2016

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The clinical significance of Alloscardovia omnincolens in the urinary tract has not been thoroughly evaluated. In this study, 15 patients with A. omnincolens present in their urine cultures were identified. A. omnincolens is only rarely associated with urinary tract symptoms and in some patients may play a commensal role. With the widespread adoption of matrix-assisted laser desorption ionization-time of flight mass spectrometry (MALDI-TOF MS), bacteria are now identified with greater accuracy than with conventional phenotypic methods (1). This is particularly true for identification of bacteria that were difficult to distinguish or identify and would have been previously classified into broad categories such as urogenital flora. These organisms can now be identified to the species level with great accuracy. Although beneficial in most circumstances, the improved ability to rapidly identify most bacteria forces clinical microbiologists and infectious disease practitioners to interpret the clinical significance of unfamiliar organisms.Alloscardovia omnincolens is one such organism. Prior to implementation of MALDI-TOF MS, this organism, a member of the Bifidobacteriaceae family, was difficult to identify in the absence of 16S rRNA sequencing (2). Appearing as small, pinpoint, alpha-hemolytic colonies on blood agar, A. omnincolens would have most likely been considered urogenital flora since it is a catalase-and oxidase-negative, Gram-positive rod that could not be accurately identified using phenotypic methods (2). This organism has been isolated and identified in urine, saliva, and blood specimens; however, its clinical significance is yet to be determined (3-6).This study was prompted by the observation that A. omnincolens was being isolated from urine cultures in pure or predominant growth with unknown clinical presentations. To better understand the significance of this organism, both a 10-month retrospective review and prospective evaluation of Ͼ3,000 urine cultures were performed. In total, the laboratory results and clinical information of 15 patients with A. omnincolens were reviewed to assess the clinical significance and colonization frequency of this organism. MATERIALS AND METHODSIdentification of isolates and cases. This study consisted of both retrospective and prospective analyses. In the retrospective analysis, the laboratory information system was used to evaluate all urine cultures submitted to our laboratory between June 2013 and April 2014. This search was conducted to identify any culture that yielded significant growth of A. omnincolens. A threshold of 10 4 CFU/ml was used to determine significant growth.To establish the rate of colonization, a prospective analysis was performed between 12 August 2014 and 26 March 2015. In this analysis, 3,395 noncontinuous urine specimens submitted for routine bacterial culture were plated (0.01 ml) to 5% sheep blood (sBAP) and MacConkey agars; sBAPs were incubated for up to 48 h at 35°C in 5% CO 2 and prospectively examined for the growth of any amount of ...

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Design, optimisation and preliminary validation of a human specific loop-mediated amplification assay for the rapid detection of human DNA at forensic crime scenes

Hird

Brown

2017

Science & Justice

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The identification of samples at a crime scene which require forensic DNA typing has been the focus of recent research interest. We propose a simple, but sensitive analysis system which can be deployed at a crime scene to identify crime scene stains as human or non-human. The proposed system uses the isothermal amplification of DNA in a rapid assay format, which returns results in as little as 30min from sampling. The assay system runs on the Genie II device, a proven in-field detection system which could be deployed at a crime scene. The results presented here demonstrate that the system was sufficiently specific and sensitive and was able to detect the presence of human blood, semen and saliva on mock forensic samples.

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The acid phosphatase test two minute cut-off: An insufficient time to detect some semen stains

Redhead¹,

Brown²

2013

Science & Justice

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An investigation of two methods of DNA recovery from fired and unfired 9 mm ammunition

et al. 2021

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Extraction-Free, Direct Determination of Caffeine in Microliter Volumes of Beverages by Thermal Desorption-Gas Chromatography Mass Spectrometry

Peng

Brown

Bowdler

et al. 2020

International Journal of Analytical Chemistry

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An extraction-free method requiring microliter (μL) volumes has been developed for the determination of caffeine in beverages. Using a pyrolysis-gas chromatography mass spectrometry system, the conditions required for the direct thermal desorption-gas chromatography mass spectrometry (TD-GC/MS) determination of caffeine were optimised. A 5 μL aliquot was introduced to the thermal desorption unit, dried, and thermally desorbed to the GC/MS. The response was linear over the range 10 to 500 μg/mL (R2 = 0.996). The theoretical limit of detection (3 σ) was 0.456 μg/mL. No interferences were recorded from endogenous beverage components or from commonly occurring drugs, such as nicotine, ibuprofen, and paracetamol. Replicate caffeine determinations on fortified latte style white coffee and Pepsi Max® gave mean recoveries of 93.4% (%CV = 4.1%) and 95.0% (%CV = 0.98%), respectively. Good agreement was also obtained with the stated values of caffeine for an energy drink and for Coca-Cola®. These data suggest that the method holds promise for the determination of caffeine in such samples.

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Melanie K. Brown

Defining the Clinical Significance of Alloscardovia omnincolens in the Urinary Tract

Design, optimisation and preliminary validation of a human specific loop-mediated amplification assay for the rapid detection of human DNA at forensic crime scenes

The acid phosphatase test two minute cut-off: An insufficient time to detect some semen stains

An investigation of two methods of DNA recovery from fired and unfired 9 mm ammunition

Extraction-Free, Direct Determination of Caffeine in Microliter Volumes of Beverages by Thermal Desorption-Gas Chromatography Mass Spectrometry

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