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1. Evaluation of a specialized filter-paper matrix for transportation of extended bovine semen to screen for bovine herpesvirus-1 by real-time PCR.

Author

Sarangi LN, Naveena T, Rana SK, Surendra KSNL, Reddy RVC, Bajibabu P, Ponnanna NM, Sharma GK, and Srinivasan VA

Subjects
Animals, Cattle, Cattle Diseases virology, DNA, Viral analysis, DNA, Viral genetics, Herpesviridae Infections diagnosis, Herpesviridae Infections virology, Herpesvirus 1, Bovine genetics, India, Molecular Diagnostic Techniques methods, Sensitivity and Specificity, Temperature, Time Factors, Cattle Diseases diagnosis, Herpesviridae Infections veterinary, Herpesvirus 1, Bovine isolation & purification, Paper, Real-Time Polymerase Chain Reaction methods, Semen virology, Specimen Handling methods
Abstract

The extended frozen semen (EFS) batches produced from infectious bovine rhinotracheitis (IBR) sero-positive cattle and buffalo bulls housed in various semen stations in India are transported to the testing laboratory in liquid nitrogen (LN 2 ) for screening bovine herpesvirus-1 (BoHV-1). This procedure is laborious and poses LN 2 related hazards. An alternative logistics for transportation of samples was investigated. Use of Flinders Technology Associates (FTA ® ) elute card was evaluated for transportation of extended bovine semen to screen BoHV-1 DNA by real-time PCR targeting gB gene and the method was compared with the OIE approved Chelex resin based method. A protocol for extraction of BoHV-1 DNA from FTA ® card spotted with extended semen was optimized. The viral DNA was found to be stable on FTA ® card for at least 28 days when the cards are stored at 4°-37 °C. The analytical sensitivity for the assay was determined using variable dilutions of BoHV-1 spiked semen and positive plasmid harbouring gB gene (97bp) spotted onto FTA ® card and it was found to be 10 0.8 TCID 50 /ml or 100 copies respectively in real-time PCR. The test could detect as low as 10 0.008 TCID 50 /ml or 1 copy of positive plasmid when more number of replicates (n = 6) of the same sample were tested. This sensitivity was found to be comparable to Chelex method and both the methods demonstrated a very strong correlation (r = 0.9774; 95% CI: 0.9620-0.9860) in terms of Ct value (p < 0.0001). The diagnostic sensitivity and specificity of the FTA method in comparison to the Chelex method was 83.08% (95% CI: 71.73%-91.24%) and 93.23% (95% CI: 89.38%-96.01%) respectively when 316 samples were screened by both the methods. The degree of agreement between these two tests was good (Kappa value: 0.738; 95% CI: 0.646-0.829). The method was found to be robust and highly repeatable in inter-assay and intra-assay precision testing. The result suggests that the FTA ® card holds promise as an alternative system for transportation of EFS for downstream screening of BoHV-1 DNA., (Copyright © 2018 Elsevier B.V. All rights reserved.)

Published
2018
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2. Rapid Veterinary Diagnosis of Bovine Reproductive Infectious Diseases from Semen Using Paper-Origami DNA Microfluidics.

Author

Yang Z, Xu G, Reboud J, Ali SA, Kaur G, McGiven J, Boby N, Gupta PK, Chaudhuri P, and Cooper JM

Subjects
Animals, Brucella abortus isolation & purification, Brucellosis, Bovine microbiology, Cattle, Herpesviridae Infections veterinary, Herpesviridae Infections virology, Herpesvirus 1, Bovine isolation & purification, Leptospira isolation & purification, Leptospirosis microbiology, Leptospirosis veterinary, Limit of Detection, Molecular Diagnostic Techniques instrumentation, Molecular Diagnostic Techniques methods, Paper, Cattle Diseases microbiology, Cattle Diseases virology, DNA, Bacterial chemistry, DNA, Viral chemistry, Microfluidics instrumentation, Microfluidics methods, Molecular Diagnostic Techniques veterinary, Semen microbiology, Semen virology
Abstract

The health and well-being of cattle is an important issue in maintaining and increasing global agricultural output. In dairy production within low and middle income countries (LMICs), there is a significant biosensing challenge in detecting sexually transmitted infection (STI) pathogens during animal husbandry, due in part to difficulties associated with the limited infrastructure for veterinary medicine. Here we demonstrate low-cost, multiplexed, and sample-to-answer paper-origami tests for the detection of three bovine infectious reproductive diseases in semen samples, collected at a test site in rural India. Pathogen DNA from one viral pathogen, bovine herpes virus-1 (BoHV-1), and two bacteria (Brucella and Leptospira) was extracted, amplified (using loop-mediated isothermal amplification, LAMP), and detected fluorescently, enabling <1 pg (∼ from 115 to 274 copies per reaction) of target genomic DNA to be measured. Data was collected as a fluorescence signal either visually, using a low-cost hand-held torch, or digitally with a mobile-phone camera. Limits of detection and sensitivities of the paper-origami device for the three pathogens were also evaluated using pathogen-inoculated semen samples and were as few as 50 Leptospira organisms, 50 CFU Brucella, and 1 TCID 50 BoHV-1. Semen samples from elite bulls at a germplasm center were also tested in double-blind tests, as a demonstrator for a low-cost, user-friendly point-of-care sensing platform, for in-the-field resource-limited regions. The sensors showed excellent levels of sensitivity and specificity, and for the first time a demonstrated ability of the application of paper microfluidics devices for the diagnosis multiple infectious diseases from semen samples.

Published
2018
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3. The fallacy of the two-minute acid phosphatase cut off.

Author

Lewis J, Jones S, Baxter F, Siemieniuk A, and Talbot R

Subjects
DNA Fingerprinting methods, Humans, Male, Time Factors, Acid Phosphatase analysis, Clinical Enzyme Tests methods, Paper, Semen enzymology
Abstract

Research was carried out to determine whether the likelihood of obtaining a positive Acid Phosphatase (AP) test result is affected by the make and type of paper used. Also, we aimed to investigate the frequency of AP positive reactions occurring after 2min using a series of known semen dilutions and to determine whether spermatozoa transfer onto the paper during the act of AP screening. In this research, most brands of paper tested were able to detect a 1 in 40 semen dilution within 2min. Leaving AP test papers for longer will allow the detection of greater dilutions of semen and as the amount of ejaculation is not reliably known in most casework situations and levels of AP activity can vary in different men, this will increase the seminal detection rate in sexual offence allegations., (Copyright © 2011. Published by Elsevier Ireland Ltd.)

Published
2012
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4. Acid phosphatase screening - wetting test paper or wetting fabric and test paper?

Author

Davidson G and Jalowiecki TB

Subjects
DNA Fingerprinting methods, Humans, Male, Time Factors, Acid Phosphatase analysis, Clinical Enzyme Tests methods, Paper, Semen enzymology, Textiles
Abstract

Detecting and locating semen stains is addressed by identifying the associated acid phosphatase activity of semen. The recovery of semen stains is critical as it can, via DNA testing, address the possible source(s) of the semen and may aid in the interpretation of a case. The purpose of these experiments, carried out on behalf of the Body Fluids Forum, was to consider whether wetting the test paper alone or wetting the semen stained fabric and the test paper affected the detection and location of the semen stains on various fabric types, or the subsequent recovery of spermatozoa from these fabrics. It became evident that the preferred approach varied depending on the fabric type being tested but that more often than not, wetting both the fabric and the test paper had a detrimental effect on the recovery of spermatozoa., (Copyright © 2011. Published by Elsevier Ireland Ltd.)

Published
2012
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5. [The demonstration of seminal fluid stains on paper. II. The treatment of laboratory studies dealing with rape].

Author

Celli R and Fazio Pellacchio MC

Subjects
Female, Humans, Male, Spermatozoa cytology, Staining and Labeling methods, Paper, Rape, Semen cytology
Abstract

The authors suggest the use of Baecchi's staining for the morphological demonstration of spermatozoa on paper tissues. They affirm that the method suggested allows good results to be obtained even using material abandoned at the site of sexual aggression.

Published
1994

11. [Recent results of biochemical studies of human sperm plasma].

Author

Schirren C

Subjects
Androgens administration & dosage, Biochemical Phenomena, Biochemistry, Chromatography, Gas, Dehydroepiandrosterone analysis, Dexamethasone pharmacology, Electrophoresis, Estrogens analysis, Fructose analysis, Gonadotropins pharmacology, Humans, Immunoelectrophoresis, Lactates analysis, Leydig Cells metabolism, Male, Paper, Proteins analysis, Pyruvates analysis, Testicular Diseases drug therapy, Testicular Diseases metabolism, Ultracentrifugation, Semen analysis
Published
1968

12. Developmental Validation of the ANDE 6C System for Rapid DNA Analysis of Forensic Casework and DVI Samples

Author

Rosemary S. Turingan, Yeshwanthi Estari, Greice Krautz-Peterson, Hua Jiang, Jessi Brown, Eugene Tan, and Richard F. Selden

Subjects
Male, Computer science, I‐Chip, computer.software_genre, 01 natural sciences, Polymerase Chain Reaction, FlexPlex assay, Identification system, Chewing Gum, 0302 clinical medicine, Rapid dna, Limit of Detection, developmental validation, disaster victim identification, Quality Assurance Standards, Papers, Microsatellite, Female, Data mining, Databases, Nucleic Acid, Paper, Concordance, short tandem repeat, ANDE, Bone and Bones, Pathology and Forensic Medicine, Specimen Handling, 03 medical and health sciences, Species Specificity, Semen, Genetics, Humans, 030216 legal & forensic medicine, Expert System, Saliva, Alleles, business.industry, 010401 analytical chemistry, Mouth Mucosa, Reproducibility of Results, Disaster victim identification, Rapid DNA Identification, DNA, DNA analysis/testing, DNA Fingerprinting, Expert system, 0104 chemical sciences, Forensic science, Disaster Victims, business, Quality assurance, computer, Tooth, Criminalistics, Blood Chemical Analysis, Microsatellite Repeats
Abstract

A developmental validation was performed to demonstrate reliability, reproducibility, and robustness of the ANDE Rapid DNA Identification System for processing of crime scene and disaster victim identification (DVI) samples. A total of 1705 samples were evaluated, including blood, oral epithelial samples from drinking containers, samples on FTA and untreated paper, semen, bone, and soft tissues. This study was conducted to address the FBI’s Quality Assurance Standards on developmental validation and to accumulate data from a sufficient number of unique donors and sample types to meet NDIS submission requirements for acceptance of the ANDE Expert System for casework use. To date, no Expert System has been approved for such samples, but the results of this study demonstrated that the automated Expert System performs similarly to conventional laboratory data analysis. Furthermore, Rapid DNA analysis demonstrated accuracy, precision, resolution, concordance, and reproducibility that were comparable to conventional processing along with appropriate species specificity, limit of detection, performance in the presence of inhibitors. No lane‐to‐lane or run‐to‐run contamination was observed, and the system correctly identified the presence of mixtures. Taken together, the ANDE instrument, I‐Chip consumable, FlexPlex chemistry (a 27‐locus STR assay compatible with all widely used global loci, including the CODIS core 20 loci), and automated Expert System successfully processed and interpreted more than 1200 unique samples with over 99.99% concordant CODIS alleles. This extensive developmental validation data provides support for broad use of the system by agencies and accredited forensic laboratories in single‐source suspect‐evidence comparisons, local database searches, and DVI.

Published
2020

13. The Differentiation of Menstrual from Venous Blood and Other Body Fluids on Various Substrates Using ATR FT-IR Spectroscopy

Author

Alicia A. Quinn and Kelly M. Elkins

Subjects
Male, Paper, Saliva, Pathology, medicine.medical_specialty, Semen, 01 natural sciences, Stain, Pathology and Forensic Medicine, 03 medical and health sciences, 0302 clinical medicine, Spectroscopy, Fourier Transform Infrared, Genetics, medicine, Humans, Cotton Fiber, 030216 legal & forensic medicine, Ftir atr, Menstrual blood, Body fluid, Chromatography, Fluid composition, Milk, Human, Chemistry, Forensic Sciences, 010401 analytical chemistry, Venous blood, Wood, Menstruation, 0104 chemical sciences, Nylons, Female, Glass, Blood Chemical Analysis
Abstract

Crime scene investigators and laboratory analysts use chemical tests to detect and differentiate body fluids. Testing often requires a sample of the stain, and the chemicals may cause degradation of the fluid or interfere with subsequent tests. Colorimetric chemical tests do not differentiate between different types of the same fluid, such as venous and menstrual blood, and there is no presumptive test available to simultaneously differentiate several body fluids. In this study, we recorded ATR FT-IR spectra of venous and menstrual blood, semen, saliva, and breastmilk. Neat and simulated casework body fluid samples were analyzed on cotton, nylon, wood, paper, and glass substrates. Differences in fluid composition, including proteins and small molecules, resulted in spectral differences. Venous and menstrual blood is differentiated by the peak at 1039 cm−1 attributed to phosphoric acid found in menstrual blood. Peak intensity is influenced by the porosity and weave of the substrate fabric.

Published
2016
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14. Direct DNA Analysis with Paper-Based Ion Concentration Polarization

Author

David Sinton, Reza Nosrati, Max M. Gong, Maria San Gabriel, and Armand Zini

Subjects
Male, Paper, Hepatitis B virus, Surface Properties, 02 engineering and technology, medicine.disease_cause, 01 natural sciences, Biochemistry, Catalysis, chemistry.chemical_compound, Colloid and Surface Chemistry, Semen, medicine, Humans, Particle Size, Detection limit, Chromatography, Chemistry, 010401 analytical chemistry, DNA, General Chemistry, Hepatitis B, 021001 nanoscience & nanotechnology, Molecular diagnostics, Spermatozoa, Molecular biology, Sperm, Nanostructures, 3. Good health, 0104 chemical sciences, Chromatin, DNA, Viral, DNA fragmentation, 0210 nano-technology, Porosity, Viral load
Abstract

DNA analysis is essential for diagnosis and monitoring of many diseases. Conventional DNA testing is generally limited to the laboratory. Increasing access to relevant technologies can improve patient care and outcomes in both developed and developing regions. Here, we demonstrate direct DNA analysis in paper-based devices, uniquely enabled by ion concentration polarization at the interface of patterned nanoporous membranes in paper (paper-based ICP). Hepatitis B virus DNA targets in human serum are simultaneously preconcentrated, separated, and detected in a single 10 min operation. A limit of detection of 150 copies/mL is achieved without prior viral load amplification, sufficient for early diagnosis of hepatitis B. We clinically assess the DNA integrity of sperm cells in raw human semen samples. The percent DNA fragmentation results from the paper-based ICP devices strongly correlate (R(2) = 0.98) with the sperm chromatin structure assay. In all cases, agreement was 100% with respect to the clinical decision. Paper-based ICP can provide inexpensive and accessible advanced molecular diagnostics.

Published
2015
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15. Extraction platform evaluations: A comparison of Automate Express™, EZ1® Advanced XL, and Maxwell® 16 Bench-top DNA extraction systems

Author

Carey Davis, Jonathan L. King, Bruce Budowle, Meredith Turnbough, and Arthur J. Eisenberg

Subjects
Male, Paper, Pcr assay, Polymerase Chain Reaction, Bone and Bones, Pathology and Forensic Medicine, Semen, Humans, Sample Type, Saliva, Alleles, Residue (complex analysis), Chromatography, Elution, Chemistry, Textiles, Extraction (chemistry), Epithelial Cells, DNA, DNA Fingerprinting, DNA extraction, Issues, ethics and legal aspects, Blood, Hair root, Cigarette butt, Tooth, Hair
Abstract

The DNA extraction performance of three low-throughput extraction systems was evaluated. The instruments and respective chemistries all use a similar extraction methodology that involves binding DNA to a coated magnetic resin in the presence of chaotropic salt, washing of the resin to remove undesirable compounds, and elution of DNA from the particles in a low-salt solution. The AutoMate Express™ (Life Technologies Corporation, Carlsbad, CA), EZ1® Advanced XL (Qiagen Inc., Valencia, CA), and Maxwell® 16 (Promega Corporation, Madison, WI) were compared using a variety of samples including: blood on swabs, blood on denim, blood on cotton, blood mixed with inhibitors (a mixture of indigo, hematin, humic acid, and urban dust) on cotton, blood on FTA® paper, saliva residue on cigarette butt paper, epithelial cells on cotton swabs, neat semen on cotton, hair roots, bones, and teeth. Each instrument had a recommended pre-processing protocol for each sample type, and these protocols were followed strictly to reduce user bias. All extractions were performed in triplicate for each sample type. The three instruments were compared on the basis of quantity of DNA recovered (as determined by real-time PCR), relative level of inhibitors present in the extract (shown as shifts in the C T value for the internal PCR control in the real-time PCR assay), STR peak heights, use of consumables not included in the extraction kits, ease of use, and application flexibility. All three systems performed well; however extraction efficiency varied by sample type and with the preprocessing protocol applied to the various samples.

Published
2012
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16. Investigative strategy for the forensic detection of sperm traces

Author

Christin Gruber, Frank Heidorn, Manfred Riße, Marcel A. Verhoff, Reinhard B. Dettmeyer, Heidrun Evers, and Gabriele Lasczkowski

Subjects
Male, Paper, medicine.medical_specialty, Acid Phosphatase, Acid phosphatase test, Anal Canal, Physiology, Genitalia, Male, Pathology and Forensic Medicine, Semen, Skin surface, medicine, Humans, Sex organ, Crime Victims, Retrospective Studies, Skin, Sexual assault, Microscopy, Mouth, Staining and Labeling, business.industry, Textiles, DNA, Genitalia, Female, General Medicine, Forensic Medicine, Female victim, Anus, DNA Fingerprinting, Spermatozoa, Sperm, humanities, Surgery, Forensic science, medicine.anatomical_structure, Tandem Repeat Sequences, Rape, Female, business
Abstract

In a retrospective study, the results from 786 samples of alleged sexual assaults during a 5-year period were evaluated. Of the samples, 758 were from female victims and 28 were from male victims. The material examined during this 5-year period consisted of 561 cotton swabs with swabs taken from the genitals, mouth, anus, or skin surface. In addition, textile products were examined 191 times, paper products 23 times, and other evidentiary materials 11 times. The acid phosphatase (acP) test was performed as a preliminary test for all samples, followed by microscopy after Baecchi staining. DNA analysis was performed on 74 samples following individual court orders. The retrospectively evaluated results from this period indicate that additional tests for the detection of sperm on textiles and paper products are dispensable after a negative acP test. This is different for genital swabs, since sperm could be found microscopically in 3% of cases with a negative acP test, and DNA analysis was also successful. However, an individual investigative strategy has to be determined for each case, as, depending on the structure of the case, the evidence of male DNA on a female victim, or on her clothes, for instance, can also have evidentiary value without microscopic proof for sperm.

Published
2009
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17. Paper-Based Quantification of Male Fertility Potential

Author

David Sinton, Maria San Gabriel, Armand Zini, Max M. Gong, Claudio E. Pedraza, and Reza Nosrati

Subjects
Infertility, Male, Paper, Clinical Biochemistry, Motility, Semen, 02 engineering and technology, Semen analysis, Biology, 01 natural sciences, Andrology, chemistry.chemical_compound, Limit of Detection, Lab-On-A-Chip Devices, medicine, Humans, Sperm motility, Infertility, Male, medicine.diagnostic_test, 010401 analytical chemistry, Biochemistry (medical), 021001 nanoscience & nanotechnology, medicine.disease, Sperm, 0104 chemical sciences, Semen Analysis, chemistry, Male fertility, Colorimetry, Formazan, 0210 nano-technology
Abstract

BACKGROUND More than 70 million couples worldwide are affected by infertility, with male-factor infertility accounting for about half of the cases. Semen analysis is critical for determining male fertility potential, but conventional testing is costly and complex. Here, we demonstrate a paper-based microfluidic approach to quantify male fertility potential, simultaneously measuring 3 critical semen parameters in 10 min: live and motile sperm concentrations and sperm motility. METHODS The device measures the colorimetric change of yellow tetrazolium dye to purple formazan by the diaphorase flavoprotein enzyme present in metabolically active human sperm to quantify live and motile sperm concentration. Sperm motility was determined as the ratio of motile to live sperm. We assessed the performance of the device by use of clinical semen samples, in parallel with standard clinical approaches. RESULTS Detection limits of 8.46 and 15.18 million/mL were achieved for live and motile sperm concentrations, respectively. The live and motile sperm concentrations and motility values from our device correlated with those of the standard clinical approaches (R2 ≥ 0.84). In all cases, our device provided 100% agreement in terms of clinical outcome. The device was also robust and could tolerate conditions of high absolute humidity (22.8 g/m3) up to 16 weeks when packaged with desiccant. CONCLUSIONS Our device outperforms existing commercial paper-based assays by quantitatively measuring live and motile sperm concentrations and motility, in only 10 min. This approach is applicable to current clinical practices as well as self-diagnostic applications.

Published
2015

18. The use of acid phosphatase test papers for DNA profiling

Author

Paul Brauner, Mark Barash, Ayeleth Reshef, Nira Gallili, and A Michael

Subjects
Male, Paper, Time Factors, Adolescent, Acid Phosphatase, Semen, Pathology and Forensic Medicine, law.invention, Silver stain, chemistry.chemical_compound, law, Humans, Polymerase chain reaction, biology, Acid phosphatase, Clinical Enzyme Tests, Forensic Medicine, DNA Fingerprinting, Sperm, Molecular biology, DNA profiling, Biochemistry, chemistry, Tandem Repeat Sequences, biology.protein, Microsatellite, DNA
Abstract

The acid phosphatase (AP) test is a routine assay used to screen casework items for the possible presence of semen. This colour test is carried out on filter paper which is retained after testing. Two-year-old AP test papers were found to contain sufficient DNA for short tandem repeat (STR) profiling. Prior to polymerase chain reaction (PCR) amplification, the DNA was preferentially separated into sperm depleted and sperm enriched cell fractions. The implication of these findings for past and present cases is discussed.

Published
2005
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19. [The demonstration of seminal fluid stains on paper. II. The treatment of laboratory studies dealing with rape]

Author

R, Celli and M C, Fazio Pellacchio

Subjects
Male, Paper, Staining and Labeling, Semen, Rape, Humans, Female, Spermatozoa
Abstract

The authors suggest the use of Baecchi's staining for the morphological demonstration of spermatozoa on paper tissues. They affirm that the method suggested allows good results to be obtained even using material abandoned at the site of sexual aggression.

Published
1994

23. [Recent results of biochemical studies of human sperm plasma]

Author

C, Schirren

Subjects
Electrophoresis, Male, Paper, Chromatography, Gas, Biochemical Phenomena, Leydig Cells, Proteins, Estrogens, Dehydroepiandrosterone, Fructose, Biochemistry, Testicular Diseases, Dexamethasone, Semen, Androgens, Lactates, Humans, Pyruvates, Immunoelectrophoresis, Ultracentrifugation, Gonadotropins
Published
1968