Your search keyword '"Christopher J. Ehrhardt"' showing total 25 results

1. Analysis of red autofluorescence (650-670nm) in epidermal cell populations and its potential for distinguishing contributors to 'touch' biological samples [version 1; referees: 2 approved]

Author

Cristina E. Stanciu, M. Katherine Philpott, Eduardo E. Bustamante, Ye Jin Kwon, and Christopher J. Ehrhardt

Subjects

Experimental Biophysical Methods, Genomics, Medicine, Science

Abstract

Interpretation of touch DNA mixtures poses a significant challenge for forensic caseworking laboratories. Front end techniques that facilitate separation of contributor cell populations before DNA extraction are a way to circumvent this problem. The goal of this study was to survey intrinsic fluorescence of epidermal cells collected from touch surfaces and investigate whether this property could potentially be used to discriminate between contributor cell populations in a biological mixture. Analysis of red autofluorescence (650-670nm) showed that some contributors could be distinguished on this basis. Variation was also observed between autofluorescence profiles of epidermal cell populations from a single contributor sampled on different days. This dataset suggests that red autofluorescence may be a useful marker for identifying distinct cell populations in some mixtures. Future efforts should continue to investigate the extrinsic or intrinsic factors contributing to this signature, and to identify additional biomarkers that could complement this system.

Published

2016

2. Optical characterization of epidermal cells and their relationship to DNA recovery from touch samples [version 1; referees: 2 approved]

Author

Cristina E. Stanciu, M. Katherine Philpott, Ye Jin Kwon, Eduardo E. Bustamante, and Christopher J. Ehrhardt

Subjects

Experimental Biophysical Methods, Genomics, Medicine, Science

Abstract

The goal of this study was to investigate the relative contributions of different cellular and genetic components to biological samples created by touch or contact with a surface – one of the most challenging forms of forensic evidence. Touch samples were generated by having individuals hold an object for five minutes and analyzed for quantity of intact epidermal cells, extracellular DNA, and DNA from pelleted cell material after elution from the collection swab. Comparisons were made between samples where individuals had washed their hands immediately prior to handling and those where hand washing was not controlled. The vast majority (84-100%) of DNA detected in these touch samples was extracellular and was uncorrelated to the number of epidermal cells detected. Although little to no extracellular or cell pellet-associated DNA was detected when individuals washed their hands prior to substrate handling, we found that a significant number of epidermal cells (between ~5x103 and ~1x105) could still be recovered from these samples, suggesting that other types of biological information may be present even when no amplifiable nuclear DNA is present. These results help to elucidate the biological context for touch samples and characterize factors that may contribute to patterns of transfer and persistence of genetic material in forensic evidence.

Published

2015

3. Nanoscale visualization of extracellular DNA on cell surfaces

Author

Anita Olsen, Christopher J. Ehrhardt, and Vamsi K. Yadavalli

Subjects

medicine.anatomical_structure, Materials science, Atomic force microscopy, Cell, medicine, Biophysics, General Earth and Planetary Sciences, Nanoscopic scale, Extracellular dna, General Environmental Science, Visualization

Published

2020

4. Chitosan Stabilized Silver Nanoparticles for the Electrochemical Detection of Lipopolysaccharide: A Facile Biosensing Approach for Gram-Negative Bacteria

Author

Christopher J. Ehrhardt, Vamsi K. Yadavalli, Muhammad R. Shah, Muhammad Imran, and Massimo F. Bertino

Subjects

silver nanoparticles, Gram-negative bacteria, lcsh:Mechanical engineering and machinery, 02 engineering and technology, medicine.disease_cause, biosensor, 01 natural sciences, Silver nanoparticle, Article, Chitosan, chemistry.chemical_compound, medicine, Escherichia coli, lcsh:TJ1-1570, Electrical and Electronic Engineering, Chromatography, biology, Mechanical Engineering, 010401 analytical chemistry, lipopolysaccharide, 021001 nanoscience & nanotechnology, biology.organism_classification, 0104 chemical sciences, Membrane, chemistry, Control and Systems Engineering, chitosan, 0210 nano-technology, Bacterial outer membrane, Biosensor, Bacteria

Abstract

Negatively charged lipopolysaccharide (LPS), a major endotoxin and component of the outer membrane of several Gram-negative bacteria, provides a useful biomarker for the indirect detection of these pathogens. For instance, Escherichia coli (E. coli) is a pathogenic bacterium that causes infections in almost all age groups, and has been implicated in food and water contamination. Current diagnostic and detection methods tend to be labor-intensive or expensive, necessitating the need for an easy, sensitive, rapid, and low-cost method. We report on the synthesis and use of positively charged chitosan stabilized silver nanoparticles (Chi-AgNPs) as a sensitive electrochemical nanobiosensor for the detection of LPS. Chi-AgNPs were synthesized through a facile, single step protocol, and characterized for size, charge, and morphology. Glassy carbon electrodes modified with Chi-AgNPs resulted in an enhancement of signal in the presence of both LPS and E. coli. Detection was accomplished over a large concentration range (several orders of magnitude) of 0.001&ndash, 100 ng/mL and 10&ndash, 107 CFU/mL. The biosensors can reliably detect LPS and E. coli at very low concentrations. Chi-AgNPs have potential as low cost, sensitive nanobiosensors for Gram-negative bacteria due to strong electrostatic interaction with LPS present in their outer membranes.

Published

2020

5. Evaluation of Bluestar ® Forensic Magnum and Other Traditional Blood Detection Methods on Bloodstained Wood Subjected to a Variety of Burn Conditions

Author

Christopher J. Ehrhardt, Catherine C. Connon, Eric J. Hazelrigg, and Autumn R. Vineyard

Subjects

Accelerant, business.industry, 010401 analytical chemistry, Smothering, 01 natural sciences, 0104 chemical sciences, Pathology and Forensic Medicine, Luminol, Toxicology, Forensic science, 03 medical and health sciences, chemistry.chemical_compound, 0302 clinical medicine, chemistry, Genetics, Medicine, 030216 legal & forensic medicine, business

Abstract

Accurate blood detection is a primary concern for forensic scientists, especially in highly compromised situations. In this study, blood was added to wood blocks and subjected to a variety of fire treatments: the absence or presence of accelerant, burn time (1, 3, or 5 min), and extinguishment method (smothering or dousing with water). Burned blocks were given a qualitative burn score, followed by removal of half of the char from each block and subsequent testing of each half for blood using luminol (13% positive; n = 96), Bluestar® Forensic Magnum (5.2% positive; n = 96), and combined phenolphthalein tetramethylbenzidine test (0% positive; n = 192). Luminol and Bluestar® Forensic Magnum performed similarly, both outperforming PTMB. Additionally, positive results were more likely from samples that were smothered, had a low burn score, and had more concentrated blood solutions (neat or 1:2). Overall, it is extremely unlikely that blood would be detected on combustible substrates exposed to direct fire.

Published

2018

6. Simplification of complex DNA profiles using front end cell separation and probabilistic modeling

Author

Susan A. Greenspoon, Nancy A. Stokes, Christopher J. Ehrhardt, Cristina Stanciu, and Emily R. Brocato

Subjects

0301 basic medicine, Fraction (chemistry), Cell Separation, Real-Time Polymerase Chain Reaction, Article, Antibodies, Fluorescence, Pathology and Forensic Medicine, Flow cytometry, 03 medical and health sciences, 0302 clinical medicine, Labelling, Genetics, Cell separation, medicine, Humans, 030216 legal & forensic medicine, Models, Statistical, medicine.diagnostic_test, Chemistry, Probabilistic logic, DNA, Cell Fraction, Cell sorting, Flow Cytometry, DNA Fingerprinting, 030104 developmental biology, DNA profiling, Molecular Probes, Biological system, Blood Chemical Analysis, Microsatellite Repeats

Abstract

Forensic samples comprised of cell populations from multiple contributors often yield DNA profiles that can be extremely challenging to interpret. This frequently results in decreased statistical strength of an individual’s association to the mixture and the loss of probative data. The purpose of this study was to test a front-end cell separation workflow on complex mixtures containing as many as five contributors. Our approach involved selectively labelling certain cell populations in dried whole blood mixture samples with fluorescently labeled antibody probe targeting the HLA-A*02 allele, separating the mixture using Fluorescence Activated Cell Sorting (FACS) into two fractions that are enriched in A*02 positive and A*02 negative cells, and then generating DNA profiles for each fraction. We then tested whether antibody labelling and cell sorting effectively reduced the complexity of the original cell mixture by analyzing STR profiles quantitatively using the probabilistic modeling software, TrueAllele® Casework. Results showed that antibody labelling and FACS separation of target populations yielded simplified STR profiles that could be more easily interpreted using conventional procedures. Additionally, TrueAllele® analysis of STR profiles from sorted cell fractions increased statistical strength for the association of most of the original contributors interpreted from the original mixtures.

Published

2018

7. Analysis of cellular autofluorescence in touch samples by flow cytometry: implications for front end separation of trace mixture evidence

Author

Eduardo E. Bustamante, Cristina Stanciu, M. Katherine Philpott, Susan A. Greenspoon, Christopher J. Ehrhardt, and Ye Jin Kwon

Subjects

0301 basic medicine, FACS, Analytical chemistry, Cell Separation, Biochemistry, Antibodies, Fluorescence, Analytical Chemistry, Flow cytometry, Specimen Handling, 03 medical and health sciences, 0302 clinical medicine, medicine, Cell separation, Humans, A-DNA, 030216 legal & forensic medicine, Biological mixtures, Isolated cell, medicine.diagnostic_test, Chemistry, Mixture interpretation, STR profiling, Epithelial Cells, DNA, Cell sorting, Flow Cytometry, Autofluorescence, 030104 developmental biology, DNA profiling, Touch, Biophysics, Research Paper, Trace

Abstract

The goal of this study was to survey optical and biochemical variation in cell populations deposited onto a surface through touch or contact and identify specific features that may be used to distinguish and then sort cell populations from separate contributors in a trace biological mixture. Although we were not able to detect meaningful biochemical variation in touch samples deposited by different contributors through preliminary antibody surveys, we did observe distinct differences in red autofluorescence emissions (650–670 nm), with as much as a tenfold difference in mean fluorescence intensities observed between certain pairs of donors. Results indicate that the level of red autofluorescence in touch samples can be influenced by a donor’s contact with specific material prior to handling the substrate from which cells were collected. In particular, we observed increased red autofluorescence in cells deposited subsequent to handling laboratory gloves, plant material, and certain types of marker ink, which could be easily visualized microscopically or using flow cytometry, and persisted after hand washing. To test whether these observed optical differences could potentially be used as the basis for a cell separation workflow, a controlled two-person touch mixture was separated into two fractions via fluorescence-activated cell sorting (FACS) using gating criteria based on intensity of 650–670 nm emissions and then subjected to DNA analysis. Genetic analysis of the sorted fractions provided partial DNA profiles that were consistent with separation of individual contributors from the mixture suggesting that variation in autofluorescence signatures, even if driven by extrinsic factors, may nonetheless be a useful means of isolating contributors to some touch mixtures. Graphical AbstractConceptual workflow diagram. Trace biological mixtures containing cells from multiple individuals are analyzed by flow cytometry. Cells are then physically separated into two populations based on intensity of red autofluorescence using Fluorescence Activated Cell Sorting. Each isolated cell fraction is subjected to DNA analysis resulting in a DNA profile for each contributor. Electronic supplementary material The online version of this article (doi:10.1007/s00216-017-0364-0) contains supplementary material, which is available to authorized users.

Published

2017

8. Testing Hormone-specific Antibody Probes for Presumptive Detection and Separation of Contributor Cell Populations in Trace DNA Mixtures

Author

Emily R. Brocato, Susan A. Greenspoon, Christopher J. Ehrhardt, Jennifer M. Miller, and Vamsi K. Yadavalli

Subjects

0303 health sciences, education.field_of_study, biology, Chemistry, Population, Cell, Cell Fraction, Fluorescence, 03 medical and health sciences, chemistry.chemical_compound, 0302 clinical medicine, medicine.anatomical_structure, DNA profiling, Biochemistry, Extracellular, medicine, biology.protein, 030216 legal & forensic medicine, Antibody, education, DNA, 030304 developmental biology

Abstract

“Touch” or trace DNA evidence represent a significant proportion of samples analyzed by forensic science laboratories. Because these samples frequently contain multiple contributors and are often challenging to analyze due to low DNA concentrations and frequent degradation, front end techniques to simplify the mixture prior to DNA profiling could significantly impact case processing and enhance success rates. The goal of this study was to investigate whether targeting hormone molecules within the cell with antibody probes could be used to selectively label and then physically isolate contributor cell populations in trace biological samples. The separation of male and female cells into distinct fractions could reduce the complexity of the mixture prior to DNA profiling. To accomplish this, we first tested the specificity of fluorescently labelled anti-testosterone and anti-dihydrotestosterone antibody probes to epidermal cells from both male and female individuals. Results show that male and female cell populations can be effectively labeled using anti-testosterone and anti-dihydrotestosterone antibody probes and that distinct differences in binding efficiency and resulting median fluorescence of cell populations were observed between several individuals. These differences were then used to design sorting criteria for physically isolating each cell population in two-person epidermal cell mixtures using fluorescence activated cell sorting (FACS). DNA profiling of separated fractions in combination with probabilistic modeling demonstrated that some cell mixtures could be enriched for one contributor in separated cell fractions and yielded statistically more discriminating profiles compared to those generated from the original mixtures. Other mixtures tested showed less evidence of effective cell separation possibly due to a number of factors including imbalance of contributor DNA ratio, intra-sex variation of antibody binding efficiency, and contributions of extracellular or cell-free DNA in the mixture sample. Screening and separation of trace DNA samples with this approach may be presumptive and ultimately constrained by specific parameters of the original mixture, however, antibody binding optimization may mitigate some of these influences.

Published

2019

9. Synthesis of chitosan coated metal organic frameworks (MOFs) for increasing vancomycin bactericidal potentials against resistant S. aureus strain

Author

Samina Perveen, Massimo F. Bertino, Salim Saifullah, Muhammad Raza Shah, Muhammad Imran, Christopher J. Ehrhardt, Tasmina Kanwal, Iqra Ghaffar, and Vamsi K. Yadavalli

Subjects

Staphylococcus aureus, Materials science, Surface Properties, Metal ions in aqueous solution, Static Electricity, Bioengineering, 02 engineering and technology, Microbial Sensitivity Tests, 010402 general chemistry, medicine.disease_cause, 01 natural sciences, Biomaterials, Chitosan, chemistry.chemical_compound, Inhibitory Concentration 50, Chitin, Coated Materials, Biocompatible, X-Ray Diffraction, Vancomycin, Drug Resistance, Bacterial, Spectroscopy, Fourier Transform Infrared, medicine, Particle Size, Metal-Organic Frameworks, Calorimetry, Differential Scanning, fungi, 021001 nanoscience & nanotechnology, Antimicrobial, Combinatorial chemistry, 0104 chemical sciences, Anti-Bacterial Agents, chemistry, Mechanics of Materials, Drug delivery, Thermogravimetry, 0210 nano-technology, Hybrid material, Porosity, medicine.drug

Abstract

Multiple drug resistant (MDR) has become a major issue in developing countries. MDR bacterial infections lead to significant increase in morbidity, mortality and cost of prolonged treatments. Therefore, designing of strategies for improving the antimicrobial potential of the therapeutic agents are highly required. Metal organic frameworks (MOFs) are highly tunable hybrid material, consist of metal ions linked together by organic bridging ligands have been used as an efficient drug delivery carrier because of their biodegradability, low toxicity and structure integrity upon loading and functionalizing process. Current study was based on the synthesis of chitosan coated MOFs with enhanced contact with S. aureus cell surface. Chitosan is deacetylated derivative of chitin and capable for non-bonding interaction with negatively charged bacterial cell leading to enhanced contact of MOFs with S. aureus. Chitosan coated MOFs were characterized with various techniques such as atomic force microscopy, scanning electron microscopy, DLS, FT-IR, TGA, DSC and Powder X-ray diffraction. They were also studied for their efficacy on resistant S. aureus, results revealed that Vancomycin bactericidal activity significantly increased upon loading in chitosan coated MOFs and caused increased inhibition of resistant S. aureus. AFM analysis of S. aureus strains clearly revealed complete distortion of morphology by treating with chitosan modified drug loaded MOFs. Findings of the current study suggest the potential of chitosan coated MOFs for reversing bacterial resistance against Vancomycin and provide new perspectives for improved antibiotic therapy of infections associated with MDR.

Published

2019

10. Technical note: Survey of extracellular and cell-pellet-associated DNA from ‘touch’/trace samples

Author

Anita Olsen, Vamsi K. Yadavalli, Mary Tootham, Mekhi Miller, M. Katherine Philpott, and Christopher J. Ehrhardt

Subjects

Male, Cell, Cell Fractionation, Pathology and Forensic Medicine, chemistry.chemical_compound, Pellet, medicine, Extracellular, Fluorescence microscope, Humans, Reproducibility of Results, DNA, Flow Cytometry, DNA Fingerprinting, Fluorescence, Cell Pellet, medicine.anatomical_structure, Epidermal Cells, Microscopy, Fluorescence, chemistry, Cell-free fetal DNA, Touch, Biophysics, Female, Law

Abstract

The goal of this study was to characterize the reproducibility of extracellular and cell pellet associated DNA yields recovered from handled substrates. Results showed that extracellular DNA yields were extremely variable between contributors—ranging between 0 and >10ng—and tended to dwarf cell pellet yields, which varied between 0 and ∼230 pg. DNA yields across multiple samples from the same contributor on different days showed similar levels of variability in both DNA fractions, indicating that extracellular DNA yield is largely influenced by extrinsic and/or environmental factors and is not a contributor-specific attribute. Microscopic surveys of cells from the pellet fraction as well as fingerprints from the same contributor samples were conducted following treatment with fluorescent DNA stain. Nearly all imaged cells exhibited diffuse fluorescence across the cell without discernable evidence of nuclei. This is consistent with the limited nature of DNA recovery from the pellet fraction and the prevalence of extracellular DNA in these samples.

Published

2021

11. Real-Time Observation of Antimicrobial Polycation Effects on Escherichia coli: Adapting the Carpet Model for Membrane Disruption to Quaternary Copolyoxetanes

Author

Sithara S. Nair, Vamsi K. Yadavalli, Dennis E. Ohman, Kenneth J. Wynne, Congzhou Wang, Olga Yu. Zolotarskaya, and Christopher J. Ehrhardt

Subjects

0301 basic medicine, Polyurethanes, Antimicrobial peptides, 02 engineering and technology, Microscopy, Atomic Force, medicine.disease_cause, Cell membrane, Surface-Active Agents, 03 medical and health sciences, chemistry.chemical_compound, Escherichia coli, Electrochemistry, medicine, Polylysine, General Materials Science, Spectroscopy, biology, Cell Membrane, Surfaces and Interfaces, 021001 nanoscience & nanotechnology, Condensed Matter Physics, biology.organism_classification, Anti-Bacterial Agents, Nanopore, 030104 developmental biology, medicine.anatomical_structure, Membrane, chemistry, Biochemistry, Cytoplasm, Biophysics, lipids (amino acids, peptides, and proteins), 0210 nano-technology, Bacteria

Abstract

Real-time atomic force microscopy (AFM) was used for analyzing effects of the antimicrobial polycation copolyoxetane P[(C12)-(ME2Ox)-50/50], C12-50 on the membrane of a model bacterium, Escherichia coli (ATCC# 35218). AFM imaging showed cell membrane changes with increasing C12-50 concentration and time including nanopore formation and bulges associated with outer bacterial membrane disruption. A macroscale bactericidal concentration study for C12-50 showed a 4 log kill at 15 μg/mL with conditions paralleling imaging (1 h, 1x PBS, physiological pH, 25 °C). The dramatic changes from the control image to 1 h after introducing 15 μg/mL C12-50 are therefore reasonably attributed to cell death. At the highest concentration (60 μg/mL) further cell membrane disruption results in leakage of cytoplasm driven by detergent-like action. The sequence of processes for initial membrane disruption by the synthetic polycation C12-50 follows the carpet model posited for antimicrobial peptides (AMPs). However, the nanoscale details are distinctly different as C12-50 is a synthetic, water-soluble copolycation that is best modeled as a random coil. In a complementary AFM study, chemical force microscopy shows that incubating cells with C12-50 decreased the hydrophobicity across the entire cell surface at an early stage. This finding provides additional evidence indicating that C12-50 polycations initially bind with the cell membrane in a carpet-like fashion. Taken together, real time AFM imaging elucidates the mechanism of antimicrobial action for copolyoxetane C12-50 at the single cell level. In future work this approach will provide important insights into structure-property relationships and improved antimicrobial effectiveness for synthetic amphiphilic polycations.

Published

2016

12. Nanoscale Phenotypic Textures of Yersinia pestis Across Environmentally-Relevant Matrices

Author

Muhammed Raza Shah, Christopher J. Ehrhardt, Vamsi K. Yadavalli, Massimo F. Bertino, and Kanwal Mohammad Iqbal

Subjects

Microbiology (medical), Yersinia pestis, Phospholipid, medicine.disease_cause, Microbiology, Article, 03 medical and health sciences, chemistry.chemical_compound, soil culture, Virology, medicine, lcsh:QH301-705.5, Unsaturated fatty acid, Fatty acid methyl ester, 030304 developmental biology, chemistry.chemical_classification, 0303 health sciences, atomic force microscopy, biology, 030306 microbiology, Fatty acid, Pathogenic bacteria, nanoscale, biology.organism_classification, Phenotype, 3D printed culture chamber, Membrane, lcsh:Biology (General), chemistry, Biophysics

Abstract

The persistence of bacterial pathogens within environmental matrices plays an important role in the epidemiology of diseases, as well as impacts biosurveillance strategies. However, the adaptation potentials, mechanisms for survival, and ecological interactions of pathogenic bacteria such as Yersinia pestis are largely uncharacterized owing to the difficulty of profiling their phenotypic signatures. In this report, we describe studies on Y. pestis organisms cultured within soil matrices, which are among the most important reservoirs for their propagation. Morphological (nanoscale) and phenotypic analysis are presented at the single cell level conducted using Atomic Force Microscopy (AFM), coupled with biochemical profiles of bulk populations using Fatty Acid Methyl Ester Profiling (FAME). These studies are facilitated by a novel, customizable, 3D printed diffusion chamber that allows for control of the external environment and easy harvesting of cells. The results show that incubation within soil matrices lead to reduction of cell size and an increase in surface hydrophobicity. FAME profiles indicate shifts in unsaturated fatty acid compositions, while other fatty acid components of the phospholipid membrane or surface lipids remained consistent across culturing conditions, suggesting that phenotypic shifts may be driven by non-lipid components of Y. pestis.

Published

2020

13. Rapid differentiation of epithelial cell types in aged biological samples using autofluorescence and morphological signatures

Author

Emily R. Brocato, M. Katherine Philpott, Christopher J. Ehrhardt, and Catherine C. Connon

Subjects

0301 basic medicine, Male, Fluorescence-lifetime imaging microscopy, Pathology, Cellular differentiation, Buccal swab, lcsh:Medicine, Social Sciences, 01 natural sciences, Epithelium, Bright Field Microscopy, Spectrum Analysis Techniques, Fluorescence Microscopy, Animal Cells, Medicine and Health Sciences, lcsh:Science, Cells, Cultured, Microscopy, Multidisciplinary, medicine.diagnostic_test, Optical Imaging, Light Microscopy, Cell Differentiation, Flow Cytometry, Clinical Laboratory Sciences, medicine.anatomical_structure, Aspect Ratio, Spectrophotometry, Physical Sciences, Female, Cytophotometry, Cellular Types, Anatomy, Research Article, medicine.medical_specialty, Imaging Techniques, Geometry, Biology, Research and Analysis Methods, Flow cytometry, Specimen Handling, 03 medical and health sciences, Diagnostic Medicine, Fluorescence Imaging, medicine, Humans, Cell Size, Forensics, Mouth, lcsh:R, 010401 analytical chemistry, Bright-field microscopy, Biology and Life Sciences, Epithelial Cells, Buccal administration, Cell Biology, 0104 chemical sciences, Autofluorescence, 030104 developmental biology, Biological Tissue, Epidermal Cells, lcsh:Q, Law and Legal Sciences, Mathematics, Developmental Biology

Abstract

Establishing the tissue source of epithelial cells within a biological sample is an important capability for forensic laboratories. In this study we used Imaging Flow Cytometry (IFC) to analyze individual cells recovered from buccal, epidermal, and vaginal samples that had been dried between 24 hours and more than eight weeks. Measurements capturing the size, shape, and fluorescent properties of cells were collected in an automated manner and then used to build a multivariate statistical framework for differentiating cells based on tissue type. Results showed that epidermal cells could be distinguished from vaginal and buccal cells using a discriminant function analysis of IFC measurements with an average classification accuracy of ~94%. Ultimately, cellular measurements such as these, which can be obtained non-destructively, may provide probative information for many types of biological samples and complement results from standard genetic profiling techniques.

Published

2018

14. Rapid Differentiation of Epithelial Cell Types in Forensic Samples Using Intrinsic Fluorescence and Morphological Signatures

Author

Catherine C. Connon, Christopher J. Ehrhardt, M. Katherine Philpott, and Emily R. Brocato

Subjects

Imaging flow cytometry, 0303 health sciences, 010401 analytical chemistry, Buccal swab, Cell, Buccal administration, Intrinsic fluorescence, Biology, 01 natural sciences, Molecular biology, Epithelium, 0104 chemical sciences, Rapid identification, 03 medical and health sciences, medicine.anatomical_structure, DNA profiling, medicine, 030304 developmental biology

Abstract

Establishing the tissue source of epithelial cells within a biological sample is an important capability for forensic laboratories. In this study we used Imaging Flow Cytometry (IFC) to analyze individual cells recovered from buccal, contact epithelial, and vaginal samples that had been dried between 24 hours and more than eight weeks. Measurements capturing the size, shape, and fluorescent properties of cells were collected in an automated manner and then used to build a multivariate statistical framework for differentiating cells based on tissue type. Results showed that cell populations from the three tissue types could be differentiated using a Discriminant Function plot of IFC measurements. Epidermal cells were distinguished from vaginal and buccal cells with an average classification accuracy of ~94%. Ultimately, cellular measurements such as these, which can be obtained non-destructively, may provide probative information for many types of biological samples and complement results from standard genetic profiling techniques.

Published

2018

15. Separation of uncompromised whole blood mixtures for single source STR profiling using fluorescently-labeled human leukocyte antigen (HLA) probes and fluorescence activated cell sorting (FACS)

Author

M. Katherine Philpott, Cristina Stanciu, Lee Dean, Jamie Sturgill, Sarah J. Seashols-Williams, Tracey Dawson Cruz, Christopher J. Ehrhardt, and Ye Jin Kwon

Subjects

Cell type, Population, Cell, Human leukocyte antigen, Biology, Pathology and Forensic Medicine, chemistry.chemical_compound, HLA-A2 Antigen, Genetics, medicine, Humans, education, Alleles, Fluorescent Dyes, education.field_of_study, Forensic Sciences, Flow Cytometry, DNA Fingerprinting, Molecular biology, medicine.anatomical_structure, STR analysis, chemistry, DNA profiling, biology.protein, Antibody, Blood Chemical Analysis, DNA, Microsatellite Repeats

Abstract

Analysis of biological mixtures is a significant problem for forensic laboratories, particularly when the mixture contains only one cell type. Contributions from multiple individuals to biologic evidence can complicate DNA profile interpretation and often lead to a reduction in the probative value of DNA evidence or worse, its total loss. To address this, we have utilized an analytical technique that exploits the intrinsic immunological variation among individuals to physically separate cells from different sources in a mixture prior to DNA profiling. Specifically, we applied a fluorescently labeled antibody probe to selectively bind to one contributor in a mixture through allele-specific interactions with human leukocyte antigen (HLA) proteins that are expressed on the surfaces of most nucleated cells. Once the contributor's cells were bound to the probe, they were isolated from the mixture using fluorescence activated cell sorting (FACS)-a high throughput technique for separating cell populations based on their optical properties-and then subjected to STR analysis. We tested this approach on two-person and four-person whole blood mixtures where one contributor possessed an HLA allele (A*02) that was not shared by other contributors to the mixture. Results showed that hybridization of the mixture with a fluorescently-labeled antibody probe complimentary to the A*02 allele's protein product created a cell population with a distinct optical profile that could be easily differentiated from other cells in the mixture. After sorting the cells with FACS, genetic analysis showed that the STR profile of this cell population was consistent with that of the contributor who possessed the A*02 allele. Minor peaks from the A*02 negative contributor(s) were observed but could be easily distinguished from the profile generated from A*02 positive cells. Overall, this indicates that HLA antibody probes coupled to FACS may be an effective approach for generating STR profiles of individual contributors from forensic mixtures.

Published

2015

16. Evaluation of the suitability of cranial measurements obtained from surface-rendered CT scans of living people for estimating sex and ancestry

Author

Christopher J. Ehrhardt, Keith L. Monson, and Terrie Simmons-Ehrhardt

Subjects

medicine.diagnostic_test, business.industry, Measurement precision, Medicine, Radiology, Nuclear Medicine and imaging, Computed tomography, business, Cartography, Cross-validation, Pathology and Forensic Medicine

Abstract

Craniometric data from computed tomography (CT) head scans of 287 living Americans of three descent groups (African, Asian, European) and both sexes were analyzed for measurement precision. Classification accuracy was estimated by a leave-one-out cross validation, and group means were compared to the Forensic Data Bank (FDB). Landmarks were placed on 3D surface models of the skulls to approximate traditional cranial measurements utilized in sex and ancestry estimations. From repeat measurements by one observer on a subset of skulls (n = 14) reflecting 14 different CT protocols, the least precise landmark was euryon (SD ≤ 4.09 mm) and the least precise distances according to the coefficient of reliability (

Published

2019

17. Analysis of Antibody Hybridization and Autofluorescence in Touch Samples by Flow Cytometry: Implications for Front End Separation of Trace Mixture Evidence

Author

Cristina Stanciu, Ye Jin Kwon, Christopher J. Ehrhardt, Eduardo E. Bustamante, M. Katherine Philpott, and Susan A. Greenspoon

Subjects

0303 health sciences, medicine.diagnostic_test, Cell, Human leukocyte antigen, Biology, Bioinformatics, Fluorescence, Molecular biology, Flow cytometry, 03 medical and health sciences, Autofluorescence, Cytokeratin, 0302 clinical medicine, medicine.anatomical_structure, Antigen, medicine, biology.protein, 030216 legal & forensic medicine, Antibody, 030304 developmental biology

Abstract

The goal of this study was to survey optical and biochemical variation in cell populations deposited onto a surface through touch or contact and identify specific features that may be used to differentially label and then sort cell populations from separate contributors in a trace biological mixture. Cell characterizations initially focused on two different protein systems, Human Leukocyte Antigen (HLA) complex and cytokeratin (CK) filaments. Hybridization experiments using pan and allele-specific HLA antibody probes showed that surface antigens on cells transferred from the palmar surface of volunteers are largely unreactive, suggesting that they cannot be used to differentiate cell populations in a touch mixture. Touch samples were also hybridized with the pan-CK probe AE1, which targets CK proteins 10, 14, 15, 16 and 19. Fluorescence levels of AE1 hybridized cells were observed to vary across donors, although these differences were not consistent across all sampling days. We then investigated variations in red autofluorescence profiles (650-670nm) as a potential signature for distinguishing contributor cell populations. Although distinct differences in red autofluorescence profiles were observed ‐‐ with one donor consistently exhibiting higher levels of fluorescence than others ‐‐ some variation was also observed in touch samples collected from the same individual on different days. While this suggests that contributor touch samples cannot be defined by a discrete level of autofluorescence, this attribute may still be a useful means of isolating contributors to some touch mixtures. To test whether these observed optical differences could potentially be used as the basis for a cell separation workflow, a controlled two person touch mixture was separated into two fractions via Fluorescence Activated Cell Sorting (FACS) using gating criteria based on intensity of 650-670nm emissions, and then subjected to DNA analysis. STR typing of the sorted fractions provided partial profiles that were consistent with separation of individual contributors from the mixture.

Published

2016

18. Open-Source Tools for Dense Facial Tissue Depth Mapping of Computed Tomography Models

Author

Terrie Simmons-Ehrhardt, Anthony B. Falsetti, Christopher J. Ehrhardt, and Catyana Skory Falsetti

Subjects

Orientation (computer vision), Computer science, business.industry, 010401 analytical chemistry, Forensic anthropology, Nasal bone, 01 natural sciences, 0104 chemical sciences, 03 medical and health sciences, Skull, 0302 clinical medicine, medicine.anatomical_structure, Face (geometry), Facial tissue, Genetics, Forehead, medicine, Nasion, Computer vision, 030216 legal & forensic medicine, Artificial intelligence, business, Genetics (clinical), Ecology, Evolution, Behavior and Systematics

Abstract

Computed tomography (CT) scans provide anthropologists with a resource to generate three-dimensional (3D) digital skeletal material to expand quantification methods and build more standardized reference collections. The ability to visualize and manipulate the bone and skin of the face simultaneously in a 3D digital environment introduces a new way for forensic facial approximation practitioners to access and study the face. Craniofacial relationships can be quantified with landmarks or with surface-processing software that can quantify the geometric properties of the entire 3D facial surface. This article describes tools for the generation of dense facial tissue depth maps (FTDMs) using deidentified head CT scans of modern Americans from the Cancer Imaging Archive public repository and the open-source program Meshlab. CT scans of 43 females and 63 males from the archive were segmented and converted to 3D skull and face models using Mimics and exported as stereolithography files. All subsequent processing steps were performed in Meshlab. Heads were transformed to a common orientation and coordinate system using the coordinates of nasion, left orbitale, and left and right porion. Dense FTDMs were generated on hollowed, cropped face shells using the Hausdorff sampling filter. Two new point clouds consisting of the 3D coordinates for both skull and face were colorized on an RGB (red-green-blue) scale from 0.0 (red) to 40.0-mm (blue) depth values and exported as polygon (PLY) file format models with tissue depth values saved in the "vertex quality" field. FTDMs were also split into 1.0-mm increments to facilitate viewing of common depths across all faces. In total, 112 FTDMs were generated for 106 individuals. Minimum depth values ranged from 1.2 mm to 3.4 mm, indicating a common range of starting depths for most faces regardless of weight, as well as common locations for these values over the nasal bones, lateral orbital margins, and forehead superior to the supraorbital border. Maximum depths were found in the buccal region and neck, excluding the nose. Individuals with multiple scans at visibly different weights presented the greatest differences within larger depth areas such as the cheeks and neck, with little to no difference in the thinnest areas. A few individuals with minimum tissue depths at the lateral orbital margins and thicker tissues over the nasal bones (>3.0 mm) suggested the potential influence of nasal bone morphology on tissue depths. This study produced visual quantitative representations of the face and skull for forensic facial approximation research and practice that can be further analyzed or interacted with using free software. The presented tools can be applied to preexisting CT scans, traditional or cone beam, adult or subadult individuals, with or without landmarks, and regardless of head orientation, for forensic applications as well as for studies of facial variation and facial growth. In contrast with other facial mapping studies, this method produced both skull and face points based on replicable geometric relationships, producing multiple data outputs that are easily readable with software that is openly accessible.

Published

2018

19. Flow cytometry dataset for cells collected from touched surfaces

Author

M. Katherine Philpott, Ye Jin Kwon, Cristina Stanciu, and Christopher J. Ehrhardt

Subjects

0301 basic medicine, Multiple days, Allophycocyanin, General Immunology and Microbiology, medicine.diagnostic_test, forensic science, flow cytometry, epithelial cell, Experimental Biophysical Methods, Articles, Genomics, General Medicine, Human leukocyte antigen, Computational biology, Biology, Data Note, General Biochemistry, Genetics and Molecular Biology, Flow cytometry, 03 medical and health sciences, 030104 developmental biology, Physical separation, Immunology, medicine, touch mixtures, General Pharmacology, Toxicology and Pharmaceutics

Abstract

‘Touch’ or trace cell mixtures submitted as evidence are a significant problem for forensic laboratories as they can render resulting genetic profiles difficult or even impossible to interpret. Optical signatures that distinguish epidermal cell populations from different contributors could facilitate the physical separation of mixture components prior to genetic analysis, and potentially the downstream production of single source profiles and/or simplified mixtures. This dataset comprises the results from antibody hybridization surveys using Human Leukocyte Antigen (HLA) and Cytokeratin (CK) probes, as well as surveys of optical properties of deposited cells, including forward scatter (FSC), side scatter (SSC), and fluorescence emissions in the Allophycocyanin (APC) channel. All analyses were performed on “touch” samples deposited by several different contributors on multiple days to assess inter- and intra-contributor variability.

Published

2016

20. Flow cytometry analysis of epithelial cell populations from touch samples using the BD Influx flow cytometry platform

Author

Ye Jin Kwon, Cristina Stanciu, M. Katherine Philpott, and Christopher J. Ehrhardt

Subjects

0301 basic medicine, Allophycocyanin, Multiple days, General Immunology and Microbiology, medicine.diagnostic_test, General Medicine, Biology, Plant biology, General Biochemistry, Genetics and Molecular Biology, Epithelium, Cell biology, Flow cytometry, 03 medical and health sciences, 030104 developmental biology, 0302 clinical medicine, medicine.anatomical_structure, Physical separation, Immunology, medicine, 030216 legal & forensic medicine, General Pharmacology, Toxicology and Pharmaceutics

Abstract

‘Touch’ or trace cell mixtures submitted as evidence are a significant problem for forensic laboratories as they can render resulting genetic profiles difficult or even impossible to interpret. Optical signatures that distinguish epidermal cell populations from different contributors could facilitate the physical separation of mixture components prior to genetic analysis, and potentially the downstream production of single source profiles and/or simplified mixtures. For this dataset, optical properties including forwards scatter (FSC), side scatter (SSC), and fluorescence emissions in the Allophycocyanin (APC) channel were measured in epithelial cell populations from touch samples collected from several different contributors on multiple days to assess inter- and intra-contributor variability.

Published

2016

21. Analysis of red autofluorescence (650-670nm) in epidermal cell populations and its potential for distinguishing contributors to 'touch' biological samples

Author

Eduardo E. Bustamante, Ye Jin Kwon, Christopher J. Ehrhardt, M. Katherine Philpott, and Cristina Stanciu

Subjects

0301 basic medicine, epidermal cell, Touch DNA, forensic science, Cell, Computational biology, autofluorescence, Biology, Intrinsic fluorescence, General Biochemistry, Genetics and Molecular Biology, 030207 dermatology & venereal diseases, 03 medical and health sciences, 0302 clinical medicine, medicine, General Pharmacology, Toxicology and Pharmaceutics, General Immunology and Microbiology, flow cytometry, touch DNA, Experimental Biophysical Methods, Articles, Genomics, General Medicine, Plant biology, DNA extraction, mixture, Research Note, Autofluorescence, 030104 developmental biology, medicine.anatomical_structure, Immunology

Abstract

Interpretation of touch DNA mixtures poses a significant challenge for forensic caseworking laboratories. Front end techniques that facilitate separation of contributor cell populations before DNA extraction are a way to circumvent this problem. The goal of this study was to survey intrinsic fluorescence of epidermal cells collected from touch surfaces and investigate whether this property could potentially be used to discriminate between contributor cell populations in a biological mixture. Analysis of red autofluorescence (650-670nm) showed that some contributors could be distinguished on this basis. Variation was also observed between autofluorescence profiles of epidermal cell populations from a single contributor sampled on different days. This dataset suggests that red autofluorescence may be a useful marker for identifying distinct cell populations in some mixtures. Future efforts should continue to investigate the extrinsic or intrinsic factors contributing to this signature, and to identify additional biomarkers that could complement this system.

Published

2016

22. Integration of gas chromatography mass spectrometry methods for differentiating ricin preparation methods

Author

Jon H. Wahl, Kathryn C. Antolick, Karen L. Wahl, Christopher J. Ehrhardt, Heather A. Colburn, Kristin D. Victry, David S. Wunschel, and Angela M. Melville

Subjects

Ricinoleic acid, Ricin, medicine.disease_cause, Mass spectrometry, Biochemistry, Gas Chromatography-Mass Spectrometry, Analytical Chemistry, Acetone, chemistry.chemical_compound, Electrochemistry, medicine, Environmental Chemistry, Spectroscopy, Chromatography, biology, Toxin, Chemistry, Ricinus, Monosaccharides, Analytic Sample Preparation Methods, Hydrogen-Ion Concentration, biology.organism_classification, Systems Integration, Castor oil, Multivariate Analysis, Seeds, Gas chromatography, Gas chromatography–mass spectrometry, Ricinoleic Acids, medicine.drug

Abstract

The investigation of crimes involving chemical or biological agents is infrequent, but presents unique analytical challenges. The protein toxin ricin is encountered more frequently than other agents and is found in the seeds of Ricinus communis, commonly known as the castor plant. Typically, the toxin is extracted from castor seeds utilizing a variety of different recipes that result in varying purity of the toxin. Moreover, these various purification steps can also leave or differentially remove a variety of exogenous and endogenous residual components with the toxin that may indicate the type and number of purification steps involved. We have applied three gas chromatography – mass spectrometry (GC-MS) based analytical methods to measure the variation in seed carbohydrates and castor oil ricinoleic acid, as well as the presence of solvents used for purification. These methods were applied to the same samples prepared using four previously identified toxin preparation methods, starting from four varieties of castor seeds. The individual data sets for seed carbohydrate profiles, ricinoleic acid, or acetone amount each provided information capable of differentiating different types of toxin preparations across seed types. However, the integration of the data sets using multivariate factor analysis provided a clear distinction of all samples based on the preparation method, independent of the seed source. In particular, the abundance of mannose, arabinose, fucose, ricinoleic acid, and acetone were shown to be important differentiating factors. These complementary tools provide a more confident determination of the method of toxin preparation than would be possible using a single analytical method.

Published

2012

23. Single cell profiling of surface carbohydrates on Bacillus cereus

Author

Congzhou Wang, Vamsi K. Yadavalli, and Christopher J. Ehrhardt

Subjects

In situ, Cell, Biomedical Engineering, Biophysics, Bacillus cereus, Mannose, Bioengineering, Microscopy, Atomic Force, Biochemistry, Biomaterials, chemistry.chemical_compound, medicine, Research Articles, Spores, Bacterial, biology, Polysaccharides, Bacterial, Lectin, Carbohydrate, biology.organism_classification, medicine.anatomical_structure, Cereus, chemistry, biology.protein, Intracellular, Biotechnology

Abstract

Cell surface carbohydrates are important to various bacterial activities and functions. It is well known that different types of Bacillus display heterogeneity of surface carbohydrate compositions, but detection of their presence, quantitation and estimation of variation at the single cell level have not been previously solved. Here, using atomic force microscopy (AFM)-based recognition force mapping coupled with lectin probes, the specific carbohydrate distributions of N -acetylglucosamine and mannose/glucose were detected, mapped and quantified on single B. cereus surfaces at the nanoscale across the entire cell. Further, the changes of the surface carbohydrate compositions from the vegetative cell to spore were shown. These results demonstrate AFM-based ‘recognition force mapping’ as a versatile platform to quantitatively detect and spatially map key bacterial surface biomarkers (such as carbohydrate compositions), and monitor in situ changes in surface biochemical properties during intracellular activities at the single cell level.

Published

2015

24. Forward-scatter and side-scatter dataset for epithelial cells from touch samples analyzed by flow cytometry

Author

Ye Jin Kwon, Christopher J. Ehrhardt, and Cristina Stanciu

Subjects

Pathology, medicine.medical_specialty, Forward scatter, Touch DNA, Sample (material), Epithelial cells, lcsh:Computer applications to medicine. Medical informatics, 01 natural sciences, Standard deviation, Flow cytometry, 03 medical and health sciences, 0302 clinical medicine, medicine, 030216 legal & forensic medicine, lcsh:Science (General), Data Article, Multidisciplinary, medicine.diagnostic_test, integumentary system, Chemistry, 010401 analytical chemistry, Biological materials, 0104 chemical sciences, lcsh:R858-859.7, Forensic science, Biomedical engineering, lcsh:Q1-390

Abstract

‘Touch’ or trace biological samples submitted to caseworking labs as evidence often contain biological material from multiple individuals which can result in mixed DNA profiles. These mixture profiles are difficult to interpret and may cause analytical bottlenecks for forensic laboratories. The data in this brief reports the variation in the relative abundance of intact epithelial cells deposited by four different donors across nine days. Touch samples were generated each day by rubbing a polypropylene tube with both hands for five minutes. Forward-scatter area (FSC-A) and side-scatter area (SSC-A) data was acquired with the BD FACSCanto™ II Analyzer. The relative abundance of different sub-populations within the FSC-A and SSC-A plots was calculated against the total number of events analyzed in each sample. Mean and standard deviation values were calculated for each donor. Keywords: Flow cytometry, Forensic science, Epithelial cells, Touch DNA

25. Preliminary assessment of three quantitative approaches for estimating time-since-deposition from autofluorescence and morphological profiles of cell populations from forensic biological samples.

Author

Amanda Elswick Gentry, Sarah Ingram, M Katherine Philpott, Kellie J Archer, and Christopher J Ehrhardt

Subjects

Medicine, Science

Abstract

Determining when DNA recovered from a crime scene transferred from its biological source, i.e., a sample's 'time-since-deposition' (TSD), can provide critical context for biological evidence. Yet, there remains no analytical techniques for TSD that are validated for forensic casework. In this study, we investigate whether morphological and autofluorescence measurements of forensically-relevant cell populations generated with Imaging Flow Cytometry (IFC) can be used to predict the TSD of 'touch' or trace biological samples. To this end, three different prediction frameworks for estimating the number of day(s) for TSD were evaluated: the elastic net, gradient boosting machines (GBM), and generalized linear mixed model (GLMM) LASSO. Additionally, we transformed these continuous predictions into a series of binary classifiers to evaluate the potential utility for forensic casework. Results showed that GBM and GLMM-LASSO showed the highest accuracy, with mean absolute error estimates in a hold-out test set of 29 and 21 days, respectively. Binary classifiers for these models correctly binned 94-96% and 98-99% of the age estimates as over/under 7 or 180 days, respectively. This suggests that predicted TSD using IFC measurements coupled to one or, possibly, a combination binary classification decision rules, may provide probative information for trace biological samples encountered during forensic casework.

Published

2023